Refine
Year of publication
Document Type
- Doctoral Thesis (155)
- Article (51)
Is part of the Bibliography
- no (206)
Keywords
- - (37)
- Staphylococcus aureus (18)
- proteomics (13)
- Virologie (11)
- Massenspektrometrie (9)
- Proteomanalyse (9)
- Bakterien (7)
- Herpesvirus (7)
- Proteomics (7)
- Virulenz (7)
Institute
- Abteilung für Mikrobiologie und Molekularbiologie (206) (remove)
Publisher
- MDPI (20)
- Frontiers Media S.A. (18)
- Nature Publishing Group (3)
- S. Karger AG (3)
- Wiley (3)
- American Society for Microbiology (ASM) (1)
- BioMed Central (BMC) (1)
- Elsevier (1)
- Springer Nature (1)
Microglia are the resident immune cells of the central nervous system (CNS) and play a major role in the regulation of brain homeostasis. To maintain their cellular protein homeostasis, microglia express standard proteasomes and immunoproteasomes (IP), a proteasome isoform that preserves protein homeostasis also in non-immune cells under challenging conditions. The impact of IP on microglia function in innate immunity of the CNS is however not well described. Here, we establish that IP impairment leads to proteotoxic stress and triggers the unfolded and integrated stress responses in mouse and human microglia models. Using proteomic analysis, we demonstrate that IP deficiency in microglia results in profound alterations of the ubiquitin-modified proteome among which proteins involved in the regulation of stress and immune responses. In line with this, molecular analysis revealed chronic activation of NF-κB signaling in IP-deficient microglia without further stimulus. In addition, we show that IP impairment alters microglial function based on markers for phagocytosis and motility. At the molecular level IP impairment activates interferon signaling promoted by the activation of the cytosolic stress response protein kinase R. The presented data highlight the importance of IP function for the proteostatic potential as well as for precision proteolysis to control stress and immune signaling in microglia function.
Kunststoffe durchdringen nahezu jeden Bereich unseres alltäglichen Lebens. Zur Herstellung bestimmter Plastikmaterialien (Epoxidharze und Polycarbonate) werden Bisphenole als Grundbaustein benötigt, deren Grundstruktur sich aus zwei Phenolringen zusammensetzt, die über eine substituierte Kohlstoffbrücke miteinander verbunden sind. Die einzelnen Bisphenole unterscheiden sich jeweils durch verschiedene Substituenten an der Kohlenstoffbrücke oder an den aromatischen Ringsystemen. Dabei gehen die großmaßstäbliche Produktion der Bisphenole sowie unser permanenter Kontakt mit bisphenolhaltigen Materialien mit einer verstärkten Nachweisbarkeit dieser Chemikalien in Umweltproben bzw. in menschlichen Geweben und Körperflüssigkeiten einher. Gleichzeitig stehen Bisphenole im Verdacht, aufgrund ihrer Toxizität und hormonähnlichen Wirkung eine Vielzahl von Erkrankungen zu begünstigen. Vor allem die Interaktion mit dem Östrogenrezeptor alpha ist gut verstanden. Daher wurde in dieser Arbeit die bakterielle Transformation von acht verschiedenen Bisphenolen (Bisphenol A, AP, B, C, E, F, PH und Z) durch die Umweltisolate Cupriavidus basilensis SBUG 290 und Bacillus amyloliquefaciens SBUG 1837 untersucht und näher charakterisiert. Beide Bakterienstämme waren in der Lage, alle eingesetzten Bisphenole zu transformieren. Dabei war die Transformation auf die Phenolringe oder daran befindliche Substituenten beschränkt. Ein mikrobieller Angriff an der ringverbindenden Kohlenstoffbrücke wurde nicht nachgewiesen. Während B. amyloliquefaciens die Schadstoffe ungeachtet ihrer Struktur jeweils phosphorylierte, transformierte C. basilensis die Bisphenole in Abhängigkeit von ihrer Struktur zu hydroxylierten Derivaten, Ringspaltungsