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- protein kinase (1)
- protein quantification (1)
- proteolysis (1)
- proteolytic activation (1)
- proteome (1)
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- proteomics (1)
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- regulatory network (1)
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- virion morphogenesis (1)
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Institute
- Abteilung für Mikrobiologie und Molekularbiologie (155) (remove)
Responses of bovine and human neutrophils to members of the Mycobacterium tuberculosis complex
(2023)
PMN are one of the most important cells of the innate immune system and are responsible for fast clearance of invading pathogens in most circumstances. The role of human PMN during mycobacterial infection have been widely studied. Nevertheless, there are contradicting results regarding their role in protection or pathology during TB. Similar studies focusing on bovine PMN and their role in M. bovis infection remain understudied. Also, not much is known about attenuation of M. tb in cattle and responses of PMN to this MTBC member.
The major aims of this study were to i) gain insights into bovine PMN biology and the cellular processes triggered by challenge with virulent mycobacteria and to ii) find out whether interspecies differences result in different outcomes upon in vitro challenge. In the first part of the work, a new isolation method for bovine PMN from whole blood was developed. Human and bovine PMN have different buoyant properties and hence need to be isolated using different procedures. The magnetic isolation method developed within this thesis is robust and results in very good yields of highly pure, viable bovine PMN populations. This is extremely advantageous and indispensable for downstream functional assays that are required to be performed on a single day.
The second goal of this study was to compare and contrast the functional differences between bovine and human PMN upon BCG infection. The findings reveal for the first time that human PMN phagocytose more BCG in comparison to bovine counterparts. Non-opsonized bacteria were internalized via the lectin-like C-domain, require cholesterol and an active cytoskeleton in human PMN, whereas opsonized bacteria entered cells via the CR3 and, in particular, CD11b. It remains unresolved why bovine PMN reacted differently, notably phagocytosis remained unaltered, to various treatments, including blocking monoclonal antibodies to CD11b and chemical inhibitors altering the cell membrane. Nonetheless, the increased uptake of BCG by human PMN correlates to more potent response of these cells in functional assays in comparison to bovine PMN. No PMN intrinsic differences were found in the basal cholesterol content. Comparative assays with the virulent strains would be essential in order to generalize these observations.
The third aim was to investigate the responses of bovine PMN to BCG, M. tb and M. bovis. While there was no difference in uptake between BCG and M. tb, serum opsonized BCG was taken up at a higher amount. This finding suggests differential binding of bacterial epitopes to host cell receptors which modulates mycobacteria uptake. However, between the virulent strains M. tb and M. bovis, the human-adapted bacillus was phagocytosed at a higher rate which hints towards the possibility of rapid recognition and clearance of M. tb in bovine host thereby possibly preventing pathology. The release of selective cytokines by PMN post infection with the virulent strains offers baseline information relevant for processes that probably occur in vivo. This work for the first time provides insights into responses of bovine PMN to mycobacteria in a two-tier approach: by cross-species analysis of PMN responses to selected mycobacterium and by head-to-head analysis of bovine PMN to animal-adapted and human-adapted mycobacteria.
As a prospect for future research in bovine PMN biology in the context of mycobacterial infection, it would be highly advantageous to compare the subcellular localization of M. tb and M. bovis in bovine PMN using confocal and/or electron microscopy. This analysis would confer proof on attachment or internalization of mycobacteria by PMN and identify the features of the mycobacteria-containing compartments. Also, in-depth investigations of additional entry pathways for the pathogen in bovine cells would be informative for unlocking downstream cell signaling events. In addition, PMN viability studies will be meaningful particularly in bovine PMN challenged with M. bovis and M. tb, given the impact of death patterns on tissue pathology. Current results and follow up studies will contribute to the understanding of the roles of PMN in controlling elimination or growth of M. bovis and M. tb in cattle.
Das Afrikanische Schweinepestvirus (ASPV) ist ein wirtschaftlich wichtiger und in Haus- und Wildschweinen Hämorrhagie mit hoher Sterblichkeitsrate verursachender viraler Erreger.
1921 erstmals in Kenia beschrieben, breitete sich die ASP seit 2007 auch über den
Kaukasus, ins Baltikum (2014), weiter in europäische und asiatische Länder und seit 2020 in Deutschland aus. Trotz der hohen genetischen Stabilität des Afrikanischen
Schweinepestvirus (ASPV) wurden Genomvarianten identifiziert, bei denen Unterschiede
in der Genexpression von Multigenfamilien (MGF) dominieren. Letztlich divergieren ASPV-Stämme in ihrer Virulenz und verursachen akut-letale bis chronische Verläufe im Schwein. Aufgrund der enormen Komplexität des Virus und seiner vielfältigen
Immunevasionsstrategien sind viele Mechanismen der Virus-Wirts-Interaktion, die zur
Immunpathogenese beitragen, nicht ausreichend verstanden und erschweren somit die
Impfstoffentwicklung. Dabei können virale Subversionsmechanismen der Wirtszelle die
antivirale Immunantwort modulieren und stehen deshalb im Fokus dieser Arbeit. Zur
Charakterisierung und mechanistischen Aufklärung dieser ASPV-spezifischen
Immunsubversionsmechanismen wurden primäre porzine Monozyten von Hausschweinen
mit hochvirulentem (Armenia) und natürlich-attenuiertem (Estonia) ASPV infiziert. Die
Resultate ergaben sowohl stammunabhängige als auch -abhängige Unterschiede in der
Regulation myeloider Oberflächenmarker infizierter Monozyten. Insbesondere
beobachteten wir eine stammunabhängige Suppression des Phagozytose-regulierenden
CD172a und eine stammabhängige Regulation von porzinem MHC I (SLA I). Weitere
Experimente zur Untersuchung der zugrundeliegenden Mechanismen ergaben, dass zwar
beide Stämme die Oberflächenexpression von CD172 unterdrücken, jedoch nur Armenia-,
im Gegensatz zu Estonia-infizierten Monozyten, eine reduzierte Recyclingrate sowie eine Abspaltung (Shedding) von CD172a von der Zelloberfläche zeigten. Dies lässt vermuten, dass die Virus-vermittelte Suppression von CD172a der beiden ASPV-Stämme auf unterschiedlichen Subversionsmechanismen beruht. Reinfektionsexperimente und
molekularbiologische Untersuchungen belegten zudem, dass das abgespaltene
Oberflächen-CD172a der Armenia-infizierten Monozyten mit einer gesteigerten
Infektionsrate einhergeht, dies ist wahrscheinlich das Ergebnis (entweder direkt oder indirekt) einer Komplexbildung zwischen dem virulenten Armenia-Virus und löslichem
CD172a. Im Gegensatz dazu resultierte die Infektion von Monozyten mit Armenia, jedoch nicht mit Estonia, in einem deutlichen Oberflächenverlust von porzinem SLA I, welches für die Antigenpräsentation gegenüber CD8+ T-Zellen essentiell ist. Weitere Versuche zeigten einen Reifungsdefekt von SLA I, der mit dem Abbau funktioneller ER-Strukturen und der Induktion von ER-Stress in Armenia-infizierten Monozyten in Zusammenhang stand. Gleichzeitig wurde eine deutlich reduzierte Überlebensfähigkeit Armenia-infizierter Monozyten beobachtet, die mit einem Verlust mitochondrialer Funktionen und der Bildung von Aggresomen aus fehlgefalteten Proteinen im Zytoplasma einherging. Vertiefende Analysen dazu zeigten einen Caspase-3 aktivierten Zelltodmechanismus und ein infektionsbedingtes, progressives Abschalten der Proteintranslation in Armenia-infizierten Zellen. Um einen möglichen Zusammenhang zwischen den beobachteten
Subversionsmechanismen und der Expression bestimmter viraler MGF-Gene zu finden,
wurden weitere ASPV-Stämme in die Untersuchungen zur CD172a- und SLA I-Oberflächenexpression einbezogen. Ähnlich wie Armenia zeigte sich auch für die Stämme
NHV und OURT88/3 eine deutliche Reduktion der SLA I-Oberflächenlevel, auch wenn diese
in vivo gering-virulent sind. Andererseits zeigte das hochvirulente Benin97/1-Isolat im Gegensatz zu Armenia keine SLA I-Subversion, sondern ähnlich wie nach Estonia-Infektion kaum veränderte SLA I-Level, was vermuten lässt, dass der SLA I Subversionsmechanismus nicht alleinig den Virulenzgrad der ASPV-Stämme bestimmt. Ein direkter Genomvergleich identifizierte verschiedene Mitglieder der MGF110- und MGF505-Gene als möglicherweise beteiligte virale Genkandidaten. Im Gegensatz hierzu ergaben sich keine detektierbaren Unterschiede bei den Analysen zur Oberflächensuppression von CD172a innerhalb der verwendeten Isolate, wie bereits bei Armenia und Estonia Infektion beobachtet. Interessanterweise beobachteten wir dabei das Vorhandensein von MGF110-14 als eine genomische Gemeinsamkeit, die für die generelle Oberflächenreduktion von CD172a, zusätzlich zu anderen Genen, die ein Shedding und die Armenia-spezifische Interaktion bestimmen könnten, verantwortlich sein könnte.
Insgesamt zeigen die Resultate dieser Arbeit erstmals, dass das virulente ASPV Armenia, anders als das attenuierte ASPV Estonia, einen ausgeprägten Funktions- und Vitalitätsverlust in seinen primären Zielzellen (z. B. Monozyten) bewirkt. Die gesteigerte Infektiosität, Induktion von zellulärem Stress und Beeinträchtigung der SLA I-vermittelten Antigenpräsentation werden in infizierten Schweinen eine entscheidende Rolle in der Virus-Verbreitung und der Immunevasion spielen. Zusammenfassend lässt sich sagen, dass die Befunde dieser Arbeit neue und vertiefte Einblicke in die zellulären Mechanismen der SLA I- und CD172a-Subversion im Zusammenhang mit der Immunevasion durch hoch-virulentes ASPV Armenia und attenuiertes ASPV Estonia gibt und zudem wichtig für das bessere Verständnis der ASP-Immunpathogenese sind.
The present study deals with the spread and population genetics of the invasive Asian bush
mosquito Ae. japonicus in Europe and Germany. Since the first detection of Ae. japonicus
in Europe in 2000, the species spread rapidly through Europe, either actively by flying or
passively by human activities. In 2017, four confirmed populations of Ae. japonicus existed
in Europe. The largest population covered western Germany, parts of France, Switzerland,
Liechtenstein, Austria and Italy. The most northern population around Hanover, Germany,
did not spread since 2013. A very small population existed in Belgium and the second largest
population covered parts of Austria, Italy, Slovenia, Croatia and Hungary. By 2019, Ae.
japonicus had established in 15 European countries.
Most of the monitoring programmes in Europe dealing with the distribution and spread of
Ae. japoncus investigate cemeteries for juvenile stages. However, activities are not
harmonised, e.g. regarding numbers of investigated collection sites and declaration of
negative sites, making data comparison between different studies difficult. Therefore,
suggestions for a standardised Ae. japonicus monitoring method have been developed and
provided.
In the present study, 445 individuals of Ae. japonicus originating from five different
European countries were investigated for population genetic analyses by sequencing parts
of the nad4 gene and genotyping seven polymorphic microsatellite loci. In total, 16 different
nad4 haplotypes were identified with haplotype H1 being the most common and widespread
one through all populations.
Within Germany, Ae. japonicus has been spreading immensely over the last decade. Even
though the present results (2017) demonstrate incipient genetic admixture of populations as
compared to previous studies (2012-2015), no complete genetic mixture has taken place yet.
The populations of Ae. japonicus still fall into two genetic clusters, but the genetic diversity
on individual level had increased considerably (from three nad4 haplotypes in 2012 to 12
according to the present thesis). Both additional introductions and mutation are possible
reasons, but determining the origin of the German populations is not possible anymore.
In the years following the invasion of Germany, Ae. japonicus spread to southeastern
Europe. In 2013, it established in Croatia, in 2017 in Bosnia and Herzegovina and in 2018
in Serbia. In the current study, immature stages of Ae. japonicus were found at 19 sites in
Croatia, two sites in Bosnia and Herzegovina and one site in Serbia. The population genetic
analyses indicate at least two independent introductions in that area. Aedes japonicus collected west of Orahovica (Croatia) seemed to be genetically similar to samples previously
investigated from Southeast Germany/Austria and Austria/Slovenia. By contrast, samples
from east of Orahovica, together with those from Serbia and Bosnia and Herzegovina, were
characterised by another genetic make-up, but their origin could not be determined.
In 2021, individuals of Ae. japonicus were detected at two collection sites in the Czech
Republic for the first time: Prachatice close to the Czech-German border and Mikulov on
the Czech-Austrian border. Population genetics and comparison of genetic data showed a
close relationship of the Prachatice samples to a German population, while for Ae. japonicus
from Mikulov close relatives could not be identified.
In the future, the global spread and establishment of invasive mosquitoes through
international trade and travel will increase. Potential vectors, like the Asian bush mosquito
Ae. japonicus, can become a problem in Europe and Germany, especially in the course of
global warming which supports pathogen transmission. Monitoring the known populations
and identifying introduction and migration routes are therefore essential for vector
managing.
Posttranslational modifications are involved in the regulation of virtually all cellular processes, including immune response, nevertheless, they are also targets manipulated by invading pathogens. The first investigated example is protein citrullination which is an important posttranslational modification that acts on a multitude of processes like supervision of cell pluripotency and rheumatoid arthritis. Citrullination of targeted arginine residues is performed by the Peptidylarginine deiminase. Within the first published manuscript, being part of this thesis, it was possible to show the use of this posttranslational modification by the human pathogen Porphyromonas gingivalis to facilitate innate immune evasion at three distinct level. P. gingivalis was demonstrated to citrullinate proteins by Porphyromonas peptidylarginine deiminase resulting in diminished phagocytosis and subsequent killing by neutrophils. Furthermore, it was shown that citrullination of histone H3 enables P. gingivalis to survive in neutrophil extracellular traps and incapacitate the lysozyme-derived peptide LP9.
The second investigated posttranslational modification is ubiquitination and its role in respiratory tract infections. Ubiquitination is the covalent attachment of a small protein that consisting of only 76 amino acids to the ε-amino group of lysine residues to posttranslational modify proteins. Acute infections of the lower respiratory tract such as viral and bacterial co-infections are among the most prevalent reasons of fatal casualties worldwide. Therefore, the interactions between host and pathogens resulting in the impairment of the hosts immune response and immune evasion of the pathogens, need to be elucidated. To get new insights in the infection driven changes in protein polyubiquitination and alterations in the abundance of ubiquitin E3 ligases involved in ubiquitination, cellular proteomes were monitored in detail by high resolution mass spectrometry. Therefore, the epithelial cell lines 16HBE14o- (Manuscript II) and A549 (Manuscript III) were co-infected with influenza A virus H1N1 and Streptococcus pyogenes or Staphylococcus aureus or with influenza A virus H1N1 and Streptococcus pneumoniae, respectively. Here, it could be shown in 16HBE14o- cells that co-infection of epithelial cells is not characterized by decreased cell survival and that observable effects on the proteome and ubiquitinome are mostly additive rather than synergistic. S. pyogenes infection affected the mitochondrial function, cell-cell adhesion, endocytosis and actin organization. Viral infection affected mRNA processing and Rho signaling. Viral and bacterial co-infection was detected to affect processes that were already affected by both of the corresponding single infections. No further pathways were strongly affected by the co-infection. A similar result has been observed in A549 cells co-infected IAV and S. pneumoniae. Overrepresented gene ontology terms depict the sum of those observed in the viral and bacterial single infection. Moreover, no significant change in cell survival upon co-infection compared to single bacterial infection was noticed for A549 cells either. This led to the suggestion that co-infection of investigated epithelial cells under examined conditions possesses additive rather than synergistic effect and thus, may not worsen the outcome of the infection within the studied conditions. Infections in other systems, may provide varying results and thus should be examined in future studies.
Until today, more than 100 years after its first description in Italy, the highly pathogenic avian influenza virus (HPAIV) has not lost its fearsome character for wild birds, poultry and humans. On the contrary, the number of outbreaks with high casualty rates in wild birds and poultry has multiplied in recent years and cases of zoonotic infections are also increasingly reported from HPAI endemic areas. The epidemiology of these infections is complex and also involves surface water and possibly sediments of shallow standing waters, which could play a role as a vector medium and/or virus reservoir. The goal of this project was to expand current knowledge of the influence of water on the spread of AIV. As part of this project, we were able to ...
1. ...improve AIV detection methods using real time RT-PCR in terms of sensitivity and breadth of viruses detected. In addition, we succeeded in economizing the procedure so that fewer resources are required and results are obtained faster (publication I: [173]).
2. ...develop an ultrafiltration-based enrichment method for AIV from surface water and evaluate it with field samples from HPAI outbreak areas in wild bird habitats (Wadden Sea coast of Schleswig-Holstein) and previously unaffected regions (Antarctic Weddell Sea) (publication II: [174]). Furthermore, protocols for testing different environmental sample matrices for AIV screening were tested and compared to results of passive monitoring by dabbing diseased or dead wild birds. AIV was detected in more than half (61%) of 44 water samples. We received additional sediment samples from 36 of the 44 water samples. In 18 of 36 of the sediments tested, as well as in 4.16% of 1705 fecal samples tested AIV was detected. However, the studies of the environmental samples mostly yielded only generic AIV detections, with viral loads in the range of the detection limit. This massively hampered further investigations for sub- and pathotyping. In contrast, 79.41% of 68 samples from passive monitoring showed high to very high HPAIV viral loads which also allowed sub- and pathotyping.
3. ...demonstrate in animal experiments that even very low titers (0.1 TCID50 ml-1) of HPAI viral infectivity in water can induce productive infection in susceptible but clinically largely resistant mallard ducks (publication III: [175]). Furthermore, we were able to develop evidence that there is a difference in virus spread that depends on the type of (contaminated) water source. This means that infections on poultry farms with inverted or nipple drinkers may follow a different course than infections in the wild, which are mediated via larger surface waters.
Overall, the results of this project highlight the important role of surface and drinking water, as well as aquatic sediments, in the spread of AIV. The methods developed here for AIV detection extend the possibilities for surveillance of AIV infections; however, passive remains superior to active surveillance of HPAIV infections in several aspects. Examination of various environmental samples did not yield a significant advantage in terms of an early warning system that would indicate the presence or spread of HPAIV in wild bird habitats prior to the occurrence of lethal infections in wild birds.
Methane (CH4) is a potent greenhouse gas with rising atmospheric concentrations.
Microorganisms are essential players in the global methane cycle. In fact, the largest part of methane emissions derives from microbial production by methanogenic Archaea (methanogens). Microorganisms do not only produce methane: methanotrophs can also oxidize the methane produced by methanogens. In addition, soil methanotrophs are the only biological methane sink, oxidizing up to 30-40 Tg of this potent greenhouse gas per year worldwide.
However, intensified management of grasslands and forests may reduce the methane sink capacity of soils.
In general, the interaction of methanogens and methanotrophs determines whether a soil is a source or a sink for methane. It is, therefore, crucial to understand the microbial part of the methane cycle and which factors influence the abundance and activity of methane-cycling microbes. However, capturing the soil microbiome's abundances, activity, and identity is
challenging. There are numerous target molecules and myriad methods, each with certain
limitations. Linking microbial markers to methane fluxes is therefore challenging. This thesis aimed to understand how methane-cycling microbes in the soil are related to soil methane fluxes and how soil characteristics and human activity influence them.
The first publication investigated the biotic and abiotic drivers of the atmospheric methane sink of soils. It assessed the influence of grassland land-use intensity (150 sites) and forest management type (149 sites) on potential atmospheric methane oxidation rates (PMORs) and the abundance and diversity of CH4-oxidizing bacteria (MOB) with qPCR in topsoils of three temperate regions in Germany. PMORs measured in microcosms under defined conditions were approximately twice as high in forest than in grassland soils. High land-use intensity of grasslands negatively affected PMORs (−40%) in almost all regions. Among the different aspects of land-use intensity, fertilization had the most adverse effect reducing PMORs by 20%.
In contrast, forest management did not affect PMORs in forest soils. Upland soil cluster (USC)α was the dominant group of MOBs in the forests. In contrast, USCγ was absent in more than half of the forest soils but present in almost all grassland soils. USCα abundance had a direct positive effect on PMOR in forests, while in grasslands, USCα and USCγ abundance affected PMOR positively with a more pronounced contribution of USCγ than USCα.
In the second publication, we used quantitative metatranscriptomics to link methane-cycling microbiomes to net surface methane fluxes throughout a year in two grassland soils. Methane fluxes were highly dynamic: both soils were net methane sources in autumn and winter and net methane sinks in spring and summer. Correspondingly, methanogen mRNA abundances per
gram soil correlated well with methane fluxes. Methanotroph to methanogen mRNA ratios were higher in spring and summer when the soils acted as net methane sinks. Furthermore, methane uptake was associated with an increased proportion of USCα and γ pmoA and pmoA2 transcripts. High methanotroph to methanogen ratios would indicate methane sink properties.
Our study links the seasonal transcriptional dynamics of methane-cycling soil microbiomes for the first time to gas fluxes in situ. It suggests mRNA transcript abundances as promising indicators of dynamic ecosystem-level processes.
We conclude that reduction in grassland land-use intensity and afforestation can potentially increase the methane sink function of soils and that different parameters determine the microbial methane sink in forest and grassland soils. Furthermore, this thesis suggests mRNA transcript abundances as promising indicators of dynamic ecosystem-level processes. Methanogen transcript abundance may be used as a proxy for changes in net surface methane emissions from grassland soils.
As the animal-to-human interface becomes increasingly narrow, transmission events of zoonotic pathogens between animals and humans become more and more probable. While SARS-CoV-2 already accomplished a spillover infection to humans and is responsible for the current pandemic, the bat H9N2 IAV with so far unknown zoonotic potential was only recently discovered. In order to identify I) the role and potential of a newly discovered, potentially pre-pandemic virus, such as the bat H9N2, or II) possible future prevailing virus mutant variants of an already known pandemic virus, such as SARS-CoV-2, it is important to characterize these emerging viruses in vivo as soon and as good as possible.
The first objective in this dissertation (Publications I and II) therefore deals with the characterization of bat H9N2 and the estimation of its zoonotic or even pandemic potential.
In Publication I, a general susceptibility of directly inoculated Egyptian fruit bats to bat H9N2 was confirmed by successful seroconversion, although exhibiting only moderate viral shedding. All three contact animals remained seronegative, though one contact bat showed slight lesions in the histopathological analysis.
Publication II further addressed the question of the zoonotic potential of this virus. Inoculation of day-old turkey hatchlings demonstrated moderate susceptibility to bat H9N2 infection with a measurable seroconversion, while day-old chicken hatchlings were not susceptible to bat H9N2. Ferrets proved to be highly susceptible to bat H9N2 with high viral shedding, a transmission efficiency rate of 100% to direct contact animals at 2 days post contact, but with only minimal clinical signs. Importantly, the virus demonstrated the ability to evade the MxA-restriction factor and to replicate efficiently in human lung tissue explants. Furthermore, seasonal IAV- and standard IAV-vaccines showed no cross reactivity against the bat-N2 protein in humans. Therefore, further research on such viruses is urgently needed in order to prevent a renewed pandemic situation in the future as caused by SARS-CoV-2.
The second objective in this dissertation dealt with the identification and characterization of emerging SARS-CoV-2 Variants of Concern (VOCs).
Therefore, in Publication III, competitive infection experiments were performed using the Syrian golden hamster, the ferret, and transgenic mouse models (K18-hACE2 and hACE2-KI). These studies revealed replicative and transmissive predominance of Alpha VOC over Beta VOC, but not over SARS-CoV-2 WT in the hamster model, although Beta VOC substantially replicated in the lungs of donor animals. In contrast, the Alpha VOC had an unambiguous replication and transmission advantage over WT SARS-CoV-2 in the ferret and both mouse models. A recombinant SARS-CoV-2 WT-SAlpha virus helped to assign the fitness advantage of this variant particularly to the spike protein-associated mutations.
In Publication IV, in vitro results inferred an early replicative fitness advantage of Omicron BA.1 over Delta VOC, although the opposite was observed in competitively inoculated hamsters, ferrets and naive hACE2-KI mice. In addition, Publication IV demonstrated a disadvantage in transmission for the VOC Omicron BA.1 over the Delta VOC and a lack of susceptibility of ferrets after a single infection with the VOC Omicron BA.1. An mRNA vaccination of K18-hACE2 mice caused a drastic reduction of infectious virus particles in organ material following an infection with a recombinant SARS-CoV-2 WT-SDelta, but not when challenged with the SARS-CoV-2 SOmicron BA.1 clone.
This dissertation includes numerous, comprehensive experimental studies that are generally important for the characterization of emerging, potentially pre-pandemic viruses and may provide crucial information about the future dominance of certain virus variants in an ongoing pandemic. Here, the need for the use of a variety of animal models becomes apparent. By characterizing and classifying potentially zoonotic strains, these methods will help to better prepare for potentially upcoming pandemics and, in the case of a zoonotic or even pandemic event, to better detect and understand the circulating strains and their evolution.
The respiratory epithelium acts as both, a barrier of the respiratory tract to Nipah virus (NiV) entry and at the same time as a significant determinant of virus shedding. Both, for humans and pigs, replication in the respiratory tract epithelia is considered a major factor in transmission to other hosts. To understand why the virus constitutes a high-risk pathogen for livestock and humans, knowledge about
viral replication and host responses in relevant cells and tissues is crucial. Most in vitro studies, however, have been performed in conventional cell lines or non-differentiated lung cells. Only a few examples exist where Henipavirus infections have been investigated in fully-differentiated lung
epithelial cell models.
Thus, one aim of this thesis was to investigate infection, replication, spread and host protein dynamics of NiV in primary bronchial epithelial cells (BEC) cultivated at the air-liquid-interphase (ALI). By
immunofluorescence imaging, the NiV infection dynamics in BEC-ALI cultures were monitored over a 12 day time course, in order to provide detailed information about the infection process in the
respiratory epithelium of pigs and ferrets. Compared to undifferentiated primary BEC, the specific infectivity of NiV in BEC-ALI cultures was low. Infections remained focal and complete infection of the
cultures was not observed, even at 12 dpi. Analysis of viral titers and viral mRNA indicated a limited
virion release from the infected ALI-cultures while most of the newly synthesized NiV-RNA remained
cell associated. Immunofluorescence analysis of cross sections from infected ALI-cultures revealed
large infected areas that exhibited a strong cytopathic effect (CPE). Disruption of the epithelium
resulted in apical release of virus antigen-positive cell detritus while ciliated areas and basal cells were
less affected. From these data it was concluded, that NiV transmission could be supported by
exhalation of cell debris associated NiV and thus may contribute to rapid spread of infection in swine
populations.
A second aim was to explore the dynamics of host responses to NiV infection in differentiated BEC-ALI
culture and to assess whether this differs to conventional cell line data available from literature. Even
though strong CPE appeared in later phases of NiV infection, at least the porcine PBEC-ALI cultures
remained robust enough to allow protein sampling over 12 days infection course. Subsequent MS-based proteomics enabled unprecedent insight in complex cell culture response upon NiV infection.
Previous reports indicated a lack of efficient interferon type I induction in non-differentiated pig or
human BEC which were considered a prerequisite for efficient replication in the respiratory epithelium
and virusspread. In contrast to non-differentiated pig BEC (PBEC), in PBEC-ALI cultures multiple factors
involved in interferon responses were upregulated upon NiV infection. Thereby it was demonstrated
that NiV infection induced a robust innate immune response upon infection with elevated components of antigen processing and presentation resulting in the conversion from the constitutive proteasome to the immunoproteasome. In contrast to previous reports about NiV-infected non-differentiated
PBEC or endothelial cells, incomplete immunoproteasome formation and limitations in interferon
response could be excluded. Thus, a model is proposed in which NiV infection and spread in differentiated PBECs is slowed by potent innate immune responses to the virus infection. Overall, the
findings highlight the important role of the respiratory epithelium not only as a physical barrier to virus
infections but also indicate itsrole as a primary site of adaptive immune induction through NiV induced
antigen processing and MHC I presentation.
Finally, to allow functional studies of Henipaviruses at the BSL-2 biosafety level a recombinant CedPV
was generated and rescued. An imaging based screening and quantitative analysis pipeline was established to investigate the role of cellular factors and to screen for potential virus and host gene
directed inhibitory factors. Accordingly, different host and viral genes were targeted with a siRNA-pool
either targeting virus or selected cellular mRNAs followed by the infection with the CedPV and the
quantification of infected cells. With proof of concept of the siRNA screening pipeline, the recombinant
CedPV clone was used as a backbone to insert variousfluorescence reporter genesin order to optimize
the analysis workflow by allowing direct virus quantification in live, unstained samples. Consequently,
this thesis provides a valuable proof for future approaches related to the function of virus proteins,
influence of host-factors and virusreplication and Henipavirus-inhibitorscreens at low biosafety levels.
The role of cell-penetrating peptides in the induction of T cell responses by virus-like particles
(2023)
Many viral structural proteins can self-assemble into virus-like particles (VLPs). VLPs can serve as an effective vaccine or be used as a vaccine platform. One of these structural proteins is the hepatitis B virus core antigen (HBcAg), which appears to be suitable as an antigen carrier due to its high immunogenicity. HBcAg has a major immunodominant region (MIR) that is presented on the surface of the VLPs after self-assembly. Foreign antigens can be inserted into this region. Since HBcAg VLPs, unlike the Hepatitis B virus (HBV), do not have an envelope, they are not able to penetrate cell membranes efficiently. As an extracellular antigen, HBcAg VLPs primarily induce a strong humoral immune response.
In the present study, we investigated the extent to which HBcAg can be modified to also elicit an enhanced cellular, particularly a cytotoxic, immune response. A cytotoxic CD8+ T cell response is predominantly induced by intracellular antigens. Therefore, our goal was to increase the cell penetration capacity of VLPs. We aimed to achieve this by fusing cell-penetrating peptides (CPPs) to HBcAg. CPPs can spontaneously penetrate cell membranes to enter the cytoplasm of cells. To guarantee that the CCPs were localized to the surface of the VLPs, we fused CPPs to the N-terminus of HBcAg. The CCPs were followed by a tag to allow the purification of VLPs. The T cell epitopes, against which the induced CTL should be directed, were derived from the Large T antigen and inserted into the MIR of HBcAg. Finally, we fused fluorescent proteins to the C-terminus of HBcAg to track the entry of VLPs into cells.
Modifications of HBcAg may lead to reduced stability or altered structure of VLPs. To analyze the stability of VLPs, we used nanoscale differential scanning fluorimetry (nanoDSF) analysis. This revealed that the N-terminal fusion of CPPs or the tag to HBcAg does not reduce VLP stability. However, some peptides incorporated into the MIR had a significant effect on the structure and stability of the VLPs. While the incorporation of a Flag-tag or a peptide from ovalbumin had no negative effect on VLP stability, the incorporation of peptides representing T cell epitopes of Large T antigen interfered with VLP formation. Denaturation and reassembly of the aggregates significantly improved the homogeneity of the VLPs, and the C-terminal addition of arginine-rich domains enhanced stability.
Using live cell imaging and flow cytometry, we demonstrated that HBcAg VLPs functionalized with CPP exhibited up to 40% more efficient penetration into professional antigen-presenting cells (JAWS II) than HBcAg VLPs without CPP. This resulted in the increased presentation of integrated T cell epitopes by dendritic cells. In vivo, we detected significantly increased induction of SV40 Large T antigen-specific CTL in mice immunized with CPP-conjugated VLPs compared to unconjugated VLPs.
In this study, we demonstrated that a stronger cellular immune response can be induced by CPP-functionalized HBcAg VLPs than with the unmodified HBcAg VLPs in vitro as well as in vivo. This discovery may have positive implications for future vaccine development where an enhanced cellular component of the immune response is desirable.
Mass spectrometry-based Proteome analysis of porcine cells infected with African swine fever virus
(2023)
ASFV, a highly contagious, pathogenic and lethal pathogen of swine, poses a major threat to domestic and wild suids worldwide as neither vaccines nor treatments are available. Compared to other well-characterized similarly complex viruses like herpesviruses or adenoviruses, the understanding of ASFV biology is poor.
To improve the understanding of ASFV biology, following the establishment of a robust protocol for the isolation of primary monocyte-derived porcine macrophages (moMΦ) and their infection with ASFV for mass spectrometry (MS)-based proteome analysis was performed.
Under both conditions, naïve and infected, the isolated cells showed cell type-specific characteristics like phagocytosis and antigen presentation and protein expression patterns, including the expression of swine leucocyte antigens and CD markers. Furthermore, moMΦ could be reproducibly infected with ASFV isolates of different genotypes and pathogenicity.
The ASFV protein expression patterns in moMΦ correlate well with those observed in established cell lines at transcript and protein level. The expression of 27 ASFV proteins was confirmed at the protein level. Among them, 9 members of multi-gene families (MGF) and 12 novel open reading frames (nORFs) were recently predicted based on transcription start site mapping.
The direct comparison of closely related ASFV genotype II isolates revealed no virulence-associated protein expression patterns beyond those expected based on the genome sequences of the isolates.
Using different MS quantification strategies, it was shown that ASFV affects both static protein expression levels and protein synthesis. These changes in protein expression impact proteins and pathways known to be targeted by ASFV, including CD-markers, ER-stress and cell death pathways, and cellular antiviral responses. Beyond these observations that further validated the moMΦ infection model, novel effects of the ASFV infection on the cellular proteome were noticed.
These effects include the decreased expression levels of cathepsins, especially cathepsins D (CTSD), H (CTSH) and L (CTSL) as well as the transient activation of MAPK14/p38 prior to its strong downregulation. In addition to MAPK14/p38 further members of the MAPK14/p38 signaling pathway, like MAPKAPK2, were affected by ASFV infection.
As these modulations of the cellular proteome would in general result in decreased pro-inflammatory responses, it did stand out that the synthesis of interferon-response related genes including MX1 and ISG15 evaded the ASFV-induced global reduction of protein synthesis. In contrast, the synthesis of genes involved in RNA processing and splicing was significantly impaired. In total, the regulations of individual host proteins assessed in the context of the whole cellular proteome integrate well with each other and other cellular responses to ASFV infection and may help to improve the understanding of host-virus interactions.
Overall, this thesis provides novel insights into the expression of ASFV-encoded ORFs of different isolates and the host response to ASFV infection. It points out that the current knowledge of the ASFV coding capacity, temporal protein expression patterns, protein functionality, post-translational modifications and host interactions is still sketchy as many aspects of ASFV replication have yet to be understood. The established moMΦ-model to study ASFV infections in vitro provides a powerful tool for future applications to increase the understanding of ASFV biology.
Hepatitis E virus (HEV) is emerging worldwide as a zoonotic pathogen that has remained largely undetected for decades, if not centuries. Its enormous success can be attributed to the wide range of host species, which can transmit the virus to humans, depending on the viral genotype. As a result, HEV is likely to remain a challenge even when the remaining hepatitis viruses (HAV, HBV, HCV), which are transmitted exclusively between humans, are under control. Although millions of HEV infections occur each year, little is known about this puzzling pathogen. One major issue in HEV research is the lack of reliable model systems. Established animal models are inefficient, expensive, or simply not representative of human HEV. On the other hand, cell culture systems are limited by the slow growth of the virus and inefficient replication and infection. The aim of this work is to with deepen the understanding of zoonotic HEV in animal hosts in Germany. For this purpose, a molecular and phylogenetic characterization of HEV sequences from rabbits and swine was conducted. A novel subtype of the zoonotic genotype HEV-3 was identified in a rabbit sample, further emphasizing the role of rabbits as HEV host species and possible reservoir of zoonotic HEV infections in Germany. On the other hand, a molecular biological screening of pigs and wild boars in Mecklenburg-Western Pomerania indicates a wide range of HEV-3 subtypes circulating in swine in north-east Germany. Furthermore, an optimized replicon system was established in order to enable characterization of various HEV sequences by reverse genetics. As a proof of concept, two rabbit HEV derived replicons were compared with two established, cell culture adapted HEV strains. The influence of different regions of the nonstructural protein on HEV replication was determined and quantified. In particular, a system was established, to reproducibly compare different strains and genotypes. This refined replicon system will enable the characterization of further HEV sequences and thus expand the knowledge on the determinants of the viral life cycle.
In vitro and in vivo analyses of mono- and mixed-species biofilms formed by microbial pathogens
(2022)
Microbial biofilms can be defined as multicellular clusters of microorganisms embedded in a self-produced extracellular matrix (ECM), which is primarily composed of polymeric biomolecules. Biofilms represent one of the most severe burdens in both industry and healthcare worldwide, causing billions of dollars of treatment costs annually because biofilms are inherently difficult to prevent, treat, and eradicate. In health care settings, patients suffering from cystic fibrosis, or patients with medical implants are highly susceptible to biofilm infections. Once a biofilm is formed, it is almost impossible to quantitatively eradicate it by mechanical, enzymatical, chemical, or antimicrobial treatment. Often the only remaining option to fully eradicate the biofilm is removing of the infected implant or body part. The primary reasons for the inherent resistance of biofilms against all forms of antimicrobial treatment are (I) a reduced metabolic activity of biofilm-embedded cells climaxing in the presence of metabolic inactive persister cells, as well as (II) the protective nature of the biofilm matrix acting as a (diffusion) barrier against antimicrobials and the host immune system. Consequently, there is an urgent need to better understand microbial biofilms from a structural and (patho-) physiological point of view in order to be able to develop new treatment strategies.
Therefore, the aims of this study were to investigate fundamental physiological properties of different clinically relevant single and multi-species biofilms, both in vitro and in vivo. Furthermore, the effectiveness of a novel treatment strategy using cold atmospheric pressure plasma was evaluated in vitro to treat biofilms of the pathogenic fungus C. albicans.
In article I, the intracellular and ECM protein inventory of Staphylococcus aureus during in vitro biofilm growth in a flow reactor was analyzed by liquid-chromatography coupled to tandem mass-spectrometry (LC-MS/MS) analysis combined with metabolic footprint analysis. This analysis showed that anaerobiosis within biofilms releases organic acids lowering the ECM pH. This, in turn, leads to protonation of alkaline proteins – mostly ribosomal proteins originating from cell lysis as well as actively secreted virulence factors – resulting in a positive net charge of these proteins. As a consequence, these proteins accumulate within the ECM and form an electrostatic network with negatively charged cell surfaces, eDNA, and metabolites contributing to the overall biofilm stability.
In article II, the in vivo metaproteome of the multi-species biofilm community in cystic fibrosis sputum was investigated. To this end, an innovative protocol was developed allowing the enrichment of microbial cells, the extraction of proteins from a small amount of cystic fibrosis sputum, and subsequent metaproteome analysis. This protocol also allows 16S sequencing, metabolic footprint analysis, and microscopy of the same sample to complement the metaproteome data. Applying this protocol, we were able to significantly enhance microbial protein coverage providing first insights into important physiological pathways during CF lung infection. A key finding was that the arginine deaminase pathway as well as microbial proteases play a so far underappreciated role in CF pathophysiology.
In articles III and IV, a novel treatment strategy for biofilms formed by the important fungal pathogen Candida albicans was evaluated in vitro. Biofilms were treated with two different sources of nonthermal plasma (with the Nonthermal Plasma Jet “kINPen09” as well as with the Microwave-induced plasma torch “MiniMIP”) and the effect on growth, survival, and viability was assessed by counting colony-forming units (CFU), by cell proliferation assays, as well as by live/dead staining combined with fluorescence microscopy, confocal laser scanning microscopy, (CLSM) and atomic force microscopy (AFM). These tests revealed that biofilms were effectively inactivated mostly on the bottom side of biofilms, indicating a great potential of these two plasma sources to fight biofilms.
The order of bats (Chiroptera) account for ~20% of all mammalian species and attracted immense global attention due to their identification as important viral reservoir. Bats can harbour a plethora of high-impact zoonotic viruses, such as filoviruses, lyssaviruses, and coronaviruses without displaying clinical signs of disease themselves. Given this striking diversity of the bat virome, their ability of self-powered flight, and global distribution, understanding chiropteran immunity is essential to facilitate assessment of future spillover events and risks.
However, scarcity of bat-specific or cross-reactive tools and standardized model systems impede progress until today. Furthermore, the richness of species led to generation of isolated datasets, hampering data interpretation and identification of general immune mechanisms, applicable for various chiropteran suborders/families. The key to unlocking bat immunity are coordinated research approaches that comprehensively define immunity in several species. In this work, an in-depth study of innate and adaptive immune mechanisms in the fructivorous Egyptian Rousette bat (Rousettus aegyptiacus, ERB) is presented.
Detailed stability analyses identified EEF1A1 as superior reference gene to ACTB, and GAPDH, which rendered unstable upon temperature increase or presence of type-I-IFN. Since the body core temperatures of pteropid bats reach from 35°C to 41°C and it has been postulated that bats display constitutive expression of IFNs, a suitable reference gene has to be stable under these physiologically relevant conditions. To study cellular innate immunity in detail, cell lines from the nasal epithelium, the olfactory compartment and the cerebrum were generated. To include immune responses of epithelia cells, essential for immunity at sites of primary viral infection, primary epithelia cells from the nasal epithelium, trachea, lung and small intestine were generated. Cellular identities were determined by comprehensive analyses of transcripts and proteins expressed by each cell line. The capacity of each cell line to produce type-I- and III-IFNs was assessed at 37°C and 40°C upon stimulation with viral mimetics. This revealed cell type-dependent differences is the capability to express IFNs upon stimulation. Furthermore, the constitutive expression of type-I- and III-IFNs was significantly elevated in higher temperatures and quantified at mRNA copy levels. To characterize ERB innate immunity upon infection with high-impact zoonotic viruses, cells from the nasal epithelium, the olfactory system, and the brain were infected with several lyssaviruses. This revealed striking differences in susceptibility: cells from the nasal epithelium rendered least whereas cells from the olfactory epithelium rendered most susceptible to viral infection and replication. Additionally, due to a lack of IFN expression in infected cells, it could be shown that LBV possibly possesses advanced strategies to ensure successful replication in ERB cells. Since the current SARS-CoV-2 pandemic put bats even further in the focus of zoonotic research, primary epithelial cells and animals were infected with this virus to monitor ERB-specific immune transcripts in cells and tissues. These studies revealed a notably early IFNG expression in the respiratory tract of infected individuals.
To understand immunomaturation in bats, the immune cell landscape in periphery and various tissue in adult and juvenile ERB was analyzed by flow cytometry and scRNA-seq, revealing intriguing, age-dependent variations in the abundance of granulocytes and lymphocytes. Flow cytometry revealed a significantly higher number of granulocytes in adults, as well as higher numbers of B cells in juveniles. scRNA-seq allowed detailed identification of different leukocyte subsets, uncovering the presence of highly-abundant NKT-like cells and a unique PLAC8 expressing B cell population. A functional characterization of phagocytic cells and lymphocytes derived from adult and juvenile ERB revealed no significant differences in cellular functionality.
In conclusion, the presented work demonstrated suitability of all established ERB cell lines to study bat immunity in vitro, which led to striking findings regarding IFN expression at steady state, or upon stimulation or viral infection. In addition, established qRT-PCR protocols allowed definition of constitutive and temperature-dependent elevation of IFN expression magnitudes, as well as insights into expression of immune-related transcripts in SARS-CoV-2 infected ERB. Finally, based on optimized scRNA-seq technologies and flow cytometry, frequencies and absolute cell counts could be determined in ERB of different ages, revealing e.g. age-dependent variations in leukocyte profile compositions.
Clostridioides difficile is the leading cause of antibiotic-associated diarrhea referring to infections of the gastrointestinal tract in the course of (broad-spectrum)antibiotic therapy. While antibiotic therapy, preferentially with fidaxomicin or vancomycin, often stops the acute infection, recurrence events due to remaining spores and biofilm-associated cells are observed in up to 20% of cases. Therefore, new antibiotics, which spare the intestinal microbiota and eventually clear infections with C. difficile are urgently required. In this light, the presented work aimed at the evaluation and characterization of three natural product classes, namely chlorotonils, myxopyronins and chelocardins, with respect to their antimicrobial activity spectrum under anaerobic conditions and their potential for the therapy of C. difficile infections. Briefly, compounds of all three classes were screened for their activity against a panel of anaerobic bacteria. Subsequently, the systemic effects of selected derivatives of each compound class were analyzed in C. difficile using a proteomics approach. Finally, appropriate downstream experiments were performed to follow up on hypotheses drawn from the proteomics datasets. Thereby, all three compound classes demonstrated significant activity against C. difficile. However, chelocardins similarly inhibited the growth of other anaerobes excluding chelocardins as antibiotic candidates for C. difficile infection therapy. In contrast, chlorotonils demonstrated significantly higher in vitro activity against C. difficile and close relatives compared to a small panel of other anaerobes. In addition, it could be shown that chlorotonils affect intracellular metal homeostasis as demonstrated in a multi-omics approach. The data led to speculate that chlorotonils eventually affect cobalt and selenate availability in particular. Moreover, a metaproteomics approach verified that oral chlorotonil treatment only marginally affected the intestinal microbiota of piglets on taxonomic and functional level. Furthermore, the proteome stress response of C. difficile 630 to myxopyronin B, which similarly showed elevated activity against C. difficile compared to a few other anaerobes, indicated that the antibiotic inhibited early toxin synthesis comparatively to fidaxomicin. Finally, evidence is provided that C. difficile 630 responds to dissipation of its membrane potential by production and accumulation of aromatic metabolites.
Avian influenza viruses (AIVs) have their natural reservoir in wild aquatic birds but occasionally
spread to terrestrial poultry. While AIVs of subtypes H5 and H7 are well known to evolve highly
pathogenic avian influenza viruses (HPAIVs) during circulation in domestic birds, non-H5/H7
subtypes exhibit only a low to moderate pathogenicity. Furthermore, spillover events to a broad
range of mammalian hosts, including humans, with self-limiting to severe illness or even fatal
outcomes, were reported for non-H5/H7 AIVs and pose a pandemic risk. The evolution of high
virulent phenotypes in poultry and the adaptation of AIVs to mammalian hosts are predominantly
linked to genetic determinants in the hemagglutinin (HA). The acquisition of a polybasic cleavage
site (pCS) is a prerequisite for the evolution of HPAIVs in poultry, while changes in the receptor
binding preference and virus stability are essential for adaptation of AIVs to mammals.
In August 2012, an H4N2 virus with the pCS motif 322PEKRRTR/G329 but preserved trypsin
dependend replication and low pathogenicity in chickens was isolated on a quail farm in California.
In the first two publications, we followed different approaches to investigate virulence factors and
the potential risk for the transition of H4N2 to high virulence in chickens. The loss of N-terminal
glycosylations in the vicinity of the pCS resulted in decreased binding to avian-like receptors and
dramatically decreased virus stability. On the other hand, one deglycosylation increased virus
replication and tissue tropism in chicken embryos but did not alter virulence or excretion in
chickens. Furthermore, additional basic amino acids in the natural pCS motif improved the trypsin-independent
cleavage of HA and caused slightly increased tissue tropism in chickens. However,
the engineered motifs alone did not affect virulence in chickens. Intriguingly, they even had a
detrimental effect on virus fitness, which was restored after reassortment with segments of HPAIV
H5N1. Together, the results show the importance of HA glycosylations on the stability of H4N2 and
reveal the important role of non-HA segments in the transition of this virus to high virulence in
poultry.
The transmission of another non-H5/H7 AIV of subtype H10N7 from birds to seals resulted in mass
deaths in harbor seals in 2014 in northern Europe. The third publication describes nine mutations
in the HA1 subunit of seal isolates compared to avian H10Nx viruses. We found that some of these
mutations conferred a dual specificity for avian and mammalian receptors and altered
thermostability. Nevertheless, the H10N7seal remained more adapted to avian host cells, despite
of the alteration in the receptor binding specificity.
Altogether, this thesis demonstrates that naturally evolved AIVs beside H5 and H7 subtypes
support a highly pathogenic phenotype in the appropriate viral background and alter virulence and
host receptor specificity by few amino acid substitutions in the HA. These findings improve our
knowledge of the potential of non-H5/H7 AIVs to shift to high virulence in birds and the adaptation
in mammals.
A significant fraction of the decaying algal biomass in marine ecosystems is expected to be mineralized by particle-associated (PA) heterotrophic bacterial communities, which are thus greatly contributing to large-scale carbon fluxes. Whilst numerous studies have investigated the succession of free-living (FL) marine bacteria, the community structure and functionality of PA bacterial communities remained largely unexplored and knowledge on specific contributions of these microorganisms to carbon cycling is still surprisingly limited. This has mostly been due to technical problems, i.e., caused by the enormous complexity of marine particles and the high abundance of eukaryotic microorganisms within these particles. This thesis presents (a) an optimized metaproteomics protocol for an in-depth characterization of marine PA bacteria, (b) an application example with FL and PA communities sampled during a spring phytoplankton bloom in 2009 in the North Sea, which confirmed the reliability of the optimized metaproteomic workflow, (c) the metaproteomic analysis of particulate communities sampled during a spring phytoplankton bloom in 2018, resulting in an as yet unprecedented number of identified protein groups of the bacterial response bloom and (d) a proteomic analysis of a PA bacterial isolate grown on the two naturally abundant marine polysaccharides laminarin and alginate. The observed succession of bacterial clades during metaproteomic analyses of the investigated blooms highlights individual niche occupations, also visible on genus level. Additionally, functional data shows evidence for the degradation of different marine polysaccharides e.g., laminarin, alginate and xylan supporting the important role of PA bacteria during the turnover of oceanic organic matter. Furthermore, most of the identified functions fit well with the current understanding of the ecology of an algal- or surface-associated microbial community, additionally highlighting the importance of phytoplankton-bacterial interactions in the oceans. More detailed insights into the metabolism of PA bacteria were gained by the proteomic characterization of a selected PA bacterial isolate grown on laminarin and alginate. Functional analyses of the identified proteins suggested that PA bacteria employ more diverse degradation systems partially different from the strategies used by FL bacteria.
Gram-negative bacteria are known to naturally produce outer membrane vesicles (OMVs), which are closed nanoparticles (10 to 450 nm) containing virulence factors and pathogen associated molecular patterns (PAMPs). For over 20 years, OMVs of Neisseria meningitidis (N. meningitidis), in combination with three purified outer membrane proteins, have been successfully used as parts of human vaccines which illustrates the safety and potential of OMV based vaccines. So far only little is known about the OMVs of fish pathogenic bacteria. The production of OMVs has been described for the fish pathogenic gram-negative bacterium Aeromonas salmonicida (A. salmonicida) which is the causative agent of furunculosis resulting in high morbidity and mortality of salmonid fish. The immunostimulatory potential of OMVs derived from A. salmonicida as well as the possibility of establishing an oral vaccine model in Oncorhynchus mykiss (O.mykiss) (Rainbow trout) has been investigated in this study by conducting in vitro and in vivo experiments. Innate immune cells such as macrophages are one of the first cells to respond to pathogens once they breach the skin barrier, therefore the monocyte/macrophage cell line RTS-11 as well as leukocytes from the head kidney, consisting of a high percentage of phagocytic cells have been investigated. Additionally, leukocytes isolated from the peritoneal cavity as the main target for injectable vaccines have been studied in the in vitro experiments. These experiments indicate that OMVs derived from A. salmonicida are recognized by the monocyte/macrophage cell line RTS-11 as well as by leukocytes from the head kidney resulting in significant changes of the mRNA expression pattern of early inflammatory markers (IL-1β, IL-6, IL-8, IL-10, TGFβ). Having used the established peritoneal inflammation model of rainbow trout it could be shown that intraperitoneal (i.p.) vaccination of rainbow trout with OMVs results in a similar local immune response, especially in the recruitment of myeloid cells, compared to the injection of inactivated bacteria. The systemic cellular immune response differed between the two vaccine groups, even though a similar humoral immune response could be observed. Interestingly, i.p.vaccination with 10 µg of OMVs resulted in similar antibody titers as observed for fish, that were i.p. vaccinated with 108 CFU of inactivated A. salmonicida. The similar antibody titers after vaccination with OMVs might be explained by a stronger activation of CD8- T cells (likely CD4+ T cells) in the head kidney as well as in the blood in the OMV vaccinated group alone, which might result in an increased stimulation of B cells to produce antibodies.
Oral vaccination has been described as the ideal vaccination method for fish, but only few vaccines for oral application are licensed. Therefore, the established oral model for vaccination of rainbow trout with attenuated viral hemorrhagic septicemia virus (VHSV) was adapted to be used for inactivated A. salmonicida, even though initial trials indicated great similarities in the cellular response after i.p. and oral vaccination with inactivated strains of A. salmonicida, particularly in the response of the myeloid cells and lymphocytes in the target organs as well as the thrombocytes in the spleen. This could not be confirmed in a second oral vaccination trial. These results show how challenging the development of oral vaccines for fish is. The main challenge is the reproducibility of reliable results, since this is influenced by the difference in uptake of vaccine pellets or antigen degradation in the gut. Future oral vaccine trials should investigate different vaccination regimes, e.g., consecutive feeding, or a different composition of vaccine pellets, in order to further investigate the possibility of establishing an oral vaccine model for trout and so that future vaccine candidates, like OMVs, can be reliably tested in fish.
Compared to other human pathogens, S. aureus outstands with a remarkably broad spectrum of deseases: from minor skin infections over endocarditis, pneumoniae, and osteomyelitis, to septic shock. The prerequisite is an arsenal of adaptation strategies, encoded in the core and variable genome. It includes the coordinated expression of adhesins and toxins, evasion of the immune system, response to stress and starvation, adaptation of the metabolism, formation of biofilms and capsules, antibiotic resistance, and persistence on the skin, in nasal epithelial cells, and even in the inner of macrophages after phagocytosis. All these adaptation strategies enable S. aureus to colonize a diversity of niches within the human host. The inevitable requirement is the ability to activate the appropriate adaptation strategy at the right time and at the right place. S. aureus overcomes this challenge with a sophisticated regulatory network. This PhD thesis covers a broad spectrum of transcriptional regulators, involved in S. aureus pathogenesis: (1) the quorum sensing system Agr (regulation of early- and late stage virulence factors), (2) the Sar family (regulation of early- and late stage virulence factors), (3) SaeRS (regulation of accessory exotoxins and adhesins), (4) CodY (response to amino acid starvation, including extracellular proteases), (5) Sigma B (general stress response, including virulence factors), (6) Rex (anaerobic energy metabolism), (7) CtsR and HrcA (protein quality control), (8) PerR and Fur (oxidative stress response), and (9) antibiotic resistance. Traditionally, Proteomics constitute the long-lasting reputation of the Institute. In fact, the majority of investigations presented in this PhD thesis was initialized by proteomic analyses as the ultimate starting point. From the first day, a major goal of this PhD thesis was to add regulator-promoter interaction studies to the methodical spectrum. In particular, to complement transcriptomic and proteomic results by answering the logical follow-up question: Which regulator is responsible for the observed changes in gene expression and protein synthesis after application of a specific stimulus?
The first chapter provides specific analyses for three major regulators: Rex, CodY, and SarA. Publications were achieved for Rex (Hecker et al., 2009; Pagels et al., 2010). Results were mainly achieved by establishing regulator-promoter interaction methods (in particular EMSA and “footprinting”). Additionally, this chapter describes method development of a novel easy-to-apply method, named REPA (restriction endonuclease protection assay).
The second chapter presents method development for the genome-wide identification of regulator-promoter interactions, named “global footprinting”. This approach combines two already well-established methods: (A) Purification of a recombinant Strep-tagged regulator via Strep-tag affinity chromatography. The modification in “global footprinting” is to incubate the regulator with fragmented genomic S. aureus DNA, resulting in co-purification and enrichment of DNA streches with specific regulator binding sites. (B) Identification and quantification of these DNA streches via “next generation sequencing” (NGS). Using this combined approach, this PhD thesis was able to localize the most affine promoter binding site for the regulator Rex precisely down to one single base pair across the whole S. aureus genome.
The third chapter describes the assembly of a data library, collecting the majority of DNA microarray data and regulator-promoter interaction studies from the worldwide literature. This data library summarizes more than 50,000 regulatory events and more than 2,000 regulator binding sites. As published in the perspectives in Fuchs et al. (2018), this data library can be incorporated into the free-accessible online data base “Aureowiki” (provided and maintained by the Department of Functional Genomics, University of Greifswald). The major effort is the consolidation of these “big data” via in silico cluster analysis, comparing 282 different experimental conditions at once. The major finding of this analysis is the identification of seven functional and regulatory gene clusters in S. aureus pathogenesis that are conserved across S. aureus strain diversity. These findings allowed the creation of a prediction tool, to provide novel experimental starting points for the worldwide S. aureus research community. This prediction tool was successfully applied on several topics, and partially published: functional and regulatory prediction for a set of 20 selected lipoproteins as potential virulence factors (Graf et al., 2018), and prediciton of protein complexes (Liang et al., 2016).
Alltogether, this PhD thesis provides new insights into the molecular mechanisms of three pathogenesis-relevant regulators: Rex, CodY, and SarA. It describes the development of three novel experimental methods for wet and dry lab applications that can be used on research topics beyond S. aureus: REPA, “global footprinting”, and cluster analysis. Finally, cluster analysis identifies seven conserved fuctional and regulatory gene clusters, involved in S. aureus pathogenesis. This cluster anaysis is used as a prediction tool to provide novel experimental starting points, and to predict the physiological mode of action of newly discovered anti-staphylococcal agents.
The aim of this work was to characterize the distribution of TULV in European common vole populations, to clarify the host association of TULV and to investigate correlations between host population dynamics and changes in TULV prevalence. Furthermore, the potential of common voles as reservoir for other rodent-borne pathogens was examined in comparison to other rodent species.
Molecular and serological analysis of rodents captured at 87 locations in Germany, France, Luxembourg, and Austria revealed TULV infections at 53.6 % of all trapping locations. The seroprevalence in common voles was low with a mean of 8.5 % (range: 0 – 19 %). TULV RNA was more often detected (mean: 15.3 %, range 0 - 37.5 %). Field voles (Microtus agrestis) and water voles (Arvicola amphibius) were less often tested positive for TULV: mean seroprevalence was 7 % for field voles and 6.7 % for water voles. RNA could be detected in 5.4 % of all tested field voles and 3.2 % of water voles and with exception of a single field vole only when TULV-RNA-positive common voles were trapped at the same location. Those results indicate that TULV infections of field and water voles are spillover infections from sympatric TULV-infected common voles. Phylogenetic analysis revealed distinct genetic differences between TULV sequences of regions of greater geographical distance which were associated with different evolutionary common vole lineages. Furthermore, we could detect genetic differences between TULV strains from trapping sites close to each other (ca. 10 km).
In a capture-mark-recapture study 1042 common voles captured in live traps in Germany were sampled as well as 225 captured in snap traps. When analyzing the seroprevalence of fluctuating common vole populations over several years and seasons we found a negative correlation between prevalence and population density in the current season but a delayed density-dependent positive correlation between the current population density and seroprevalence in the next season. However, this trend varied geographically between the four trapping locations. Usually, population density as well as seroprevalence peaked at the end of the reproductive period in autumn with the exception of Weissach (2010-2012), Jeeser (2010) and Gotha (2012) where population peaks in summer were observed.
In a pilot study in Austria common voles were captured as well as three other rodent species. They were investigated not only for presence of different viruses (TULV, Dobrava- Belgrade orthohantavirus (DOBV), Puumala orthohantavirus (PUUV), Lymphocytic choriomeningitis mammarenavirus (LCMV), Cowpox virus (CPXV)) but also pathogenic bacteria and endoparasites (Leptospira spp., Toxoplasma gondii, Borrelia afzelii, Coxiella burnetii, Rickettsia spp. und Bartonella spp.). Of all four captured species, common voles were most often infected with at least one pathogen (66.7 %), followed by wood mice (Apodemus sylvaticus) (57.7 %), bank voles (Myodes glareolus) (35 %) and yellow-necked field mice (Apodemus flavicollis) (34.5 %). Common voles were also exceptionally susceptible to multiple infections: 66.7 % of them were infected with two or three different pathogens, compared to 6.9 % of yellow-necked field mice and 2.5 % of bank voles. No multiple infections could be detected in wood mice.
The broad geographic distribution of TULV in its reservoir host is in contrast to the rare reports of human infection but might be explained with a low pathogenicity for humans or with the low prevalence in host populations. In addition, the rare detection of human TULV infections could be a result of the used diagnostic methods. Since the reservoir population is known for its dramatic changes in population density and recurring superabundances which facilitates frequent contact to humans, TULV should more often be considered as cause for human disease in future analysis. In
addition, several other zoonotic pathogens could be detected in common voles which could influence TULV infections in the reservoir host but also TULV transmission to humans and therefore deserve more attention in future research.
Coding constraints imposed by the very small genome sizes of negative-strand RNA viruses (NSVs) have led to the development of numerous strategies that increase viral protein diversity, enabling the virus to both establish a productive viral replication cycle and effectively control the host antiviral response. Arenaviruses are no exception to this, and previous findings have demonstrated that the nucleoprotein (NP) of the highly pathogenic Junín virus (JUNV) exists as three additional N-terminally truncated isoforms of 53 kD (NP53kD), 47 kD (NP47kD), and 40 kD (NP40kD). The two smaller isoforms (i.e. NP47kD and NP40kD) have been characterized as products of caspase cleavage, which appears to serve a decoy function to inhibit apoptosis induction. However, whether they have additional functions in the viral replication cycle remains unknown. Further, the origin and function of NP53kD has not yet been described.
In order to first identify the mechanism responsible for production of the NP53kD variant, a possible role of additional caspase cleavage sites was first excluded using a site mutagenesis approach. Subsequently, alanine mutagenesis was then used to identify a region responsible for NP53kD production. As a result, three methionine residues were identified within the characterized sequence segment of NP, linking the production of NP53kD to an alternative in-frame translation initiation. Further site-directed mutagenesis of the previously identified putative in-frame methionine codons (i.e. M78, M80 and M100) finally led to the identification of translation initiation at M80 as being predominantly responsible for the production of NP53kD. Once the identity of all three NP isoforms was known, it was then of further interest to more deeply characterize their functional roles. Consistent with the N-terminal domain containing RNA binding and homotrimerization motifs that are relevant for the viral RNA synthesis process, it could be demonstrated that all three truncated NP isoforms lost the ability to support viral RNA synthesis in a minigenome assay. However, they also did not interfere with viral RNA synthesis by full-length NP, nor did they affect the ability of the matrix protein Z to inhibit viral RNA synthesis. Moreover, it was observed that loss of the oligomerization motifs in the N-terminus also affected the subcellular localization of all three NP isoforms, which were no longer localized in discrete perinuclear inclusion bodies, but rather showed a diffuse distribution throughout the cytoplasm, with the smallest isoform NP40kD also being able to enter the nucleus. Surprisingly, the 3'-5' exonuclease function of NP, which is associated with the C-terminal domain and plays a role in inhibiting interferon induction by digestion of double-stranded RNAs, was found to be retained only by the NP40kD isoform, despite that all three isoforms retained the associated domain. Finally, previous studies using transfected NP and chemical induction of apoptosis have suggested that cleavage of NP at the caspase motifs responsible for generating NP47kD and NP40kD plays a role in controlling activation of the apoptosis pathway. Therefore, to further characterize the connection between the generation of NP isoforms and the regulation of apoptosis in a viral context, recombinant JUNVs deficient in the respective isoforms were generated. Unlike infections with wild-type JUNV, mutations of the caspase cleavage sites resulted in the induction of caspases activation. Surprisingly, however, this was also the case for mutation of the alternate start codon responsible for NP53kD generation.
Taken together, the data from this study suggest a model whereby JUNV generates a pool of smaller NP isoforms with a predominantly cytoplasmic distribution. As a result of this altered localization, NP53kD appears to be able to serve as the substrate for further generation of NP47kD and NP40kD by caspase cleavage. Not only does this cleavage inhibit apoptosis induction during JUNV infection, it also results in a cytoplasmic isoform of NP that retains strong 3'-5' exonuclease activity (i.e. NP40kD) and thus may play an important role in preventing viral double-stranded RNA accumulation in the cytoplasm, where it can lead to activation of IFN signaling. Overall, such results emphasize the relevance of alternative protein isoforms in virus biology, and particularly in regulation of the host response to infection.
Primary producers, alongside heterotrophic bacteria and viruses, modulate the essential global carbon cycle. About half of the Earth’s net primary production originates in the marine environment. By effecting these systems and the burial of carbon, bacteria play a significant role in the world’s climate, especially with regard to rising temperatures and increasing anthropogenic carbon dioxide production.
Particles present substrate-rich niches for particle-associated bacteria, but are rare in the marine system. Particle-associated bacteria, comprising of chemotactic motile free-living and particle-attached bacteria, were shown to have higher respiration rates, were larger in cell and genome size and showed a higher hydrolytic activity of extracellular enzymes compared to the free-living fraction.
Understanding the contribution of particle-associated bacteria to the degradation of algal biomass is essential to understand the marine carbon cycle. However, the identification of this group is difficult and required refinement.
Sequential filtration, the most commonly used technique for the separation of bacterial fractions, provides only access to a part of the particle-associated microbiome, and includes with large and clustered bacteria undesired false-positives. To overcome these limitations, separation by gravity in Imhoff sedimentation cones was explored in this thesis to access, identify and define particle-associated microbiomes, in comparison and conjunction with the established separation techniques like sequential filtration and centrifugation.
The cultivability on agar plates was assessed, aiming at the question which portion of the colony-forming bacteria belong to free-living non-motile or motile bacteria or to particle-attached bacteria. As continuous cultivation on plates often involves loss of cultures, colonies of the original plate were used to obtain partial 16S rRNA sequences of individual colonies and of plate microbiomes.
For future studies on particle-associated bacteria, a representative strain collection was established from particle-attached bacteria retained on 3 μm filters and from particle-associated bacteria collected together with settled algae in sedimentation cones.
To understand the contribution of top-down selection to a yearly recurring bacterioplankton bloom at our sampling site Helgoland, particle-associated strains were included in isolation experiments for flavophages, since Flavobacteriia are among the most important responder to the yearly observed blooms.
Overall, this thesis provides new insights into the isolation and cultivation of particle-associated bacteria – an important, but currently not fully understood fraction of organisms within the marine system.
The here presented dissertation investigated the molecular mechanisms, by which the food industry model bacteria Pseudomonas fluorescens and Listeria monocytogenes, grown either as planktonic cultures, were inhibited by plasma treated water (PTW) produced by a microwave-induced plasma source (MidiPLexc). As a starting point, optimal operating parameters were determined with 5 standard liters per minutes(slm)compressed air during the treatment of 10 ml deionized water within a treatment time of up to 15 min (pre-treatment time). Treatment times of 1, 3 and 5 min were selected (post-treatment time). In addition to physical parameters, i.e. temperature measurements at different spots at the plasma source during the production of the PTW, the chemical composition of PTW was determined by pH measurements, chronoamperometry (determination of the H2O2 concentration), ion chromatography (determination of the NO2-, NO3- and ONOO- concentrations) and mass spectrometry (qualitative determination of the molecules). In addition, concentration changes of reactive species over a period of 3 h indicated a decrease of the NO2- concentration as well as an increase of the NO3- and ONOO- concentration in the PTW. Microbiological assays, i.e. quantification of colony-forming units (CFU), fluorescence and XTT assays, revealed a significant reduction of the proliferation ability of the cells, membrane damages and metabolic activity have been demonstrated for planktonic cultures as well as mono- and multispecies biofilms. PTW effects on biofilm structures were investigated using microscopic methods such as fluorescence microscopy, confocal laser scanning microscopy (CLSM), atomic force microscopy (AFM), and scanning electron microscopy (SEM), as well as physical methods such as contact angle measurements. Significant changes in the biofilm structure have been shown, which indicate an ablation of the biofilm mass from top to bottom by approximately 2/3 of the biofilm mass and a destruction of the extracellular matrix (ECM) by the reactive species within the PTW. Subsequently, fresh-cut lettuce has been treated with PTW produced by up-scaled plasma sources. Apart from qualitative parameters of the lettuce after PTW treatment such as texture and color, the concentration of PTW reactive species have been determined. These experiments showed that the composition of the reactive species were slightly different from that of the laboratory-scaled plasma source MidiPLexc. Notably, the PTW treatment did not cause significant changes in texture and color of the fresh-cut lettuce. Finally, a synergistic effect of PTW treatment followed by plasma-processed air (PPA) drying was demonstrated application-specific.
The genus Capripoxvirus of the family Poxviridae consists of the species lumpy skin disease virus, sheeppox virus and goatpox virus that affect cattle, sheep and goats, respectively. Whereas lumpy skin disease virus (LSDV) is transmitted mainly mechanically via blood-feeding insects and possibly hard ticks, the major transmission routes of sheeppox virus (SPPV) and goatpox virus (GTPV) are via direct contact and aerosols. Affected animals develop fever and display clinical signs such as ocular and nasal discharge, lymphadenopathy and characteristic lesions of the skin. Severe clinical course, especially in combination with respiratory signs, can result in the death of the affected animals. In endemic regions, mortality of capripox virus-induced diseases is low (1-10%). However, mortalities of up to 75% have been reported for LSDV and up to 100% for SPPV and GTPV in exotic breeds and high-producing dairy or beef animals. The loss of quality of the leather, reduced weight gain and milk yield as well as complete loss of affected animals have severe impact on national and global economies. Therefore, capripox virus-induced diseases have significant impact on both the affected individual animal as well as on the existence of small-scale farmers and large agricultural enterprises. However, until now, only live attenuated vaccines are commercially available. These attenuated vaccines are not authorized in the European Union and their administration would comprise the disease-free status of the respective country. Thus, reliable diagnostic tools for the detection and characterization of capripox viruses as well as safe and efficient control measures are of high importance.
The objectives of the present thesis were the development, validation and comparison of diagnostic tools, the establishment of challenge infection models and the performance of pathogenesis studies for all three capripox virus species, and the development and testing of different inactivated prototype vaccine candidates against LSDV.
First, new real-time quantitative polymerase chain reaction (qPCR) assays for robust detection and differentiation of LSDV field strains, LSDV vaccine strains, SPPV and GTPV were developed and extensively validated. In the following, two single assays were combined to duplex assays, one for the differentiation between LSDV field strains and LSDV vaccine strains, and the second for discrimination of SPPV and GTPV. Finally, a diagnostic workflow based on these new duplex assays in combination with already published methods was established. This workflow enables time-saving, robust and reliable detection, species-specific identification and genetic and phylogenetic characterization of all three capripox virus species. In addition, already existing serological examination methods (serum neutralization assay and commercial enzyme-linked immunosorbent assay) were compared regarding their sensitivity and specificity. Furthermore, pathogenesis studies with different capripox virus isolates were performed in the respective target species, and the suitability of selected virus isolates as challenge viruses for future vaccine studies was analyzed. Pathogenesis studies with isolates GTPV-“V/103” and LSDV-“Macedonia2016” revealed that both are proper candidates for challenge models. Finally, three different SPPV isolates (SPPV-“V/104”, SPPV-“India/2013/Surankote” and SPPV-“Egypt/2018”) were tested in sheep regarding their virulence to find a suitable challenge model for SPPV, and SPPV-“India/2013/Surankote” was chosen for future vaccine studies.
Once appropriate challenge models were established, different inactivated prototype vaccines against LSDV were developed, and vaccine safety as well as vaccine efficacy were tested in cattle. Eventually, a Polygen-adjuvanted inactivated LSDV-vaccine candidate was selected that is able to fully prevent cattle from any LSDV-related clinical signs after severe challenge infection. Furthermore, molecular and serological data indicate that this inactivated prototype vaccine is even able to induce a kind of “sterile immunity” against LSDV in those cattle. It has to be mentioned that a commercially available vaccine similar to this prototype vaccine would be a great advance for the control of LSDV.
In the future, additional studies addressing diagnostics and optimized control of capripox viruses should be performed. Firstly, probe-based real-time qPCR assays for the differentiation of SPPV and GTPV vaccine strains from their respective virulent field strains should be developed and included into the diagnostic workflow. Secondly, further tests of the inactivated prototype vaccine, e.g. determination of the minimum protective dose and the possibility of cross-protection in sheep and goats against SPPV and GTPV, respectively, should be performed.
Pestivirus-Replikons als Werkzeug für heterologe Genexpression und molekulare Charakterisierung
(2021)
Replikons sind autonom replizierende RNA-Moleküle die nicht in der Lage sind, infektiöse Viren zu bilden. Sie sind wichtige Hilfsmittel zur molekularen Charakterisierung von Viren. Außerdem werden sie erfolgreich als Expressionssystem für Proteine und zur Entwicklung von Impfvektoren eingesetzt. Im Rahmen der vorliegenden Arbeit wurde ein Replikon-basiertes Testsystem für den Nachweis spezifischer Antikörper gegen das atypische porzine Pestivirus (APPV) in Schweineseren etabliert. Auf Basis eines Klons des Virus der bovinen Virusdiarrhoe Typ 1 (BVDV) wurden die ursprünglichen BVDV Glykoproteine E1 und E2 gegen die Glykoproteine des APPV ausgetauscht. Die Expression mittels Replikon gewährleistet die natürliche Konformation der Proteine und damit die Bindung der entsprechenden Antikörper. Dieses System ermöglichte die serologische Untersuchung von 1115 Schweineseren ohne vorherige Isolation oder Zellkulturadaptation des Virus. Mit diesem neu entwickelten System konnte eine Seroprävalenzstudie gestartet und eine hohe Prävalenz von APPV in der untersuchten deutschen Schweinepopulation gezeigt werden.
Im weiteren Verlauf dieser Arbeit wurden Replikons zur Charakterisierung des atypischen Pestivirus Bungowannah Pestivirus (BuPV) eingesetzt. Während die Replikons mit Deletionen der Gene für die einzelnen Strukturproteine C, E1 und E2 oder die gesamte Strukturproteinregion keine Besonderheiten im Vergleich zu bereits untersuchten Pestivirus-Replikons aufwiesen und keine infektiösen Virionen mehr produzieren konnten, zeigten BuPV-Replikons mit ERNS-Deletion die Fähigkeit, zwei weitere Replikationszyklen zu durchlaufen und Zellen zu infizieren, allerdings mit einem sehr deutlichen Wachstumsdefizit. Dieser Defekt scheint in der Virusassemblierung und/oder der Freisetzung aus der Zelle zu liegen. Es konnte somit erstmals gezeigt werden, dass ERNS nicht essentiell für die Bildung infektiöser Bungowannah-Viren ist, jedoch sehr wichtig für eine effiziente Virusvermehrung. Diese Eigenschaft der ERNS deletieren BuPV macht diese besonders interessant als Vektoren für die Entwicklung neuer Replikon-basierter Expressionssysteme und einer Vakzinplattform. ERNS-Deletionsmutanten wurden daher auf ihre Fähigkeit hin untersucht, eine effiziente Expression verschiedener immunogener Proteine zu gewährleisten. Die Konstrukte waren dabei in der Lage, die ausgewählten Proteine effizient zu exprimieren und konnten zudem effizient zu Virus-Replikon-Partikel (VRP) verpackt und in einer trans-komplementierenden Zelllinie vermehrt werden.
Auch der für das parentale Virus beschrieben Zelltropismus konnte für die generierten BuPV-VRP gezeigt werden. Zusätzlich zu den beschriebenen Eigenschaften sind es der nicht-zytopathogene Charakter und die in den meisten Regionen fehlende Immunität gegen BuPV, die das hohe Potential dieses Systems als universellen Vakzinvektor herausstellen.
Zusätzlich wurde im Rahmen dieser Arbeit ein erstes DNA-basiertes System zur Herstellung rekombinanter BuPVs etabliert. Dieses System ermöglicht sowohl die Virusproduktion ausgehend von einem T7-RNA-Polymerase Promotor, als auch von einem Polymerase-II-Promotor. Die infektiösen Viren zeigten gleiche Wachstumseigenschaften wie Viren, welche mit dem konventionellen RNA-System generiert wurden. Auf Basis des neuen DNA-Systems konnte auch ein Replikon mit Deletion im ERNS-Gen etabliert werden. Dieser Klon zeigte nach der Transfektion eine sehr geringe Replikationsrate, konnte jedoch zur weiteren Konstruktion eines „single round infectious particle“ (SRIP) eingesetzt werden. Diese SRIP sind durch die Koexpression des deletierten ERNS in der Lage, sich selbst zu verpacken und bilden damit ein ideales System zum Transport selbst-replizierender RNA. Durch seine selbstlimitierenden Eigenschaften könnte es zur Entwicklung und Etablierung einer effizienten und sicheren Vakzineplattform eingesetzt werden. Allerdings ist dafür eine weiterreichende Optimierung notwendig.
Insgesamt zeigten die Untersuchungen, dass sich pestivirale Replikons sowohl als effizientes und schnelles Testsystem für die Untersuchung der Verbreitung neu auftretender Pestiviren, als auch zur Entwicklung effizienter RNA- und DNA-basierter Transport- und Verpackungssysteme viraler Proteine, eignet.
LPAIV H9N2 and HPAIV H5N8 clade 2.3.4.4 viruses have been frequently isolated from domestic and wild birds in Germany and they are endemic in poultry worldwide. H9N2 is known to donate gene segments to other AIV with high case fatality rate in humans (e.g. H5N1, H7N9). Similarly, H5N8 devastated poultry worldwide since 2014 and has been recently isolated from humans. Therefore, it is important to understand the genetic predisposition for adaptation of H9N2 and H5N8 AIV in poultry and mammals. In the first publication, we focused on the variable hemagglutinin cleavage site (HACS) of European and Non-European H9N2 viruses, since the HACS is a main virulence determinant of AIV in birds. We found a preferential substitution of non-basic amino acids (G, A, N, S, D, K) in the HACS at position 319 of European H9N2 viruses compared to non-European H9N2 viruses. Recombinant viruses carrying different non-basic amino acids in the HACS modulated replication in vitro. While these non-basic amino acids did not affect virulence or transmission in chickens, they modulated virulence and replication in turkeys. Moreover, H9N2 viruses with non-basic amino acids in the HACS were able to replicate in mammalian brain cells for multiple cycles even without trypsin. In the second publication, we addressed the question whether reassortment between two recent German H9N2 and H5N8 clade 2.3.4.4. B viruses is possible and analysed the impact on virus fitness in mammals and birds. We found that H9N2 PB1 and NP segments were not compatible to generate infectious H5N8 viruses and this incompatibility was due to mutations outside the packaging region. However, H9N2 NS alone or in combination with PB2 and PA significantly increased replication of H5N8 in human cells. Moreover, H9N2 PB2, PA and/or NS segments increased virulence of H5N8 in mice. Interestingly, in chickens, reassortment with H9N2 gene segments, particularly NS, partially or fully impaired chicken-to-chicken transmission. These results indicate that the evolution of H9N2/H5N8 reassortants showing high virulence for mammals is unlikely to occur in chickens. In the third publication, we focused on the NS1 protein of different HPAIV H5N8 clade 2.3.4.4 viruses from 2013 to 2019 and studied the impact of its C-terminus (CTE) variation on virus fitness in chickens and ducks. Our findings revealed a preferential selection for a certain NS1 CTE length in 2.3.4.4. H5N8 clade A (237 aa) and B (217 aa) viruses over the common length of 230 aa. Indeed, the NS1 CTE can affect virus virulence and pathogenesis in a species and virus clade dependent manner. In chickens, although there was no impact on virulence, NS1 CTE of H5N8-A and H5N8-B, regardless of the length, have evolved towards higher efficiency to block the IFN response. In ducks, NS1 CTE contributed to efficient transmission, replication and high virulence of H5N8-B. In the fourth publication, we assessed the impact of variable length of NS1 on H5N8 virus replication in human cells and virulence in mice. We showed that NS1 of H5N8-B virus unlike the vast majority of NS1 of AIV, shared preferences for short NS1 similar to human and zoonotic influenza viruses. This virus (i) was able to efficiently block IFN and apoptosis induction which might be the first steps for efficient adaptation to human cells and (ii) without prior adaptation replicated at higher levels and was more virulent in mice than H5N8-A. The virulence of the latter virus increased after shortening the NS1 similar to H5N8-B virus. Therefore, it is conceivable that truncation in NS1 is a determinant for adaptation of H5N8 in mammals irrespective of its impact on virus fitness in poultry. Findings in this dissertation indicated that HA mutations in the European H9N2 and NS1 variations in H5N8 viruses play a role in virus fitness in poultry and/or mammals. These results improve our current understanding for AIV adaptation and are useful to assess the potential of these viruses to infect mammals.
Ebolaviruses are zoonotic pathogens causing severe hemorrhagic fevers in humans
and non-human primates with high case fatality rates. In recent years, the number and
scope of outbreaks has increased, highlighting the importance of better understanding
the molecular aspects of ebolaviral infection and host cell interactions in order to be able to better control this virus.
To facilitate virus genome replication, transcription and protein expression,
ebolaviruses recruit and interact with specific host factors. These interactions play a key role in viral infection and influence virus survival and disease outcome. Based on a genome-wide siRNA screen, the three host factors CAD, NXF1 and UAP56 were
recently identified to be involved in ebolavirus genome replication and/or transcription
and/or mRNA-translation. However, mechanistical details of how these host factors
affect the ebolavirus lifecycle remained elusive.
In this thesis I analyzed the functional interactions between EBOV and these newly
identified host proteins in order to better understand the virus-host interface. To this
end I used siRNA knockdown as well as overexpression of these host proteins in
combination with different reverse-genetics based lifecycle modelling assays to
investigate the influence of CAD, NXF1 and UAP56 on individual aspects of the EBOV
lifecycle. Using these systems in relation with a host factor knockdown I was able to
show that the provision of pyrimidines by CAD plays an important role for both EBOV
genome replication and transcription, whereas NXF1 is predominantly required for
mRNA transport. I furthermore used immunofluorescence analysis to examine whether
these host factors are recruited by one or more EBOV proteins to inclusion bodies,
which represent physical sites of ebolavirus genome replication. During these
experiments, I was able to show that CAD and NXF1, and possibly also UAP56, are
recruited to EBOV inclusion bodies in order to fulfill their individual function for EBOV RNA synthesis or later steps in protein expression. Additionally, I was able to show that the uptake of NXF1 into NP-induced inclusion bodies is most likely mediated via the C-terminal domain of NP, and that the FG-repeat interaction domains of NXF1 are sufficient for recruitment. Further, my data indicate that RNA interaction of both NXF1 and NP is not required for this process, but rather important for exit of NXF1 from inclusion bodies. I therefore suggest that the viral mRNA is transferred in inclusionbodies from NP to NXF1, which leads to a rapid export of the NXF1 packed viral mRNA into the cytosol for mRNA translation.
The exact mechanism of how these host factors are recruited into inclusion bodies and whether they have similar functions in the lifecycle of other negative-sense RNA viruses still needs to be investigated. Nevertheless, this study increases our understanding of virus-host interaction of ebolaviruses, and thus helps to identify targets for the development of novel therapeutics against these viruses.
Streptococcus pneumoniae is a commensal of the human upper respiratory tract and moreover, the
causative agent of several life-threatening diseases including pneumonia, sepsis, otitis media, and
meningitis. Due to the worldwide rise of resistance to antibiotics in pneumococci the understanding
of its physiology is of increasing importance. In this context, the analysis of the pneumococcal
proteome is helpful as comprehensive data on protein abundances in S. pneumoniae may provide
an extensive source of information to facilitate the development of new vaccines and drug
treatments.
It is known that protein phosphorylation on serine, threonine and tyrosine residues is a major
regulatory post-translational modification in pathogenic bacteria. This reversible post-translational
modification enables the translation of extracellular signals into cellular responses and therewith
adaptation to a steadily changing environment. Consequently, it is of particular interest to gather
precise information about the phosphoproteome of pneumococci. S. pneumoniae encodes a single
Serine/Threonine kinase-phosphatase couple known as StkP-PhpP.
To address the global impact and physiological importance of StkP and PhpP which are closely
linked to the regulation of cell morphology, growth and cell division in S. pneumoniae, proteomics
with an emphasis on phosphorylation and dephosphorylation events on Ser and Thr residues was
applied. Thus, the non-encapsulated pneumococcal D39Δcps strain (WT), a kinase (ΔstkP) and
phosphatase mutant (ΔphpP) were analyzed in in a mass spectrometry based label-free
quantification experiment. The global proteome analysis of the mutants deficient for stkP or phpP
already proved the essential role of StkP-PhpP in the protein regulation of the pneumococcus.
Proteins with significantly altered abundances were detected in diverse functional groups in both
mutants. Noticeable changes in the proteome of the stkP deletion mutant were observed in
metabolic processes such as “Amino acid metabolism” and also in pathways regulating genetic
and environmental information processing like “Transcription” and “Signal transduction”.
Prominent changes in the metabolism of DNA, nucleotides, carbohydrates, cofactors and vitamins
as well as in the categories “Transport and binding proteins” and “Glycan biosynthesis and
metabolism” have been additionally detected in the proteome of the phosphatase mutant. Still, the
quantitative comparison of WT and mutants revealed more significantly altered proteins in ΔphpP
than in ΔstkP. Moreover, the results indicated that the loss of function of PhpP causes an increased
abundance of proteins in the pneumococcal phosphate uptake system Pst. Furthermore, the
obtained quantitative proteomic data revealed an influence of StkP and PhpP on the twocomponent
systems ComDE, LiaRS, CiaRH, and VicRK.
Recent studies of the pneumococcal StkP/PhpP couple demonstrated that both proteins play an
essential role in cell growth, cell division and separation. Growth analyses and the phenotypic
characterization of the mutants by electron-microscopy performed within this work pointed out
that ΔphpP and ΔstkP had different growth characteristics and abnormal cell division and cell
separation. Nevertheless, the morphological effects could not be explained by changes in protein
abundances on a global scale. So, the in-depth analysis of the phosphoproteome was mandatory
to deliver further information of PhpP and StkP and their influence in cell division and
peptidoglycan synthesis by modulating proteins involved in this mechanisms.
For more detailed insights into the activity, targets and target sites of PhpP and StkP the advantages
of phosphopeptide enrichment using titanium dioxide and spectral library based data evaluation
were combined. Indeed, the application of an adapted workflow for phosphoproteome analyses
and the use of a recently constructed broad spectral library, including a large number of
phosphopeptides (504) highly enhanced the reliable and reproducible identification of
phosphorylated proteins in this work.
Finally, already known targets and target sites of StkP and PhpP, detected and described in other
studies using different experimental procedures, have been identified as a proof of principle
applying the mass spectrometry based phosphoproteome approach presented in this work.
Referring to the role of StkP in cell division and cell separation a number of proteins participating
in cell wall synthesis and cell division that are apparently phosphorylated by StkP was identified.
In comparison to StkP, the physiological function and role of the co-expressed phosphatase PhpP
is poorly understood. But, especially the list of previously unknown putative target substrates of
PhpP has been extended remarkably in this work. Among others, five proteins with direct
involvement in cell division (DivIVA, GpsB) and peptidoglycan biosynthesis (MltG, MreC, MacP)
can be found under the new putative targets of PhpP.
All in all, this work provides a complex and comprehensive protein repository of high proteome
coverage of S. pneumoniae D39 including identification of yet unknown serine/threonine/tyrosine
phosphorylation, which might contribute to support various research interests within the scientific
community and will facilitate further investigations of this important human pathogen.
Ebolaviruses are dependent on host cell proteins for almost all steps in their viral life cycle. While some cellular factors with crucial roles in the ebolavirus life cycle have been identified, many of them remain to be identified or fully characterised. This thesis focuses on the characterisation and identification of host cell interactions of the highly pathogenic Ebola virus (EBOV), probing host-virus interaction at various stages of the viral life cycle. Beginning with viral budding, the function of a recently proposed late domain motif within the EBOV matrix protein VP40 was examined using an EBOV transcription and replication-competent virus-like particle (trVLP) system. Although this motif has been suggested to interact with the endosomal sorting complex required for transport (ESCRT), we could show that this late domain motif does not contribute to EBOV budding.
While many host cell proteins have been identified so far that are important for viral budding, only a few proteins are known that are necessary for EBOV RNA synthesis. Thus, to identify host proteins that are involved in viral replication and transcription, we performed a genome-wide siRNA screen in the context of an EBOV minigenome assay. Using this approach, we identified several proteins that appear to be important for viral RNA synthesis or protein expression. Two of the most prominent hits in our screen were CAD (Carbamoyl-phosphate synthetase 2, aspartate transcarbamylase and dihydroorotase) and NXF1 (nuclear RNA export factor 1). CAD catalyses the first three steps in the de novo pyrimidine biosynthesis, while NXF1 is the main nuclear export protein for cellular mRNAs. In subsequent characterisation studies, using a range of life cycle modelling systems as well as molecular analyses, we could demonstrate that the canonical function of CAD during the pyrimidine biosynthesis is necessary for EBOV replication and transcription. In contrast to this, for NXF1 we discovered a so-far unknown function: Again, by applying different life cycle modelling alongside with molecular assays, we provided evidence that the EBOV nucleoprotein recruits NXF1 into inclusion bodies, the site of EBOV RNA synthesis, where it binds viral mRNAs to export them from these structures. Importantly, for both CAD and NXF1 we were able to recapitulate key data in the context of live EBOV infection, confirming their roles in the viral life cycle.
Both of these identified host factors are promising targets for antiviral therapies and indeed de novo pyrimidine synthesis is emerging as a possible antiviral target for a number of viruses. Similarly, as we could show NXF1 to be important in the life cycle of the highly pathogenic Junín virus, this raises the possibility that disruption of this interaction may result in broad-spectrum antiviral activity. Moreover, for an increasing number of negative-sense RNA viruses inclusion bodies as site of viral RNA synthesis are described to have a liquid organelle character. Therefore, our findings on NXF1 also provide an intriguing model to explain how negative-sense RNA viruses in general overcome this obstacle and export viral mRNAs from inclusion bodies.
Technological advances in light microscopy have always gone hand in hand with unprecedented biological insight. For microbiology, light microscopy even played a founding role in the conception of the entire discipline. The ability to observe pathogens that would otherwise evade human observation makes it a critical necessity and an indispensable tool to infectious disease research. Thus, the aim of this thesis was to optimize, extend, and functionally apply advanced light microscopy techniques to elucidate spatio-temporal and spatio-morphological components of bacterial and viral infection in vitro and in vivo.
Pathogens are in a constant arms race with the host’s immune system. By finding ways to circumvent host-mediated immune responses, they try to evade elimination and facilitate their own propagation. The first study (publication I) demonstrated that the obligate intracellular pathogen Coxiella burnetii is not just able to infect natural killer (NK) cells, but is actually capable of surviving the harsh degradative conditions in the cytotoxic lymphocyte’s granules. Using live-cell imaging of reporter-expressing Coxiella burnetii, the transient NK cell passage was closely monitored to provide detailed spatio-temporal information on this dynamic process in support of a range of static analyses. Bacterial release from NK cells was pinpointed to a time frame between 24 to 48 hours post-infection and the duration of release to about 15 minutes.
The second approach (publications II-V) aimed at shedding light on the greater spatio-morphological context of virus infection. Thus far, most studies investigating the distribution or tropism of viruses in vivo have used conventional immunohistochemistry in thin sections. Omitting the native spatial context of the infection site in vivo inherently bears the risk of incomplete description. While the microscopic tools and sample preparation protocols needed for volumetric 3D immunofluorescence imaging have recently been made available, they had not gained a foothold in virus research yet. An integral part of this thesis was concerned with the assessment and optimization of available tissue optical clearing protocols to develop an immunofluorescence-compatible 3D imaging pipeline for the investigation of virus infection inside its intact spatio-morphological environment (publication II). This formed the basis for all subsequent volumetric analyses of virus infection in vivo presented here. Consequently, this thesis provided a valuable proof of concept and blueprints for future virus research on the mesoscopic scale of host-pathogen interactions in vivo (publications II-V), using rabies virus (RABV; publications II-IV) and the newly-emerged severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2; publication V) as infection models for the nervous system and the respiratory tract, respectively.
Applying and further improving this volumetric 3D imaging workflow enabled unprecedented insights into the comprehensive in vivo cell tropism of RABV in the central (CNS) (publication III) and peripheral nervous system (PNS) (publication IV). Accordingly, differential infection of CNS-resident astrocytes by pathogenic and lab-attenuated RABV was demonstrated (publication III). While either virus variant showed equal capacity to infect neurons, as demonstrated by quantitative image analysis, only pathogenic field RABVs were able to establish non-abortive infection of astrocytes via the natural intramuscular inoculation route. A combined 3D LSFM-CLSM workflow further identified peripheral Schwann cells as a relevant target cell population of pathogenic RABV in the PNS (publication IV). This suggested that non-abortive infection of central and peripheral neuroglia by pathogenic RABV impairs their immunomodulatory function and thus represents a key step in RABV pathogenesis, which may contribute significantly to the establishment of lethal rabies disease.
Finally, utilizing the full volumetric acquisition power of LSFM, a further refined version of the established 3D imaging pipeline facilitated a detailed mesoscopic investigation of the distribution of SARS-CoV-2 in the respiratory tract of the ferret animal model (publication V). Particularly for this newly-emerged pathogen of global concern, in-depth knowledge of host-pathogen interactions is critical. By preserving the complete spatio-morphological context of virus infection in the ferret respiratory tract, this thesis provided the first specific 3D reconstruction of SARS-CoV-2 infection and the first report of 3D visualization of respiratory virus infection in nasal turbinates altogether. 3D object segmentation of SARS-CoV-2 infection in large tissue volumes identified and emphasized a distinct oligofocal infection pattern in the upper respiratory tract (URT) of ferrets. Furthermore, it corroborated a preferential replication of SARS-CoV-2 in the ferret URT, as only debris-associated virus antigen was detected in the lower respiratory tract of ferrets, thus providing crucial information on the spatial distribution of SARS-CoV-2.
Infectious diseases remain a significant threat to the wellbeing of humans and animals
worldwide. Thus, infectious disease outbreaks should be investigated to understand the
emergence of these pathogens, leading to prevention and mitigation strategies for future
outbreaks. High-throughput sequencing (HTS) and bioinformatic analysis tools are reshaping
the surveillance of viral infectious diseases through genome-based outbreak investigations. In
particular, analyzing generic HTS datasets using a metagenomic analysis pipeline enable
simultaneous identification, characterization, and discovery of pathogens.
In this thesis, generic HTS datasets derived from the 2018-19 WNV epidemic and USUV
epizooty in Germany were evaluated using a unified pipeline for outbreak investigation and an
early warning system (EWS). This pipeline obtained 34 West Nile virus (WNV) whole-genome
sequences and detected several sequences of Usutu virus (USUV) and other potential
pathogens. A few WNV and USUV genome sequences were completed using targeted HTS
approaches. Phylogenetic and phylogeographic inferences, reconstructed using WNV wholegenome sequences, revealed that Germany experienced at least six WNV introduction events.
The majority of WNV German variants clustered into the so-called “Eastern German clade
(EGC),” consisting of variants derived from birds, mosquitoes, a horse, and human cases. The
progenitors of the EGC subclade probably circulated within Eastern Europe around 2011. These
flavivirus genome sequences also provided substantial evidence for the first reported cases of
WNV and USUV co-infection in birds. Phylogenetic inferences of USUV genome sequences
showed the further spread of the USUV lineage Africa 3 and might indicate the overwintering
of the USUV lineage Europe 2 in Germany. Among viral sequences reported in the EWS, Hedwig
virus (HEDV; a novel peribunyavirus) and Umatilla virus (UMAV; detected in Europe for the
first time) were investigated using genome characterization, molecular-based screening, and
virus cultivation since these viruses were suspected of causing co-infections in WNV-infected
birds. The EWS detected overall 8 HEDV-positive and 15 UMAV-positive birds in small sets of
samples, and UMAV could be propagated in a mosquito cell culture Future studies are necessary
to investigate the pathogenicity of these viruses and their role in the health of wild and captive
birds.
In conclusion, this study provided a proof-of-concept that the developed unified and
generic pipeline is an effective tool for outbreak investigation and pathogen discovery using the
same generic HTS datasets derived from outbreak and surveillance samples. Therefore, this
thesis recommends incorporating the unified pipeline in the key response to viral outbreaks to
enhance outbreak preparedness and response.
Orthohantaviruses are rodent-borne pathogens distributed all over the world, which do not cause visible disease in their reservoir host. Puumala orthohantavirus (PUUV) causes most human hantavirus disease cases in Europe and is transmitted by the bank vole (Clethrionomys glareolus). Hantaviruses have a tri-segmented genome consisting of the large (L) segment, coding for the RNA-dependent RNA polymerase (RdRP), the medium (M) segment, encoding the glycoproteins, and the small (S) segment. The S-segment contains two major overlapping open reading frames (ORF) coding for the nucleocapsid (N) protein and a non-structural (NSs) protein, a putative type I interferon (IFN-I) antagonist. To date, pathogenesis and reservoir host adaptation of hantaviruses are poorly understood due to missing adequate cell culture and animal models.
In contrast to previous studies, in this work, data from spring and summer 2019 indicated a high vole abundance, a high PUUV prevalence in voles and high human incidence for some endemic regions in Germany, but elsewhere values were low to moderate. Regional and local human health institutions need to be aware about the heterogeneous distribution of human PUUV infection risk.
For a better understanding of virus-host associations, two novel cell lines from bank voles and common voles each were generated and their susceptibility and replication capacities for a variety of zoonotic and non-zoonotic viruses were analyzed. The PUUV strain Vranica/Hällnäs showed efficient replication in a new bank vole kidney cell line, but not in four other cell lines of bank and common voles. Vice versa, Tula orthohantavirus (TULV) replicated in the kidney cell line of common voles, but was hampered in its replication in other cell lines. Several viruses, such as Cowpox virus, Vaccinia virus, Rift Valley fever virus, and Encephalomyocarditis virus 1 replicated in all four cell lines. West Nile virus, Usutu virus, Sindbis virus and Tick-borne encephalitis virus replicated only in a part of the cell lines. These results indicate a tissue or species specific tropism for many of the tested viruses and the potential value of vole cell lines to address such questions in detail.
Using one of these new cell lines, the first German PUUV strains were isolated from bank voles caught in the highly endemic region around Osnabrück. Complete genomes were determined by target-enrichment-mediated high-throughput sequencing from original lung tissue, after isolation and after additional passaging in VeroE6 cells and a bank vole-derived kidney cell line. Different single amino acid substitutions were observed in the RdRP of the two stable PUUV isolates. The PUUV strain isolated on VeroE6 cells showed a lower titer when propagated on bank vole cells compared to VeroE6 cells. Additionally, glycoprotein precursor (GPC)-derived virus-like particles of a German PUUV strain from the same region allowed the generation of monoclonal antibodies that reacted with the isolated PUUV strains.
To investigate the role of PUUV and other vole-borne hantavirus NSs proteins, the evolution of the NSs and N encoding sequences was investigated by a field study in bank voles and the NSs sequences were characterized in vitro for their inhibitory effect on the human interferon-β promoter. Analysis of blood and lung samples of 851 bank voles trapped during 2010-2014 in Baden-Wuerttemberg and North Rhine-Westphalia resulted in detection of 27.8% PUUV-specific antibody positive bank voles, whereas in 22.3% PUUV-specific RNA was detected. In the hantavirus outbreak years 2010 and 2012 PUUV prevalence in bank voles was higher compared to 2011, 2013 and 2014. Sequences of the S segment of all positive bank voles showed amino acid and nucleotide sequence types of the NSs-ORF with temporal and/or local variation, whereas the N-ORF was highly conserved. One sequence type persisted over the whole observation period in both regions. The NSs coding sequence was highly divergent among regional bank vole populations in the outbreak year 2012.
Transfection experiments resulted in the detection of different products of the NSs-ORF of PUUV, TULV, Prospect Hill and Khabarovsk orthohantaviruses, due to translation initiation at different methionine codons along the coding sequence. Using luciferase reporter assays, the NSs proteins of PUUV, TULV, Prospect Hill and Khabarovsk orthohantaviruses showed inhibition of IFN-I induction of up to 70%, whereas Sin Nombre and Andes orthohantavirus NSs proteins showed a reduced effect compared to the other NSs proteins. The first 20 amino acids of the N-terminal region of PUUV NSs were found to be crucial for IFN-I promoter inhibition.
In conclusion, the newly established cell lines, antibodies, reporter assays and PUUV isolates are highly valuable tools for future hantavirus research. The activity of PUUV NSs protein in human cells contributes to our understanding of virus-host interactions and highlights the importance of corresponding future reservoir host studies. Hantavirus surveillance studies showed the necessity for timely information of the potential human PUUV infection risk to public health institutions in endemic areas to initiate appropriate actions.
Infections with bacterial pathogens are a major cause of morbidity and mortality
worldwide. Furthermore, the extensive use of antibiotics increased the frequency of infections with drug-resistant pathogens. Streptococcus pneumoniae, a major cause of
bacterial pneumonia, is among the pathogens that often show resistances. As an
additional side effect, the use of antibiotics can disrupt the patient’s intestinal microbiome, allowing Clostridioides difficile to cause severe, recurring and hard-to-treat
colitis. Hence, new antimicrobials are needed to combat infections caused by these
pathogens. A promising approach is the usage of antimicrobial peptides (AMPs), defense
molecules produced by organisms from all domains of life. AMPs can specifically perforate
bacterial membranes and stimulate the overall immune response of the host.
In this work, the proteomic adaptations of S. pneumoniae to the human antimicrobial
peptides LL-37 and hBD3 were assessed by high-resolution mass spectrometry and
compared to general membrane stress, in order to evaluate the specificity of the bacterial
reactions. Furthermore, C. difficile was challenged with the Lactococcus lactis-derived
AMP nisin, and the proteomic alterations were examined. In essence, application of LL-37
and hBD3 changed the abundance of pneumococcal proteins involved in membrane
transport, including a putative AMP transporter, a protease, virulence proteins and
genetic regulators. Moreover, a challenge with LL-37 caused an increase of proteins
involved in cell surface modifications that alter the bacterial membrane charge and repel cationic molecules such as LL-37. In support of this, mutants unable to express these
proteins were more sensitive to LL-37. In contrast, general membrane stress, induced by
the application of cationic detergents, produced a diverse proteomic adjustment, though the same two-component regulatory system was activated. In C. difficile, levels of flagella proteins were significantly increased shortly after treatment with nisin, being in
accordance with subsequent electron microscopy data and pointing at a role of these
proteins in adaptation to nisin. Interestingly, a flagella-overexpressing mutant showed an
enhanced resistance towards nisin, independent of bacterial motility.
Taken together, the bacterial pathogens under investigation seem to possess
mechanisms to reduce the effect of AMPs on their physiology, a finding that should be
considered developing drugs based on AMPs. Although AMPs exhibit membrane
perturbations as a common mechanism of action, bacterial adaptation to AMPs appear
multifactorial and dependent on the exact pathogen observed and AMP used.
Bisherige Analysen von RABV-Pathogenitätsdeterminanten wurden mit laboradaptierten, teils attenuierten Viren durchgeführt. Es ist unklar, ob bisher untersuchte Faktoren auch für hoch virulente RABV-Feldviren relevant sind. Der hier durchgeführte systematische Vergleich von Feldviren und Laborstämmen im infizierten Tier konnte Unterschiede hinsichtlich der Fähigkeit immunkompetente Neuroglia des ZNS zu infizieren als mögliche Pathogenitätsdeterminante aufzeigen. Darüber hinaus wurden erstmals SZ-Neuroglia peripherer Nerven als Zielzellen für die RABV-Infektion identifiziert.
Für die Analyse von RABV-infizierten Geweben wurde ein modernes 3D Imaging-Verfahren angewandt. Gehirne aus experimentell infizierten Mäusen und Frettchen wurden wie in Veröffentlichung 1 beschrieben immunfluoreszenz-gefärbt, optisch geklärt und hochauflösend mit einem konfokalen Laserscan Mikroskop untersucht. RABV N und P Protein konnten dreidimensional in räumlicher Umgebung zu zellulären Strukturen des Wirtes visualisiert werden. Diese Untersuchung bewies die besondere Eignung des Verfahrens zur Identifizierung vereinzelter Zielstrukturen und wurde für nachfolgende systematische Analysen im ZNS und PNS verwendet.
Der RABV-Zelltropismus wurde als vermutlich wichtige Pathogenitätsdeterminante in Veröffentlichung 2 untersucht. RABV Feldviren vom Hund (rRABV Dog), Fuchs (rRABV Fox) und Waschbär (rRABV Rac) konnten im Vergleich zu den laboradaptierten Viren (rCVS-11, SAD L16 und ERA) nicht-neuronale Zellen im ZNS wie Astroglia produktiv infizieren. Der Anteil infizierter Astrozyten ist mit 7-17 % nach i.m. Inokulation vergleichbar mit dem der Neuronen (7-19 %). Interessanterweise wurde eine Inokulationsroutenabhängige Infektion von Astrozyten mit dem moderat virulenten Laborstamm rCVS-11 beobachtet. Diese systematische und quantitative Analyse des RABV-Astrozyten- und Neuronentropismus zeigt, dass mit abnehmender Virulenz die Fähigkeit der Viren produktiv in Astroglia im ZNS zu replizieren abnimmt. Die Fähigkeit eine produktive Infektion in Astrozyten auszubilden, scheint demnach ein grundlegender Unterschied zwischen Feldviren und weniger virulenten Laborstämmen zu sein.
Weiterführend wurde in Veröffentlichung 3 die Virusausbreitung vom ZNS in periphere Nerven untersucht. Hinterbeine, Wirbelsäule inklusive Rückenmark, Gehirn und weitere Kopfbereiche experimentell infizierter Mäuse wurden mittels Lichtblatt- und konfokaler Laserscanmikroskopie analysiert. Zum Ersten Mal konnte eine RABV-Infektion peripherer Neuroglia dargestellt werden. Eine produktive Infektion immunkompetenter SZ im PNS ist also möglicherweise, genauso wie die Infektion von Astrozyten im ZNS, entscheidend für die RABV-Neuropathogenese. Die Detektion von RABV-Antigen im Hinterbein nach i.c. Inokulation beweist eine anterograde axonale Virusausbreitung vom ZNS in periphere Nerven. Interessanterweise konnte das Virus auch in Bereichen des Nasopharynx und des Zungenepithels nachgewiesen werden, worüber möglicherweise zusätzlich zur Speicheldrüse Virus in den Nasenrachenraum ausgeschieden wird. Zusammenfassend konnten mit dieser Arbeit neue Einblicke hinsichtlich des Zelltropismus und der Ausbreitung von RABV in vivo im Modellorganismus Maus gewonnen werden. Die Fähigkeit der untersuchten hoch virulenten Feldviren nicht-neuronale, immunkompetente Neuroglia des ZNS und PNS zu infizieren unterscheidet diese von den weniger virulenten bzw. apathogenen Virusstämmen und könnte ein entscheidender Faktor bei der Ausbildung einer Tollwut-Enzephalitis darstellen.
More than half of the infectious diseases in humans are caused by zoonotic pathogens or pathogens of animal origin that were transmitted to humans a long time ago. Two important rodent-associated zoonotic pathogens are hantaviruses and human-pathogenic Leptospira spp. Both pathogens induce lifelong infection in the rodent hosts that shed the pathogen. Infection with these zoonotic pathogens in humans can cause clinical symptoms. Since some rodents, like the common vole (Microtus arvalis) and the bank vole (Clethrionomys glareolus syn. Myodes glareolus), have cyclic mass reproduction, this can result in years of population outbreaks in an increased number of disease cases in humans. This was found to be the case with the leptospirosis outbreaks in Germany and tularemia outbreaks in Spain, which were traced back to increased common vole density, as well as with the hantavirus disease outbreaks in several European countries, which were associated with bank vole population outbreaks.
The aim of this work was to define the distribution and prevalence of different hantaviruses and leptospires as well as their coinfection in different European rodents, with a focus on voles from the genus Microtus and the identification of factors that affect the pathogen prevalence in rodent hosts. Therefore, common voles, bank voles, striped field mice (Apodemus agrarius) and other rodents were screened by molecular methods for the presence and prevalence of Leptospira spp. and different hantaviruses. Additionally, in selected studies, the presence of anti-hantavirus antibodies was screened by enzyme-linked immunosorbent assay (ELISA) using recombinant hantavirus-nucleocapsid proteins. The prevalence of hantavirus, Leptospira spp. and double-infections with both pathogens was analyzed using individual and population-based factors. Small mammals from four different European countries, Spain in the West, Germany and Austria in Central and Lithuania in Northeastern Europe, were included in the studies.
With the molecular screenings, two new hantavirus strains were detected in continental Europe and were named Traemmersee hantavirus (TRAV) and Rusne hantavirus (RUSV) after the trapping locations in Germany and Lithuania, respectively. TRAV was detected in a field vole (Microtus agrestis) from the federal state of Brandenburg, Germany, while RUSV was detected in root voles (Microtus oeconomus) from Lithuania. Phylogenetic analysis of both hantaviruses indicates their close relation to Tatenale hantavirus and Kielder hantavirus, which were discovered in field voles in Great Britain. A pairwise evolutionary distance (PED) analysis showed that all four hantaviruses belong to the same hantavirus species, for which the putative name “Tatenale orthohantavirus” was proposed. Additionally, a recombinant RUSV antigen was generated and used successfully in ELISA for the detection of RUSV-specific antibodies and for the analysis of the cross-reactivity of monoclonal and polyclonal antibodies.
In Germany, Tula orthohantavirus (TULV) was foremost detected in common voles in Thuringia and Brandenburg but was also detected in field voles in Brandenburg. Puumala orthohantavirus (PUUV) was detected in Thuringia at the virus distribution border, but sequences differed strongly from known sequences from another neighboring trapping location. While in Austria Dobrava-Belgrade orthohantavirus (DOBV), genotype Kurkino, was detected for the first time in striped field mice, no hantavirus RNA was detected in common voles from Spain. The cause of this absence in the Iberian common vole population might be its long-term isolation from the common vole populations more to the east. The TULV prevalence in Germany in this study was dependent on the season and on the prior growth of the reservoir population. An individual factor that affected the hantavirus prevalence, was the increasing age of the common vole.
Leptospira spp.-DNA was detected in common voles from Spain and Germany, as well as in one striped field mouse from Austria. Except for the two detections of L. borgpetersenii in Spain, which were probably the result of spillover infections, only the genomospecies L. kirschneri was detected in common voles from Spain and Germany. The high prevalence of Leptospira spp., as well as the detection of only one genomospecies, confirm that L. kirschneri is the genomospecies for which the common vole is the main reservoir. Important factors for the Leptospira spp. prevalence were found to be, in addition to temperature and rainfall, the season and the preceding common vole density. Like the case with hantavirus, the age of the vole was found to be an influencing factor.
In Germany, coinfections of TULV and Leptospira spp. were detected. These were associated with high common vole density and increased with the age of the common vole. Furthermore, the incidence of coinfections seems to be impacted more by the Leptospira spp. than by the hantavirus prevalence.
As part of this thesis, TULV and PUUV were detected in previously untested regions in Germany, DOBV was detected for the first time in Austria and the distribution range of the putative species “Tatenale orthohantavirus” was extended to continental Europe for the first time with detection in two countries. Screenings in Spain indicate that certain common vole populations can be free from TULV infection. Furthermore, leptospires were detected in rodents from Spain, Germany and Austria. It was verified that certain Leptospira genomospecies are host-specific. Factors that influence the prevalence of infection or coinfection by hantaviruses and leptospires were determined.
The origin and hosts associated with the Tatenale orthohantavirus should be clarified in further studies including the field vole and the root vole as well as other members of the genus Microtus in Europe and Asia. The development of a RUSV-antigen-based ELISA will enable future screening in humans and therefore might provide information about the human pathogenicity of this pathogen. For final confirmation of the zoonotic potential, isolation of the virus and development of a focus reduction neutralization test are necessary. The expansion of the striped field mouse to Austria and the detectable carryover of DOBV associated with this implies that further screening studies to more precisely characterize the distribution of DOBV (and other pathogens) are needed. The studies of DOBV spread in Austria as well as PUUV spread in Germany could help to better understand the emergence of zoonotic pathogens in new regions. The here described hantavirus-Leptospira spp. and Neoehrlichia mikurensis-Bartonella spp. coinfections should be further analyzed to characterize the interactions of the pathogens in the context of a microbiome and their influence on epidemiological aspects of the involved pathogens. The here identified individual and population-based impact factors for the TULV and Leptospira spp. prevalence should support the development and optimization of prediction models.
Lyssaviruses, the causative agents of rabies, are a long-known threat for animals and humans. To date, terrestrial rabies still accounts for tens of thousands of human deaths annually, notwithstanding ambitious vaccination campaigns targeting susceptible dog and wildlife populations that act as reservoirs for the prototypic rabies virus. Moreover, the continuing discovery of newly emerging virus species in hitherto unconcerned chiropteran hosts and geographic regions drive the expansion of the Lyssavirus genus by unveiling its actual variety, host range and distribution.In this work, the genetic diversity of three distinct lyssaviruses, namely EBLV-1, KBLV and RABV, was elucidated by in-depth genomic analyses to provide further insight into lyssavirus evolution. The generation of full-genome sequences from primarily bat-associated Danish EBLV-1 samples significantly increased the number of available Danish EBLV-1 genome sequences while phylogenetic and phylogeographic analysis revealed a stronger phylogeographic structure for the cluster A1 of the sublineage EBLV-1a than it was postulated in previous studies. In addition, the acquisition of a nearly complete genome sequence for the Kotalahti bat lyssavirus provided the basis for the classification of this putative new lyssavirus species as a recognized member of the genus. Furthermore, phylogenetic analysis revealed the affiliation of KBLV to a group of Myotis-associated lyssaviruses giving a deeper insight into the shared evolutionary history of lyssaviruses co-evolving with particular bat species. Moreover, a deep-sequencing approach was utilized to assess the high genetic diversity of vaccine virus populations, uncovering three independent patterns of single nucleotide variants (SNVs) that became selected in ERA-related vaccine-induced cases. However, no apparent influence of the genetic diversity of vaccine viruses on microevolutionary processes like a potential reversion to virulence or a species-specific adaptation of the vaccine virus strains could be detected, leaving the question for the cause of rabies induction in the affected animals unanswered. Lastly, the successful implementation of a hybridization capturing system for the generation of full-genome sequences and deep-sequencing variant analyses of RABV and KBLV samples was demonstrated for a diagnostic bait set, highlighting the versatility and consistency of this approach to assess the genetic spectrum of known and novel lyssavirus species while setting the basis for its application and optimization in upcoming projects.In conclusion, as shown by the studies in this work, the investigation of lyssavirus genomes at the sub-consensus, full-genome and population level remains crucial to assess the complexity of lyssavirus evolution, as it provides an indispensable source of information to cover the diversity of the genus and understand evolutionary dynamics on a long-term and microevolutionary scale.
Phospholipide wie Phosphatidylinositol und Phosphatidylcholin sind essenzielle Bestandteile aller biologischen Membranen und für deren Integrität und Funktion unerlässlich. Sind Inositol und Cholin (IC) im Medium vorhanden, ist die Hefe Saccharomyces cerevisiae in der Lage, diese aufzunehmen und zu verarbeiten. Unter Mangelbedingungen können diese Stoffe von der Zelle selbst synthetisiert werden. Daher ist es sinnvoll, die Phospholipid¬biosynthese-Gene differenziell zu exprimieren, was auf der Ebene der Transkriptions¬initiation geschieht. Bei IC-Mangel werden die Gene (z. B. das Inositol-3-Phosphat Synthase Gen INO1) durch Bindung des heterodimeren Aktivatorkomplexes Ino2/Ino4 an das Promotorelement ICRE („inositol/ choline responsive element“) aktiviert, um die Biosynthese zu gewährleisten. Sowohl Ino2 als auch Ino4 sind für die ICRE-Bindung nötig, während die transkriptionale Aktivierung nur durch Ino2 mit Hilfe zweier Transkriptionsaktivierungsdomänen TAD1 und TAD2 vermittelt wird. Ist dagegen ausreichend IC vorhanden, werden die Gene reprimiert, indem der Repressor Opi1 an den Aktivator Ino2 bindet, sodass es zu einer Konformationsänderung kommt und eine Dimerisierung mit Ino4 nicht mehr möglich ist.
Um eine erfolgreiche Transkriptionsinitiation zu gewährleisten, bilden neben der RNA-Polymerase II eine Reihe genereller Transkriptionsfaktoren (A, B, D, E, F und H) sowie der Mediatorkomplex im Promotorbereich der Zielgene den sog. Präinitiationskomplex (PIC). Die von diesen basalen Faktoren gewährleistete geringe Grundexpression kann von Aktivatorproteinen, die an positiv-regulatorische Elemente („upstream activation site“, UAS) binden, deutlich verstärkt werden. Hierzu nutzen Aktivatorproteine verschiedene Mechanismen, zu denen die Auflockerung der Chromatinstruktur durch Histonmodifikationskomplexe wie SAGA oder Chromatinremodellierungskomplexe wie SWI/SNF, die bessere Bindung der Transkriptionsfaktoren am Basalpromotorbereich oder die Beschleunigung des Übergangs vom geschlossenen zum offenen PIC gehören.
Im Verlauf dieser Arbeit konnten zahlreiche Interaktionen zwischen dem Aktivator Ino2 und Faktoren der Transkriptionsmaschinerie nachgewiesen werden, die vermutlich die Häufigkeit der Trans¬kriptions-initiation beeinflussen. Einige der Untereinheiten des Transkriptionsfaktors TFIID interagie¬ren mit Ino2. Ein Schwerpunkt dieser Arbeit lag auf der Charakterisierung der Interaktion der Ino2-TAD1 mit Taf1 und Taf12. Der Austausch der Aminosäuren Asparaginsäure-20 und Phenyl¬alanin-21 in Ino2 führte zu einem Interaktionsausfall mit beiden Tafs. In Taf1 konnten zwei basisch-hydro¬phobe Aminosäure-Bereiche (K206 Y207 und L208 L209 K210) innerhalb der minimalen Aktivator¬binde¬domäne 2 (ABD2) identifiziert werden, die kritisch für den Kontakt zum Aktivator sind. Es konnte ferner gezeigt werden, dass basische und hydrophobe Aminosäuren in Kombination für die Bindung an den Aktivator verantwortlich sind und dass der Austausch gegen Alanin (KY-AA) zu einem Abfall der Expression des INO1-Gens auf 44% führt. Darüber hinaus konnte der Bromo¬domänen¬faktor Bdf1 als Interaktionspartner von Ino2 identifiziert werden. Bdf1 vervollständigt Hefe-Taf1, während Säuger-Taf1 selbst Bromodomänen zur Erkennung von Histonacetylierungen beinhaltet. Innerhalb der Taf12-Minimaldomäne sind die Aminosäuren K150 L151 R175 und L176 wesentlich für die Bindung an Ino2. Eine Teildeletion von Taf12, die unter anderem den Verlust dieser Aminosäuren zur Folge hat, führt zu einer auf 76% reduzierten INO1-Expression.
Ein weiterer Transkriptions¬faktor, der von Ino2 kontaktiert wird, ist TFIIA mit seinen Untereinheiten Toa1 und Toa2. Die Proteine kontaktieren beide TADs des Aktivators, allerdings konnten innerhalb der minimalen Interaktionsdomänen der Toa-Proteine keine für diese Interaktion verantwortliche Aminosäuren identifiziert werden. Veränderungen der Toa1-Sequenz hatten keinen phänotypischen Einfluss auf die Phospholipidbiosynthese, allerdings führten einige Veränderungen (RKRK-Motiv im AS-Bereich 253-259) zu letalen Folgen für das Wachstum der Zellen, weil die Bildung des TFIIA-TBP-TATA-Komplexes beeinträchtigt ist. Wahrscheinlich hat die Interaktion zwischen Ino2 und TFIIA eine verstärkende Wirkung auf die Transkriptionsinitiation der Phospholipidbiosynthese-Gene, indem die Interaktion zwischen TFIIA und TFIID stabilisiert wird und TFIIA die interaktive Oberfläche am Promotor für Interaktionen mit anderen Proteinen vergrößert.
Die Verschiebung der Nucleosomen in Promotorbereichen durch Chromatinremodellierungs¬kompexe wie SWI/SNF ist ein weiterer Mechanismus der Transkriptionsaktivierung. In früheren Arbeiten wurde bereits die Interaktion zwischen Ino2, Aro80 bzw. Gal4 und der SWI/SNF ATPase-Untereinheit Swi2 beschrieben. Im Zuge dieser Arbeit konnte eine minimale Interaktionsdomäne im AS-Bereich 238-307 kartiert werden. Essenzielle Aminosäuren für die Bindung an Ino2 und andere Aktivatoren konnten nicht identifiziert werden.
Sug1 und Sug2 sind ATPasen der regulatorischen 19S-Untereinheit des 26S Proteasoms. Neben der Degradation fehlgefalteter polyubiquitinierter Proteine haben sie auch eine nicht-proteolytische Bedeutung für die Transkriptionsinitiation. Bekannt ist, dass proteasomale ATPasen an aktiven Promotoren zu finden sind und mit Aktivator¬proteinen (z. B. Gal4) interagieren können. Die vorlie¬gende Arbeit zeigt, dass auch Ino2 von Sug1 und Sug2 kontaktiert wird. Möglicherweise dienen sie am INO1-Promotor als Stabilisatoren und Vermittler zwischen Ino2 und der Transkriptionsmaschi¬nerie und erleichtern den Übergang des Präinitiationskomplexes in den Elongationskomplex.
Unter reprimierenden Bedingungen bindet Opi1 an Ino2 und rekrutiert die Corepressorkomplexe Sin3 und Cyc8/Tup1, die ihrerseits Histondeacetylasen in Promotornähe bringen und die Transkrip¬tion durch lokale Chromatinverfestigung reprimieren. Frühere Arbeiten hatten gezeigt, dass die Corepressoren auch mit Ino2 und weiteren Aktivatoren (Hac1 und Pho4) interagieren und dass sie in Abhängigkeit von Ino2, nicht aber von Opi1, am INO1-Promotor vorliegen. In dieser Arbeit wurde die Interaktion zwischen Ino2 und Sin3 bzw. Cyc8 charakterisiert. Sin3 und Cyc8 kontaktieren einen Bereich des Aktivators, der die TAD2 und die RID (Repressorinteraktionsdomäne) enthält. Es war bekannt, dass die Aminosäuren Phenylalanin-130, Leucin-131 und Asparaginsäure-132 essenziell für die Interaktion mit Opi1 sind. In dieser Arbeit wurde gezeigt, dass deren Austausch gegen Alanin auch einen Interaktionsverlust mit Cyc8 und Sin3 bewirkt. Darüber hinaus konnte gezeigt werden, dass diese FLD-AAA-Mutation zu einer praktisch konstitutiven Expression des INO1-Gens führt, allerdings auf niedrigerem Niveau als im Fall dereprimierter Zellen mit einem Wildtyp Ino2. In Hac1 und Pho4 konnten Aminosäuren mit vergleichbarer Bedeutung für die Corepressorbindung nicht identifiziert werden. Offenbar können die Corepressoren je nach physiologischer Situation in der Zelle positiv oder negativ auf die Transkriptionsinitiation wirken.
Viral diseases are a threat to bacteria and enormous animals alike. Vaccines are available against several viruses. However, for some viruses, like ASFV, we still lack vaccines, while for others, like IAV, they are not as effective as we need them to be. To a large extent, this is because we do not fully understand the mechanisms conferring antiviral immunity. To improve our understanding of antiviral immunity, we used a model species that is in many immunological aspects closer to humans than the widely used laboratory mice, pigs. In this thesis, pigs were investigated as a potential biomedical model species for viral respiratory infections in humans and as a natural host for viral infections. Both approaches provide valuable insights into aspects of porcine immunology that can either be used as the foundation for translational research or for the design of targeted therapeutics and vaccines for pigs.
Insights into fundamental characteristics of the porcine immune system form the basis for translational studies. Paper I pioneered a detailed characterization of porcine iNKT cells. To make pigs and porcine iNKT cells more available for scientific investigations, we established multicolor flow cytometry analysis platforms that allow for a more detailed investigation of these cells than previously possible. We found porcine iNKT cells circulating in peripheral blood to be a rare population among CD3+ lymphocytes that displays a pre-activated effector state and can be divided into at least three functional subsets. Upon antigenic activation, they proliferated rapidly, secreted pro-inflammatory cytokines, and exerted cytotoxicity. Moreover, we provided first evidence for a role of iNKT cells in porcine IAV and ASFV infections, which we investigated in more detail in paper IV. Central characteristics, i.e., phenotype and functional properties, exhibit a high degree of similarity between humans and pigs. Moreover, differences between human and murine iNKT cells are more pronounced than between humans and pigs.
Based on the results obtained in paper II, the established biomedical model could be used for further studies of infectious respiratory diseases. IAV infections pave the way for secondary co-infections with increased morbidity and lethality. These bactoviral co-infections are a threat to both pigs and humans. The shared susceptibility as well as homologies on the physiological and immunological level make pigs exceptionally suitable animal models for studies of these infections. Paper I and II can also be interpreted under translational aspects. Activation of iNKT cells in porcine vaccination studies showed promising results. Based on these and our findings, this might be a suitable approach for humans as well. Along with other studies, our results suggest that pigs might be a well-suited large animal model for research in infectious diseases. This is true especially for respiratory infections, such as seasonal IAV infections, for which pigs are natural hosts and contribute to viral spread and emergence as “mixing vessels”, which can result in pandemic strains like H1N1pdm09. We could show that porcine iNKT cells as well as the antiviral responses of cTC against H1N1pdm09 in pigs are comparable to human cells and processes. The increased implementation of pigs in basic and applied research might enable an improved translation of scientific knowledge to human and veterinary medicine.
In two further studies, papers III and IV, we investigated T-cell responses during a viral infection, ASF, for which pigs are the only natural hosts. Immune responses were similar after highly and moderately virulent ASFV infection in domestic pigs and wild boar, respectively. However, they differed between both species. Antiviral immunity in domestic pigs was predominantly exerted by αβ T cells, CD8α+ and DP αβ T cells, while the response in wild boar was dominated by γδ T cells, mainly CD8α+ effector cells. Since wild boar show a higher disease severity and lethality, even during infection with moderately virulent ASFV “Estonia2014”, a shift to γδ T cells seems to be detrimental. In contrast, domestic pigs survive infections with moderately virulent ASFV “Estonia2014”, which indicates that CD8α+ or DP αβ T cells confer protection at least in infections with non-highly virulent ASFV strains. Interestingly, in paper V we found higher and prolonged inflammation in domestic pigs, correlating with increased T-cell influx. However, histopathological analyses revealed no direct explanation for the differences in disease progression and lethality in domestic pigs and wild boar. These findings require further studies to elucidate the underlying mechanisms.
The lack of basic data about immunological differences between domestic pigs and wild boar hampers attempts to understand immunity against ASFV. We found differences between both suid subspecies already at steady state and even more prominent during ASFV infections in papers III-V. Most apparently, T-cell responses in wild boar were heavily biased towards γδ T cells, while immune responses in domestic pigs were based on αβ T cells. However, information about even basic characteristics, like the composition, phenotypes, and functional qualities of wild boar’s immune system, is missing. Therefore, essential baseline data must be obtained in order to adequately assess changes in future studies.
Analyses like these reveal major advantages of pigs as a biomedical model. On the one hand, similar to conventional model species, researchers can investigate every tissue at any desired time. Tissue from human patients is often scarce or not at all available, so models that can be investigated at specific times after infection are needed. On the other hand, results obtained in pigs are more comparable to humans than data from murine studies. Moreover, pigs are susceptible to similar pathogens as humans and experimental infections can be investigated without the need for major genetic manipulations. However, there are also limitations of the porcine model system. Analysis tools are not as advanced as they are for mice, especially in terms of availability of mAbs or genetically modified organisms. Still, given the major advantages that become more and more obvious, efforts should be made to make pigs more applicable for basic and translational research. In addition, findings derived from pigs can be used for the species itself. Pigs are a major livestock species and new treatments, or vaccines could also be used for them. Therefore, this research could eventually also improve animal welfare.
In summary, the presented thesis significantly enhanced our knowledge of porcine immune processes for cTC in general and iNKT cells in particular. Results were obtained both at steady state and in the context of IAV and ASFV infections, and thus, made pigs more available as a model for future research. The use of multicolor flow cytometry provided a broad overview of the ongoing immune reactions and enables further, more wide-ranging studies that can also address open questions in even more complex infection scenarios.
Der Erreger des Q-Fiebers ist C. burnetii, ein zoonotisches intrazelluläres Bakterium. Die Gram-negativen Coxiellen kommen in zwei verschiedenen antigenen Lipopolysaccharid (LPS)-Formen vor: als virulente Ph I-LPS- und/oder avirulente Ph II-LPS-Bakterien. C. burnetii wird durch Kontakt mit infizierten Tieren sowie infektiösen Stäuben übertragen. Akute fiebrige Infektionen können beim Menschen im weiteren Verlauf eine Pneumonie oder Hepatitis auslösen. Zu einem geringen Prozentsatz entstehen chronische Infektionen mit persistierenden Coxiellen. Eine C. burnetii-Infektion bewirkt sowohl eine humorale als auch zelluläre Immunantwort. Neben Monozyten und Makrophagen dienen auch dendritische Zellen (DCs) den Coxiellen als geeignete Wirtszellen. DCs gehören zu den Immunzellen der first-line-of-defense des angeborenen Immunsystems und treten während einer Coxiellen-Infektion ebenso wie die mit ihnen kooperierenden natürlichen Killerzellen (NK-Zellen) früh mit dem aufgenommenen bakteriellen Pathogen in Kontakt. Durch Antigenpräsentation infizierter DCs wird die für die anti-Coxiellen Abwehr maßgebliche T-Zell-Immunität initialisiert und die nachgeschaltete Immunantwort funktional ausgerichtet.
Trotz dieser zentralen Immunfunktion sind die zellulären Vorgänge von DCs während einer C. burnetii-Infektion, insbesondere mit Blick auf die zelluläre Selbstverteidigung gegenüber den vermutlich initial auftretenden Ph II-LPS-Varianten, nicht ausreichend verstanden. Zudem ist bisher nicht hinreichend geklärt, welchen Einfluss FN-γ, das von aktivierten NK-Zellen produziert wird, sowie die Sauerstoffumgebung auf die zelluläre Abwehr infizierter APCs nimmt.
Das Forschungsziel dieser Promotionsarbeit war es daher, einen detaillierten Einblick in die Prozesse der Coxiellen-Infektionen von DCs und NK-Zellen zu erhalten und hierbei insbesondere die IFN-γ-Wirkung auf die DC-Pathogen-Wechselwirkung sowohl unter norm- als auch hypoxischen Bedingungen zu untersuchen.
Die im ersten Teil der Promotionsarbeit durchgeführten zellbiologischen, immunologischen und proteinbiochemischen Analysen im murinen Zellsystem belegen eine pathogenausgelöste Subversion der funktionalen Aktivierung/Induktion der MHC I-Antigenpräsentation Coxiellen-infizierter DCs. Die infektionsbedingte Beeinträchtigung der MHC-Antigenpräsentation infizierter DCs lässt sich in direkter Weise auf einen autokrinen Suppressionseffekt des αVβ8-Integrin-aktivierten TGF-β und nicht auf die subversive Wirkung von Coxiellen-LPS als Virulenzfaktor zurückführen. Untersuchungen im Zusammenhang mit IFN-γ zeigen, dass dieses Zytokin in infizierten DCs eine Wiederherstellung der MHC I-Induktion und -Oberflächenexpression bewirkt, welche mit einer funktionalen Prozessierung und MHC-Präsentation pathogener Peptidantigene verbunden ist. Weitere Studien belegen zudem, dass IFN-γ-behandelte DCs in der Lage sind, die Etablierung/Vermehrung intrazellulärer Coxiellen negativ zu beeinflussen. Die durchgeführten siRNA- und CRISPR/Cas9-Experimente zeigen, dass die zelluläre Selbstverteidigung infizierter DCs maßgeblich durch das IFN-γ-induzierbare iNOS/NO-System vermittelt wird. Als reaktives Stickstoffradikal scheint Stickstoffmonoxid (NO) sowohl Komponenten der bakteriellen Elektronentransportkette als auch die autophagische Ausbildung und Integrität parasitophorer Vakuolen zu beeinträchtigen. Parallel hierzu schützen sich infizierte DCs über einen metabolischen Wechsel zur aeroben Glykolyse vor mitotoxischer NO-Wirkung und sichern so während der intrazellulären Coxiellen-Eliminierung ihr eigenes Überleben.
Weitere Untersuchungen dieser Arbeit belegen zudem, dass auch C. burnetii zu einer entsprechenden Gegenwehr fähig ist. Um der NO-vermittelten Abwehr infizierter DCs entgegenzuwirken, induzieren Coxiellen zur Minderung antibakterieller Radikal-Effekte ihre Cytochrom bd-, Katalase- und SOD-Expression. Infektionsstudien mit T4SS-defekten Coxiellen weisen ferner darauf hin, dass das bakterielle Sekretionssystem vermutlich eine wichtige Rolle bei der Wirksamkeit der NO-vermittelten Abwehr infizierter DCs spielt, da sich Coxiellen ohne intaktes T4SS offensichtlich dem negativen NO-Einfluss entziehen und/oder keine entsprechenden Angriffsziele für NO bieten. Studien C. burnetii-infizierter Makrophagen bestätigen, dass das iNOS/NO-System eine essenzielle antibakterielle Selbstverteidigung von APCs darstellt. So zeigen auch Makrophagen eine deutliche Beeinträchtigung intrazellulärer Coxiellen-Vermehrung unter iNOS-vermittelter NO-Synthese. Die im weiteren Verlauf der Arbeit untersuchten norm- und hypoxischen Infektionsmodelle infizierter DCs lassen vermuten, dass hypoxische Kulturbedingungen die Coxiellen dazu veranlassen, ein sporenähnliches Stadium ohne produktive Vakuolenbildung auszubilden. Diese hypoxische Überlebensform intrazellulärer Coxiellen zeichnet sich durch IFN-γ-Resistenz, eine durch modifizierte Genexpression optimierte Sauerstoffverwertung und Radikalentgiftung sowie die Erhaltung ihrer Infektiosität aus. Dies deutet darauf hin, dass Hypoxie den intrazellulären Coxiellen weitere Möglichkeiten zur effizienten Immunevasion eröffnet, die einen unentdeckten Bakterienverbleib innerhalb infizierter Wirtszellen begünstigt und so vermutlich chronische C. burnetii-Infektionen fördert.
Für die Synthese und Freisetzung des APC-stimulierenden IFN-γ sind im Zuge angeborener Immunität vor allem die mit DCs kooperierenden NK-Zellen verantwortlich. Die im zweiten Teil dieser Promotionsarbeit durchgeführten Studien zur Charakterisierung der Interaktion zwischen NK-Zellen und Coxiellen belegen, dass NK-Zellen von C. burnetii infiziert werden, sie jedoch die Etablierung und Replikation internalisierter Bakterien durch Ausschleusung in die extrazelluläre Umgebung unterbinden. Dieser Prozess geht mit einer funktionalen NK-Zell-Aktivierung einher, welche durch Phospho-Aktivierung der PKC ϴ sowie IFN-γ- und Granzym B-Ausschüttung charakterisiert ist. Verschiedene mikroskopische Analysen zeigen zudem, dass die intrazellulären bakteriellen Strukturen in unmittelbarem Kontakt mit den sekretorischen Granula stehen und die Coxiellen-Freisetzung über Degranulierung infizierter NK-Zellen erfolgt. Der Abtötung innerhalb der sekretorischen Granula infizierter NK-Zellen scheint sich C. burnetii durch seine Säure- und Protease-Resistenz zu entziehen. Freigesetzte Coxiellen erhalten nach Degranulierung größtenteils ihre Integrität und Fähigkeit zur Infektion benachbarter Wirtszellen. Obschon Coxiellen der Eliminierung durch die sekretorischen Granula entgehen und dies eine kritische Achillesferse der angeborenen Immunantwort darstellt, verbleibt über das gleichzeitig ausgeschüttete IFN-γ infizierter NK-Zellen ein positiver Effekt auf die antibakterielle APC-Aktivität.
In ihrer Gesamtbetrachtung tragen die erzielten Ergebnisse dieser Promotionsarbeit zu einem besseren und tieferen Verständnis der C. burnetii-Infektion von DCs und NK-Zellen bei und geben neue Einsichten in die zelluläre Selbstverteidigung sowie die IFN-γ-basierte Immunkooperation innerhalb der frühen Phase der anti-Coxiellen Abwehr. Im weiteren Infektionsverlauf können jedoch diese immunologischen Prozesse durch auftretende Hypoxie vermutlich eingeschränkt und die Eliminierung intrazellulärer Coxiellen erschwert sein.
In recent years, negative impact of pharmaceutical products on natural environment became an issue of high public interest. Pharmaceutical residues are detected in various ecosystems worldwide. Due to increasing production and consumption of medicines this problem is intensified. Therefore, an efficient way to restrain release into the world’s water system is required.
This work presents an enzymatic approach for the degradation of pharmaceuticals in wastewater treatment plants, using laccase and cytochrome P450 — two enzymes of high biotechnological and industrial potential. Laccase genes from fungi Trametes versicolor and Pycnoporus cinnabarinus were isolated and overexpressed in the non-conventional yeast Arxula adeninivorans. This organism served also as cytochrome P450 gene donor.
Recombinant laccase Tvlcc5 was purified by immobilized-metal ion affinity chromatography and biochemically characterized using 2,2'-azino-bis(3-ethylbenzothiazoline-6-sulfonic acid) (ABTS) as substrate for enzyme activity assays. The optimal temperature and pH were found to be 50 °C and 4.5–5.5, respectively. The half-life of Tvlcc5 at 60 °C was around 20 min. It was demonstrated that the presence of copper ions is essential for the synthesis of active protein. Moreover, negative impact of chloride anions on laccase activity was shown.
Cultivation conditions for the Tvlcc5 producing strain A. adeninivorans G1212/YRC102-TEF1-TVLCC5-6H were optimized. It was found that maintaining the pH at a constant level between pH 6.0 and 7.0 is essential for the production of active enzyme. Optimal cell growth and laccase accumulation were reached at 20 °C and in medium supplemented with 0.5 mM CuSO4. Performed fed-batch cultivation resulted in a laccase activity of 4986.3 U L-1.
Factors influencing the synthesis of Tvlcc5 leading to increased production of this protein were investigated. It was found that using three non-native signal peptides (cutinase 2 from A. adeninivorans (ACut2), α-mating factor from S. cerevisiae (MFα), and acid phosphatase from P. pastoris (PHO1) signal peptides) enhances the secretion of active enzyme by 20–80%. Besides that, additional overexpression of copper transporters positively affects laccase production.
Finally, it was proven that recombinant Tvlcc5 is a promising agent for the degradation of certain pharmaceuticals. After 24 h of incubation, the concentration of diclofenac and sulfamethoxazole decreased to 46.8% and 51.1%, respectively. Furthermore, it was shown that the addition of the redox mediator ABTS significantly shortens the degradation time of these substances.
Wie andere Vertreter der Paramyxoviridae vergrößert das NDV durch Editierung von Transkripten seine Kodierungskapazität. Durch co-transkriptionelle mRNA-Editierung kodiert das P-Gen beim NDV sowohl für das P-, das V-, als auch das W-Protein. Die drei Proteine gleichen sich N-terminal, wohingegen die C-Termini in Länge und AS-Zusammensetzung variieren. Während sowohl Expression als auch Inkorporation des P- und V-Proteins in das NDV-Partikel nachgewiesen wurde, gab es bisher keinen Beweis für die Existenz des W-Proteins.
Für den Nachweis der Expression des NDV W-Proteins wurden W-spezifische Seren auf Grundlage von Peptiden generiert, welche im spezifischen C-Terminus lokalisiert waren und vorhersagbare antigene Regionen beinhalteten. Je eines der Kaninchenseren ermöglichte die Detektion von Plasmid-exprimiertem NDV W-Protein, sowie W-Protein in infizierten Zellen mittels indirekter IF und WB-Analyse.
Eine Inkorporation des W-Proteins in NDV-Virionen deuteten WB- und massen-spektrometrische Analysen an, während die Abwesenheit des Proteins für rekombinante NDV deren W-Protein Expression durch unterschiedliche Mutations-ansätze unterbunden wurde, in infizierten Zellen und Viruspartikeln bestätigt werden konnte.
Untersuchungen infizierter Zellen mit Hilfe konfokaler Mikroskopie zeigten eine Akkumulation des W-Proteins im Zellkern. Diese Lokalisation wurde auf eine zweigliedrige NLS im spezifischen C-Terminus zurückgeführt und die Funktionalität der NLS anhand der zytoplasmatischen Verteilung des Proteins in transfizierten bzw. infizierten Zellen nach Mutation der zwei basischen Cluster bestätigt.
Vergleichende Untersuchungen rekombinanter und WT-NDV zeigten keinen Einfluss der NLS bzw. der Expression des W-Proteins auf die Virusreplikation in vitro.
Bei der Analyse wirtsspezifischer, IFN-antagonistischer Funktionen des NDV W-Proteins in der späten Phase der Typ-I-IFN-Antwort mit Hilfe eines Hühnerzell-basierten IFN signaling Assays konnte sowohl für das W-Protein eines lentogenen (NDV Cl30), als auch eines velogenen NDV-Stammes (NDV Herts_I) kein inhibierender Effekt auf den untersuchten Signalweg gezeigt werden. Stattdessen deutete sich für das NDV Cl30 W-Protein ein aktivierender Effekt an.
Sequenzanalysen zur Vorhersagbarkeit von W-Proteinen bzw. C-terminal kodierten NLS in NDV-Stämme unterschiedlicher Virulenz und Genotypen ließen keinen Rückschluss auf einen Einfluss des W-Proteins auf die Pathogenität von NDV zu.
Im Gegensatz zum W-Protein war die Expression des NDV V-Proteins essentiell für die Replikation von NDV in vitro und in ovo.
Für die Analyse des Einflusses von V-Proteinen unterschiedlicher Herkunft auf die Replikation eines lentogenen NDV in vitro wurden diese in verschiedenen rekombinanten Viren von einem zusätzlich inserierten ORF exprimiert und die Expression der homo- und heterologen V-Proteine durch stammspezifische Seren überprüft, wofür im Vorfeld ein NDV R75/95 V-spezifisches Peptidserum generiert wurde. Keines dieser rekombinanten Viren zeigte Replikationsvorteile in vitro im Vergleich zum parentalen Virus.
Ein Hinweis auf einen Einfluss der Herkunft des V-Proteins konnte mit Hilfe des Hühnerzell-IFN signaling Assays erhalten werden. Während das V-Protein eines lentogenen NDV (NDV Cl30) keinen inhibierenden Effekt zeigte, deutete sich ein leicht inhibierender Effekt für das velogene NDV Herts_I V-Protein in einer Zelllinie an.
Pilotstudien zur potenziellen IFN-antagonistischen Funktion des V-Proteins wurden nach vorheriger Transfektion und Überexpression von V-Proteinen unterschiedlicher Pathotypen bzw. nach Vorbehandlung von Zellen mit Hühner-IFN-α vor Infektion durchgeführt. Die Replikation des korrespondierenden WT-Viruses bzw. rekombinanten Virus mit homo- oder heterologer V-Proteinexpression war in vitro in beiden Fällen nicht verändert.
Lipoproteins of Staphylococcus aureus represent a major class of surface proteins, which are anchored to the outer leaflet of the cell membrane. Although they play a key role in the immune response and virulence, the majority of lipoproteins in this organism is still of unknown function. The aim of our study was to investigate the function of so far poorly or uncharacterized lipoproteins in S. aureus strain Newman. To this end, an integrated bioinformatical approach was applied to define the pan-lipoproteome of 123 completely sequenced S. aureus strains. In total, this analysis predicted 192 different potential lipoproteins, with a core lipoproteome of 39 and a variable lipoproteome of 153 lipoproteins. Out of those 192 lipoproteins, 141 are so far functionally uncharacterized. Primarily focusing on members of the core-lipoproteome with unknown or poorly characterized function, 24 lipoproteins or co-encoded neighbor proteins were selected for further characterization. Of those 24 proteins, 20 S. aureus markerless deletion mutants were constructed (S. aureus delta l01 - delta l20) and screened for an altered growth behavior under various conditions. Here, three mutants showed a temperature-sensitive phenotype, two mutants formed aggregates in the TSB of the manufacturer Merck (TSBMerck), and four mutants showed reduced growth under osmotic stress with 8% NaCl. An altered aggregation behavior was observed for four mutants in the presence of Triton X-100 and for eleven mutants in the presence of SDS. Furthermore, ten mutants revealed an impaired biofilm formation capacity as well as reduced hemolytic activity. Interestingly, S. aureus deletion mutants delta l14 (delta NWMN_1435) and delta l16 (delta NWMN_0646) showed an altered phenotype under nearly all tested growth and stress conditions. Most strikingly, both deletion mutants demonstrated dramatic defects in cell morphology and cell division during the transient growth phase in TSBMerck and were therefore selected for further detailed characterization. Electron microscopy imaging of the two mutants revealed an irregular cell shape, increased cell size, multiple displaced division septa, and incomplete separation of daughter cells resulting in the formation of cell aggregates in TSBMerck. Complementarily, microarray-based transcriptome analysis and whole-genome sequencing of S. aureus delta l14 and delta l16 suppressor mutants strongly point to a functional association of both lipoproteins with cell envelope- or cell division-related processes. Specifically, multiple hints suggest a functional connection of both lipoproteins with lipo- or wall teichoic acids. Of note, the phenotypes of S. aureus delta l14 and delta l16 are conditional and appear under some, but not all growth conditions. Thus, it is conceivable that the function of L14 and L16 is modulated by metabolic processes, or that the proteins might be part of a “backup system” becoming important only under certain conditions. Collectively, we propose that L14 and L16 fulfill a basic role in cell envelope- or cell division-related processes under specific growth conditions. Particularly, the activity of L14 and L16 might be necessary for the function or localization of lipo- or wall teichoic acids, and thus, might be linked to the regulation of autolysins. In conclusion, this study reveals important insights into the function of two so far uncharacterized but highly conserved lipoproteins in S. aureus.
Vergleichende Untersuchungen zu rekombinanten Toxoplasma-gondii-Isolaten natürlichen Ursprungs
(2020)
Toxoplasma gondii ist ein weltweit vorkommender einzelliger Parasit mit hohem zoonotischen Potential. In Nordamerika und Europa haben sich drei klonale Toxoplasma-Linien durchgesetzt, Typ I, Typ II und Typ III. Sie unterscheiden sich hinsichtlich ihrer Virulenz in Labormäusen: Toxoplasma gondii vom Typ I gilt im Allgemeinen als hochvirulent, wohingegen Typ II und III wenig virulent in Labormäusen sind. In Deutschland dominieren T. gondii vom Typ II. Trotz selten vorkommender natürlicher sexueller Rekombinationen von T. gondii in Deutschland konnten in einer vorausgegangenen Studie rekombinante T. gondii-Typ II-III-Oozysten aus dem Kot einer natürlich infizierten Katze in Deutschland isoliert werden. Mittels klonaler Vereinzelung wurden in einer weiteren vorausgegangenen Studie aus diesen Oozysten die fünf Tachyzoiten-Klone B6-H6, 2-C10, 2-H8, C12 und A7 generiert, die sich in der Verteilung ihrer Typ II- und III-Allele voneinander unterschieden. Ziel dieser Arbeit war es, die fünf Klone vergleichend zu untersuchen hinsichtlich ihrer Geno- und Phänotypen. Besonderes Augenmerk wurde dabei auf die bekannten polymorphen Virulenzfaktoren ROP18, ROP5, ROP16 und GRA15 gelegt, die maßgeblich für Unterschiede in der Labormausvirulenz zwischen den klonalen Linien sorgen können. ROP18 und ROP5 sind an der Inhibition der IRG-vermittelten Zerstörung der parasitophoren Vakuole, dem Hauptabwehrmechanismus in Mäusen, beteiligt. Während alle fünf Klone das virulente Allel von ROP5 besaßen, hatten nur zwei der fünf Klone, B6-H6 und 2-C10, das virulente Allel von ROP18, dessen virulenter Genotyp in einer hohen Expression resultiert. Diese beiden Klone lösten auch eine 100 %-ige Mortalität in den infizierten BALB/c-Mäusen aus. Hier stimmte der virulente ROP18-Genotyp mit der hohen Mausvirulenz überein. Die anderen drei Klone, 2-H8, C12 und A7, besaßen das nicht virulente Allel von ROP18. Von letzteren drei Klonen lösten jedoch lediglich nur C12 und A7 eine geringere, 30 %-ige Mortalität in infizierten BALB/c-Mäusen aus. Hier würde der nicht-virulente ROP18-Genotyp die niedrigere Virulenz erklären. Der Klon 2-H8, der ebenso ein nicht-virulentes ROP18-Allel besaß, löste dagegen eine 100 %-ige Mortalität aus. Demnach ließe sich die Virulenz der infizierten BALB/c-Mäuse in dieser Studie nur in vier von fünf Klonen mit dem ROP18-Genotypen erklären. Neben ROP5 und ROP18 wurden auch die Virulenzfaktoren ROP16 und GRA15 untersucht. Diese regulieren das Zytokinprofil in infizierten Makrophagen und können dadurch Einfluss auf den klinischen Verlauf der Infektion nehmen. Von ROP16 und GRA15 besaßen jeweils alle fünf Klone das virulente Allel. Daher kann auch der Genotyp dieser Virulenzfaktoren hier nicht alleine die Unterschiede in der BALB/c-Mausvirulenz erklären. Auch das Expressionsprofil der Virulenzfaktoren in in-vitro inokulierten J-774A.1-Makrophagen mit geringen, wahrscheinlich nicht biologisch relevanten Abweichungen, ließ keine eindeutigen Rückschlüsse für die Ursache der unterschiedlichen Mausvirulenzen zu. Die in-vitro-Inokulation von J-774A.1-Makrophagen mit den Klonen ergab weiterhin, dass der mittelvirulente Klon C12 in der Lage war, die Makrophagen deutlich früher zu infizieren und eine höhere IL-12-Expression hervorzurufen. In überlebenden BALB/c-Mäusen verursachte er einen geringeren Gewichtsverlust gegenüber den anderen Klonen. Es kann für diese Studie festgehalten werden, dass sich die Virulenz der Klone in Labormäusen nicht allein durch das Vorhandensein virulenz-vermittelnder ROP18- oder anderer Virulenzgene erklären ließ. Durch die sexuelle Rekombination zwischen T. gondii des Typs II und III waren offenbar Allelkombinationen entstanden, welche auf ein komplexes multifaktorielles Netzwerk schließen lässt, das ursächlich für die Unterschiede in der Mausvirulenz und der Makrophagenfunktionalität zu sein schien.
Der Kernexport neusynthetisierter Kapside stellt einen Schlüsselprozess in der Herpesvirus-Replikation dar. Die zugrundeliegenden Mechanismen dieser Vesikel-vermittelten Translokation sind jedoch noch nicht vollständig verstanden. Der nuclear egress wird dabei maßgeblich von zwei viralen Proteinen dirigiert, die in PrV und HSV-1/-2 als pUL31 und pUL34 bezeichnet werden und in allen Herpesviren konserviert sind. Beide Proteine interagieren an der inneren Kernmembran, wo sie den sogenannten nuclear egress complex (NEC) bilden. Während pUL34 ein membranständiges Protein in der Kernmembran ist, gelangt das lösliche pUL31 über einen aktiven Transport in den Kern. Obwohl der erste Schritt der Freisetzung aus dem Kern, die Vesikelbildung und Abschnürung an der inneren Kernmembran, schon gut untersucht ist und auch die Kristallstrukturen des NEC für verschiedene Herpesviren ermittelt werden konnte, sind noch viele Fragen offen. So war zu Beginn dieser Arbeit noch unklar wie die Kapside in diese Hüllen rekrutiert werden und welche Rolle die nicht konservierte und offensichtlich flexible N-terminale Domäne von pUL31, die nicht in den Kristallstrukturen dargestellt werden konnte, für die Regulierung dieses Prozesses spielt. So konzentrierte sich diese Arbeit auf die Fragen, wie die Kapside mit dem NEC interagieren (Paper I und II) und wie der pUL31-N-Terminus diesen ungewöhnlichen Transportweg beeinflusst (Paper III).
Paper I und II: Untersuchungen zur Nukleokapsid/NEC Interaktion
Unklar ist, wie der NEC mit seiner Fracht, den Nukleokapsiden, interagiert. Auf Grundlage der vorhandenen Kristallstrukturen des Komplexes unterschiedlicher Herpesviren wurde eine Interaktionsdomäne in pUL31 postuliert und angenommen, dass dies mittels elektrostatischer Wechselwirkungen erfolgt. Um dies näher zu untersuchen, wurden in dieser Arbeit geladene Aminosäuren, die als mögliche Interaktionspartner in Frage kommen, zu Alanin mutiert. Die so generierten pUL31 Mutanten wurden, nach Transfektion entsprechender Expressionsplasmide in Kaninchennierenzellen (RK13), auf ihre Lokalisation und nach Koexpression mit pUL34 auf Interaktion getestet. Die Funktionalität der mutierten Proteine während der Virusreplikation wurde mit Hilfe stabiler Zelllinien nach Infektion mit PrV-∆UL31 untersucht. Über elektronenmikroskopische Analysen wurde der Einfluss auf den Kernexport im Detail betrachtet. Hierbei konnte einem konservierten Lysin an Position 242 in PrV pUL31 im Prozess der Kapsidumhüllung eine Schlüsselrolle zugeordnet werden. Dieses Lysin befindet sich im membrandistalen Bereich des NECs, in der Alphahelix H10 von PrV pUL31. Die Substitution des K242 zu Alanin führte zu einem Abschnüren und einer Akkumulation leerer, Virushüllen-ähnlicher Vesikel im PNS, obwohl reife Kapside im Kern und in unmittelbarer Nähe zu den Akkumulationen vorhanden waren. Dies führte zu der Hypothese, dass die Ladung des Lysins direkt an der Interaktion mit dem Kapsid beteiligt ist (Paper I).
Obwohl das Lysin 242 in der Struktur des Dimers oberflächenexponiert erschien, zeigten Modellierungen im NEC Oligomer, dass diese Aminosäure vermutlich zu tief in der Struktur verborgen ist um als direkter Interaktionspartner in Frage zu kommen. Um die im vorherigen Paper aufgestellte Hypothese zu verifizieren oder auch zu widerlegen, wurde das Lysin nicht nur durch Alanin, sondern auch durch andere nicht geladene, sowohl positiv als auch negativ geladene oder in ihrer Größe variierende Aminosäuren substituiert (Paper II).
Die neu generierten Substitutionsmutanten wurden nach Transfektion der Expressionsplasmide auf ihre Lokalisation und nach Kotransfektion mit pUL34, auf ihre Interaktion untersucht. Die Funktionalität der mutierten Proteine wurde ebenfalls mit Hilfe stabil exprimierender Zelllinien analysiert. Die vorliegenden Phänotypen wurden weiter mittels elektronenmikroskopischer Analysen bestimmt. Es stellte sich heraus, dass unabhängig von der vorhandenen Ladung der Aminosäure an Position 242 der Kernexport signifikant beeinträchtigt wurde. In Strukturanalysen der einzelnen Mutanten zeigte sich, dass vielmehr die Ausrichtung und Größe der Seitenkette der ersetzten Aminosäure entscheidend war. So störte beispielsweise die Substitution zu Serin und Tyrosin, die die Lage der Seitenketten des ursprünglich vorliegenden Lysins imitierten, die Funktion des pUL31 am wenigsten und die Titer erreichten fast Wildtypwerte. Dagegen führten Substitutionen zu deutlich längeren Aminosäuren, wie Glutaminsäure oder Arginin, zu massiven Beeinträchtigungen des nuclear egress. Allerdings führte keine der Substitutionen zu einem unkontrollierten Abschnüren von Vesikeln ohne Aufnahme eines Kapsids an der inneren Kernmembran.
Die hier gezeigten Ergebnisse entkräfteten die Annahme einer elektrostatischen Interaktion über pUL31 K242 mit den Nukleokapsiden in PrV. Vielmehr deuteten sie auf eine strukturell basierte Störung der Kapsidaufnahme in die Vesikel hin (Paper II).
Mittels serieller Passagen von Virusmutanten die das UL31 mit der K242A Substitution exprimierten, wurde nach möglichen kompensatorischen (second-site) Mutationen gesucht, die den Defekt ausgleichen und darüber hinaus Aufschluss auf die molekularen Ursachen ziehen lassen.
Die generierten Virusrekombinanten erreichten bereits nach ca. 10 Passagen Wildtpy-ähnliche Titer. Aus den Passagen wurden verschiedene Isolate charakterisiert. Es zeigte sich zwar keine Reversion zum Lysin 242, vielmehr waren jedoch entweder weitere Mutationen in pUL31 oder in pUL34 zu finden. Während die detektierten pUL34 Mutationen zu einem späteren Zeitpunkt charakterisiert werden müssen, wurden die second-site mutierten pUL31 Proteine auf Lokalisation, Kolokalisation und Kompensation des K242A Defektes getestet. Die Ergebnisse bestärkten die Annahme eines Strukturdefektes durch K242A. Darüber hinaus konnten durch Rückmutation des K242A Defektes in den second-site mutierten pUL31 zwei Helices bestätigt werden (H5 und H11), die ähnlich der H10 einen starken Einfluss auf den Kernexport besitzen.
Die erhaltenen Ergebnisse zeigten, dass die Aminosäure an Position 242 nicht direkt mit den Nukleokapsiden interagiert, dass eingeführte Mutationen jedoch die Umorganisation des NEC-Oligomers, welche offensichtlich notwendig für die effiziente Kapsidumhüllung an der inneren Kernmembran ist, stört und so den nuclear egress inhibiert (Paper II).
Es zeigte sich, dass sich die Struktur-Funktions-Beziehungen in den NECs komplexer darstellen als vermutet. Die Ergebnisse dieser Arbeit können zwar nicht den Mechanismus des Kapsidexports bzw. der Kapsidbindung und -inkorporation aufklären doch zeigen sie, dass die Interaktionen der NECs miteinander sehr viel komplexer aber auch wesentlich flexibler sind als zunächst angenommen.
Paper III: Untersuchung der N-terminalen Domäne von PrV pUL31
Neben einem Kernlokalisationssignal (NLS) beherbergt der N-terminus verschiedener pUL31 Homologer auch zahlreiche vorhergesagte Phosphorylierungsstellen, die an der Regulation des Kernexportes beteiligt sind bzw. sein könnten. Dieser flexible N-terminale Bereich hat in PrV pUL31 eine Länge von 25 Aminosäuren, wobei auffallend viele basische Aminosäuren in Clustern und verschiedene mögliche Phosphorylierungsstellen enthalten sind. Computer-unterstütze Analysen (NLStradamus) erkennen in der Aminosäuresequenz ein bipartites NLS (AS 5-20). Um die Rolle des N-terminalen Bereiches in PrV pUL31 näher zu untersuchen, wurde dieser schrittweise verkürzt und die basischen Aminosäuren, sowie die möglichen Phosphorylierungsstellen, durch gerichtete Mutagenese durch Alanin ersetzt. Getestet wurden diese Mutanten nach Transfektion der entsprechenden Expressionsplasmide in RK13 Zellen auf ihre Lokalisation und, nach Koexpression von pUL34, auf Interaktion und der Umorganisation der Kernmembran. Über stabil-exprimierende Zelllinien und nach Infektion mit der UL31 negativen Virusmutante (PrV-∆UL31) wurde die Funktionalität in eplikationsassays und auch ultrastrukturell charakterisiert. Erstaunlicherweise zeigte sich, dass weder das bipartite NLS noch die vorhergesagten Phosphorylierungsstellen eine entscheidende Rolle spielen. Vielmehr konnte der größte Teil des N-Terminus ohne sichtbaren Funktionsverlust deletiert werden, sofern mindestens ein Cluster basischer Aminosäuren in dieser Region erhalten blieb. Die Ergebnisse zeigten, dass der basische Charakter dieser Region entscheidend für die korrekte Lokalisation, sowie für die Bildung und Funktionalität des NEC ist. Weiterhin konnte gezeigt werden, dass die Phosphorylierung im N-Terminus von PrV pUL31, wie auch die roteinkinase pUS3, zwar nicht essenziell für die Freisetzung der Nukleokapside aus dem perinukleären Spalt sind, jedoch diesen Prozess unterstützen (Paper III).
Reactive species play an essential role in orchestrating wound healing responses. They act as secondary messengers and drive redox-signaling pathways that are involved in the hemostatic, inflammatory, proliferative and remodeling phases of wound healing. Cold plasma produces a profusion of short- and long-lived redox species that promotes wound healing, however, until today, the knowledge of CAP mediated wound healing remained scarce. In this thesis, CAP mediated wound healing mechanism and their effect on extracellular matrix and adhesion molecules have been investigated. To this end, a keratinocyte cell line (HaCaT), skin fibroblast cell line (GM Fbs) and an in vitro coculture model including both HaCaT and GM Fbs at a 2:1 ratio, were employed to investigate the cross talk between these two skin cell types.
We examined the impact of CAP on extracellular matrix proteins and cell adhesion molecules in GM Fbs and observed a significant impact of cold plasma treatment on the expression level of collagen moieties, cell adhesion molecule like integrin, cadherin, versican, MMPs as well as extracellular matrix proteins.
Moreover, scratch assays with monocultures of HaCaT, GM Fbs and coculture of these two cell types were performed. We detected that, CAP accelerated the migratory capability of HaCaT cells cocultured with fibroblasts. In fact, compared to HaCaT monoculture, a significant acceleration on cell migration was observed in coculture upon CAP treatment. NAC, a potent antioxidant could abrogate this CAP-stimulated cell migration in coculture, further pointing towards the importance of well-orchestrated reactive species in wound healing. To better understand this CAP-mediated effect on cell migration, we examined the signaling pathways involved in tissue homeostasis and regeneration. We checked the HIPPO signaling pathway and observed an upregulation of several signaling molecules at transcriptional level in GM Fbs upon CAP treatment.
YAP is the central nuclear executer of HIPPO signaling pathway. YAP was upregulated in both HaCaT cells and GM Fbs. The major downstream effectors of the HIPPO signaling pathway (CTGF and Cyr61) were also upregulated in dermal fibroblasts at both transcriptional and protein level. However, administration of antioxidant NAC inhibited CAP-mediated wound healing and abrogated the gene expression of the HIPPO downstream effectors. These results confirm that the upregulation of YAP-CTGF-CYR61 axis is due to CAP-generated redox species. In HaCaT cells, both CTGF and Cyr61 was minimally transcribed. Even though CTGF was rarely detected in HaCaT cells on the protein level,Cyr61 remained undetected. This again shows the importance of the cross talk between fibroblasts and keratinocytes.
The coculture with the inclusion of fibroblasts showed an accelerated migration rate, compared to HaCaT monoculture which specifies a cross talk between these two cell types. Thus, monoculture of HaCaT cells were incubated with CAP-treated and untreated fibroblast conditioned medium. Interestingly, we observed that HaCaT cells exhibited an improved cell migration rate when incubated with CAP-treated fibroblast-conditioned media compared to that observed after incubation with untreated media. Upon investigation, an induction of CTGF and Cyr61 secretion was observed upon CAP treatment in the fibroblast-conditioned media. Furthermore, exposure to recombinant CTGF and Cyr61 could also significantly improve HaCaT cell migration which confirms that CAP mediated accelerated cell migration is due to activation of YAP-CTGF-Cyr61 axis.
In conclusion, this study revealed a completely new mechanical insight of CAP mediated wound healing. Along with several other ECM molecules, CAP activates a regenerative signaling pathway i.e., HIPPO signaling pathway in dermal fibroblasts at the onset of wound healing. Dermal fibroblasts drive a paracrine interaction by secreting CTGF and Cyr61 in close vicinity of wound, resulting in accelerated keratinocyte migration and wound healing in coculture.
Die McsB Argininkinase spielt in grampositiven Bakterien wie Bazillen, Staphylokokken und Listerien durch die Phosphorylierung von Guanidinogruppen eine gesonderte Rolle innerhalb der Familie der Kinasen. Insbesondere während der bakteriellen Stressadaptation scheint diese Art der posttranslationalen Proteinmodifikation von großer Bedeutung zu sein. Um die Funktionsweise der McsB Kinasefunktion in Verbindung mit dessen McsA Modulatorprotein besser verstehen zu können, wurden konservierte Arginine gegen Lysin substituiert. Auf diese Weise konnten entscheidende intramolekulare Positionen identifiziert werden, die für die Ausbildung der Autokinase- bzw. Phospho-Transferase Aktivität von Bedeutung sind. Diese konnten darüber hinaus in Einklang mit der McsB Struktur (Suskiewicz et al., 2019) gebracht werden.
Eines der Zielproteine für die McsB vermittelte Argininphosphorylierung (Arg-P) ist dabei der CtsR Regulator, welcher die Genexpression der Clp-Maschinerie in Bacillus subtilis reprimiert. Mit Hilfe globaler Transkriptomanalysen war es möglich, neben den bereits etablierten Zielgenen auch eine Art fine-tuning Regulation des MhqR Regulons aufzuzeigen.
Zwei weitere Proteine, die durch McsB vermittelte Arg-Ps beeinflusst werden, sind der Modulator der generellen Stressantwort, MgsR, und die intrinsisch inaktive Glutamat-Dehydrogenase GudB. Insbesondere GudB fällt durch die Identifikation von 15 Phospho-sites auf, wohingegen lediglich zwei Arg-P Bindungsstellen für MgsR nachgewiesen werden konnten (Elsholz et al., 2012; Schmidt et al., 2014; Trentini et al., 2016). Dennoch ist die GudB Stabilität nur geringfügig durch die McsB Kinasefunktion beeinflusst, wohingegen die MgsR Degradation entscheidend durch Arg-Ps beeinflusst scheint. Durch die Substitution der Arginine von MgsR gegen Glutamat wurde eine Art Phospho-Mimikry integriert. So konnten die Auswirkungen auf Regulatoraktivität und Stabilität von MgsR durch mögliche Arg-Ps im Detail untersucht werden.
In diesem Zusammenhang wurden durch detaillierte Untersuchungen der MgsR Degradation zusätzliche Informationen zur Funktionsweise von McsB als Adapterprotein gesammelt. Dieses legten die Vermutung nahe, dass McsB nicht nur als ClpC-Adapterprotein fungiert, sondern darüber hinaus auch die ClpX-abhängige Proteindegradation unterstützt.
Rekombinante Vektorvakzinen, basierend auf Viren der Newcastle-Krankheit (NDV) haben sich als kostengünstig, schnell herstellbar und sicher für die Applikation bei Geflügel und Säugetieren erwiesen. Im Rahmen dieser Arbeit wurden zwei rekombinante Vakzineviren, die das lentogene NDV Clone 30 als Vektor nutzen, für die Prävention der hochpathogenen aviären Influenza (HPAI) bei Hühnerküken, die maternale aviäre Influenzavirus-spezifische Antikörper (AIV-MDA) aufweisen, und die Pest der kleinen Wiederkäuer (PPR) bei Ziegen evaluiert.
Während bekannt ist, dass rekombinante NDV/AIV-H5-Vakzineviren in spezifisch pathogenfreien Eintagsküken eine protektive Immunantwort induzieren, ist diese bei Küken in HPAI-Endemiegebieten meist durch vorhandene AIV-MDA negativ beeinflusst. Durch die Generierung einer NDV-Rekombinanten (rNDVsolH5_H5), die das HA des HPAIV H5N1 von zwei individuellen Fremdgenen exprimiert, konnte eine Überexpression des H5 und in Folge der okulonasalen Immunisierung von zwei- und drei-Wochen-alten AIV-MDA+-Küken die Überwindung der AIV-MDA und die Bildung von wirtseigenen AIV-H5-spezifischen Antikörpern erreicht werden. Die in Folge einer HPAIV H5N1-Belastungsinfektion vermittelten Protektionsraten beliefen sich auf 85 % bei zwei-Wochen-alten und auf 100 % bei drei-Wochen-alten Hühnern, deren Ausscheidung des virulenten Wildtypvirus im Vergleich zu Kontrolltieren signifikant reduziert war. Auch wenn das rekombinante Impfvirus in ein-Wochen-alten AIV-MDA+-Küken replizieren konnte, weist die Schutzrate von 40 % darauf hin, dass die Immunisierung sehr junger AIV-MDA+-Küken nicht zu empfehlen ist.
Die subkutane Immunisierung von Ziegen mit dem rekombinanten Vektorvirus rNDV_HKur, das das Hämagglutinin des Morbillivirus der kleinen Wiederkäuer (small ruminant morbillivirus, PPRV) exprimiert, schützte diese vor einer virulenten Wildtypvirus-Infektion. Nach zweimaliger Applikation wurden, wie nach der Impfung mit einer atttenuierten PPRV-Lebendvakzine, weder Erkrankungszeichen beobachtet noch eine hämatogene Streuung und nur geringgradige Replikation bzw. Ausscheidung des PPR-Wildtypvirus nachgewiesen, was auf die Bildung PPRV-neutralisierender Antikörper nach der Immunisierung zurückzuführen ist. Somit konnte gezeigt werden, dass sich das rekombinante NDV/PPRV-H für die Prävention der PPR bei Ziegen eignet. Mit NDV als Vektorvirus konnten nachweislich die Anforderungen sowohl bezüglich der DIVA-Applikation als auch einer hohen Thermostabilität erreicht werden.
Um NDV als Vektorvirus gezielt zu verändern bzw. für dessen unterschiedliche Anwendungen zu verbessern, ist es von Vorteil die Funktion der einzelnen viralen Proteine zu kennen. Mit dem erstmaligen Nachweis der Expression des W-Proteins können nun mit Hilfe des generierten W-spezifischen Peptidantiserums weitere in-vitro- und in-vivo-Analysen erfolgen, um dessen Funktion im viralen Replikationszyklus näher zu untersuchen.
Herpesviruses are enveloped DNA viruses which are dependent on two fusion steps for efficient replication in the host cell. First, they have to fuse their envelope with the cellular plasma membrane or with the vesicle membrane after endocytic uptake to enter the host cell and second, they have to export the newly generated nucleocapsids from the site of assembly to the cytoplasm by fusion of the primary virion envelope with the outer nuclear membrane (ONM). The main goal of this project was to provide a better understanding of how herpesvirus capsids exit the nucleus. On the one hand this thesis aimed at finding cellular proteins involved in nuclear egress (Paper I), while on the other the focus was on further characterization of the viral nuclear egress complex (NEC, Paper II) and its interaction with the capsid (Paper III).
It is the hallmark of viruses, including herpesviruses, to hijack host cell proteins for their efficient replication. Some of those interactions are well characterized, while others might not yet have been discovered. In the last step of the nuclear egress, where the primary virion membrane fuses with the ONM, most likely a cellular machinery is involved. The presented work focused on Torsin, the only known AAA+ ATPase localizing in the endoplasmic reticulum and the perinuclear space (PNS). For this, the effect of overexpression of WT and mutant proteins, as well as CRISPR/Cas9 generated knock-out cell lines, on PrV replication was analyzed. Neither single overexpression nor single knockouts of TorA or TorB had any significant effects on virus titers. However, infection of TorA/B double knockout cells revealed reduced viral titers and an accumulation of primary virions in the PNS at early infection times, indicating a delay in nuclear egress.
The process of nuclear egress has been intensively investigated without revealing all its details. To address some of the missing aspects we generated monoclonal antibodies (mAbs) against the NEC and its components (pUL31 and pUL34) for a better visualization of the process in transfected as well as infected cells. These mAbs provide a useful tool for future analyses.
The publication of the NEC crystal structure formed the basis for intensive research on the molecular details of the NEC formation and its interaction with the nucleocapsid. Recently, our lab showed that lysine (K) at position 242 in the membrane-distal part of pUL31 is crucial for incorporation of the nucleocapsid into budding vesicles. Replacing K by alanine (A) resulted in accumulations of vesicles in the PNS, while mature capsids were not incorporated. To test whether this is due to electrostatic interference or structural restrictions we substituted K242 by different aa to determine the requirements for nucleocapsid uptake into the nascent primary particles. To analyze whether the defect of pUL31-K242A can be compensated by second-site mutations, PrV-UL31-K242A was passaged and mutations in revertants were analyzed. Different mutations have been identified compensating for the K242A defect. A considerable number of mutations indicates that the NEC is much more flexible than previously thought. Further, we gained information that the K at position 242 is not directly involved in capsid interaction, while it is more likely involved in rearrangements within the NEC coat.
Untersuchung von Virulenzdeterminanten des Newcastle Disease Virus mit Hilfe von Virusrekombinanten
(2020)
Die Newcastle Krankheit (Newcastle Disease, ND) wird durch das aviäre Paramyxovirus-1 (APMV-1) verursacht und zählt zu den bedeutendsten Viruserkrankungen des Geflügels, wobei die Ausprägung der Krankheitssymptome sehr stark variiert. Das APMV-1 der Taube (pigeontype paramyxovirus, PPMV-1) infiziert größtenteils Brief-, Rasse-, Stadt- und Wildtauben, jedoch ist auch Wirtschaftsgeflügel für diesen Erreger empfänglich. Die Krankheit ist weltweit verbreitet und besonders die schweren Verlaufsformen, ausgelöst durch den mesogenen und den velogenen Pathogenitätstyp, führen bis heute zu hohen wirtschaftlichen Verlusten. Durch die Entwicklung des reversen genetischen Systems für das NDV ist es möglich, verschiedene Bereiche des viralen Genoms unterschiedlich pathogener NDV-Isolate auszutauschen und rekombinante Viren zu generieren, um mögliche Virulenzdeterminanten zu identifizieren. Lange Zeit galt die Aminosäuresequenz an der proteolytischen Spaltstelle des Fusionsproteins als die Virulenzdeterminante des NDV. Studien der letzten Jahre belegen aber zunehmend, dass es weitere Sequenzabschnitte im Genom gibt, die Einfluss auf die Pathogenität haben. Besonders bei den Taubenisolaten zeigte sich, dass diese trotz einer polybasischen Aminosäuresequenz an der proteolytischen Spaltstelle des F-Proteins, die typisch für meso- und velogene APMV-1 ist, mit einem ermittelten intrazerebralen Pathogenitätsindex (ICPI) < 0,7 als lentogen (niedrig virulent) einzuordnen sind.
Die Bestimmung der Gesamtsequenz des vorliegenden PPMV-1 Isolates R75/98 und die Herstellung des entsprechenden rekombinanten Virus rR75/98 waren Ziel dieser Arbeit. Nach der in vitro-Charakterisierung, die keine signifikanten Unterschiede zwischen dem Wildtyp und der Rekombinante zeigte, verdeutlichte die ICPI-Bestimmung, dass sich R75/98 und rR75/98 in ihrer Pathogenität unterschieden. Während R75/98 mit einem ICPI von 1,1 als mesogen eingestuft wurde, entsprach das rekombinante Virus rR75/98 mit einem ICPI von 0,28 dem lentogenen Pathotyp. Durch einmalige Passage der Rekombinante im Tier entstand das Reisolat RrR75/98, welches sich in seinen in vitro-Eigenschaften nicht von den beiden anderen Isolaten unterschied, aber in seiner Pathogenität (ICPI 0,93) wieder dem mesogenen Ausgansvirus R75/98 entsprach. Unter Nutzung des Next Generation Sequencing war es möglich, die Grundlagen für diese Pathogenitätsunterschiede aufzuzeigen. Während es zwischen R75/98 und rR75/98 insgesamt acht Aminosäuresubstitutionen gab (drei im F-Protein, zwei im HN-Protein und drei im L-Protein), die zu einer Verminderung der Pathogenität führten, wurden nur zwei Aminosäuremodifikationen (jeweils eine im F- und L-Protein) nachgewiesen, um die Pathogenitätssteigerung vom lentogenen rR75/98 hin zum mesogenen RrR75/98 hervorzurufen. Beide Aminosäureaustausche haben einen Effekt auf die vorhergesagte Proteinstruktur und beeinflussen vermutlich die Proteinfaltung, was wiederum eine nicht unwesentliche Auswirkung auf die biologische Aktivität des Virus haben kann. Besonders die Modifikation im F-Protein an Aminosäureposition 472 verdeutlicht, dass neben der Aminosäuresequenz an der proteolytischen Spaltstelle andere Bereiche dieses Proteins Einfluss auf die NDV-Virulenz haben.
Zur Untersuchung des Einflusses einzelner Abschnitte des F-Proteins auf die Pathogenität wurden im ursprünglich lentogenen NDV Clone 30 einzelne Sequenzbereiche durch die des mesogenen PPMV-1 R75/98 substituiert, die entsprechenden rekombinanten Viren generiert und charakterisiert. Es zeigte sich, dass sowohl die Expression als auch die Inkorporation der chimären Fusionsproteine mittels Western-Blot nachgewiesen werden konnte. Die Rekombinanten unterschieden sich weder in Größe noch in Form (Elektronenmikroskopie) und die chimären Fusionsproteine konnten an der Plasmamembran der Wirtszellen detektiert werden. Alle Rekombinanten waren in der Lage, Synzytien auszubilden und in verschiedenen Zelllinien (Wachtelmuskelzelle, Hühnerembryofibroblasten) bzw. in embryonierten Hühnereiern zu replizieren. Bei der Bestimmung des ICPIs zeigten sich jedoch Unterschiede. Zwei der sechs Rekombinanten wurden als lentogen eingestuft, die anderen vier wurden dem mesogenen Pathogenitätstyp zugeordnet. Es konnte gezeigt werden, dass neben der Interaktion der homologen F1- und F2-Untereinheit, die zytoplasmatische Domäne des Fusionsproteins einen bedeutenden Einfluss auf die Pathogenität von NDV hat. Auch für andere Vertreter der Paramyxoviren ist bekannt, dass die zytoplasmatische Domäne der beiden Oberflächenproteine F und HN mit dem M-Protein interagiert und diese Interaktion wichtig für den Zusammenbau der Viruspartikel, den Knospungsvorgang und die Freisetzung der Viren ist.
Neben dem Fusionsprotein existieren zusätzlich Virulenzdeterminanten in den weiteren NDV-Proteinen. Während es bereits Untersuchungen zum Einfluss auf die Pathogenität für die Proteine NP, P, V, M, F, HN und L gibt, war es noch nicht möglich, eine Aussage zum W-Protein zu treffen, da der Nachweis dieses Proteins bis dato nicht erfolgte. Zunächst wurde für unterschiedlich pathogene NDV der Bereich der P-Gen-Editierungsstelle amplifiziert, gefolgt von einer Tiefensequenzierung, um zusätzlich zur P- und V-mRNA auch die W-mRNA nachzuweisen und deren mengenmäßigen Anteil zu bestimmen. Im Rahmen dieser Arbeit wurden außerdem Plasmide hergestellt, die für weiterführende Arbeiten genutzt werden konnten, in denen erstmals der Nachweis des W-Proteins für NDV gelang.
Das Bovine Virale Diarrhoe Virus (BVDV) gehört zum Genus Pestivirus innerhalb der Familie der Flaviviridae. BVDV verursacht eine gefährliche Durchfallerkrankung bei Rindern,
besonders Kälbern, die Bovine Virusdiarrhoe (Mucosal Disease). BVDV gehört zu den einzelsträngigen RNA-Viren und ist eng verwandt mit dem Erreger der Klassischen Schweinepest sowie der Border Disease der Schafe. Wie andere Pestiviren, ist BVDV ein behülltes Virus, auf dessen Hülle drei Strukturproteine (Erns, E1 und E2) zu finden sind. In dieser Arbeit wurden die Glykoproteine E1 und E2 genauer charakterisiert, um Hinweise auf den Mechanismus der Knospung (Budding) von Pestiviren zu erhalten. Dazu ist die subzelluläre Lokalisation, die Topologie sowie der Retentionsmechanismus für E1 und E2 genauer untersucht worden. Die subzelluläre Lokalisation der Hüllproteine wurde mit Hilfe von Kolokalisationsanalysen mit spezifischen Kompartimentmarkerproteinen bestimmt. Sowohl als Einzelexpression als auch nach Expression als E1-E2-Vorläuferprotein zeigte sich eine Anreicherung der beiden Proteine vorwiegend im ER. Die Lokalisationsanalyse E2s in mit verschiedenen BVDV-Stämmen infizierten Zellen zeigte ein sehr ähnliches Bild wie die Einzelexpression. Die, die intrazelluläre Retention vermittelnden, Regionen wurden zunächst mit CD72-Fusionsproteinen eingegrenzt und zeigten, dass die Transmembrandomänen der Proteine für die Retention entscheidend waren.
Anhand verschiedenster Mutanten, welche Substitutionen, Insertionen und Deletionen im Bereich des C-Terminus von CD72-E1 bzw. E2 (ohne CD72-Fusionspartner) beinhalteten,
konnten einzelne Aminosäuren identifiziert werden, die essentiell für die Retention sind oder diese zumindest beeinflussen. Für E2 konnte das Arginin an Position 355 als wichtig für die Retention bestätigt und weiterführend untersucht werden. Mit Mutationen des Glutamins an Position 370 konnte außerdem der modulierende Effekt des cytoplasmatischen Rests auf die Retention E2s gezeigt werden. Die Retention von E1 ist unabhängig von der Länge der TMD und wird durch mehrere polare Aminosäuren (K174, R177, Q182) beeinflusst. Die Topologieuntersuchungen
für E1 und E2 nach Einzelexpression mit Tag-markierter Proteinvarienten zeigte, dass die reifen Proteine eine einspännige Transmembrandomäne mit dem N-Terminus auf der luminalen und dem C-Terminus auf der cytosolischen Seite des ERs besitzen.
Phylogeny of the Koi herpesvirus and development of a vaccine against the Koi herpesvirus disease
(2019)
The aim of this presented dissertation was a stable, live attenuated and protective KHV usable as vaccine. Moreover this vaccine should by cost effective and easy to apply. Differentiation of infected and vaccinated animals was preferred by genetic and / or serological means. After achieving an attenuated virus, whole genome sequencing should be done to examine the genetic of the vaccine as one feature of biosafety. Besides biosafety additional knowledge on the virulence of Alloherpesviruses, especially of KHV was anticipated. Additionally the diagnostics of KHV and KHVD should be improved to increase reliability and to gain more insights into the relationship of different KHVs and hopefully to detect the source of an outbreak.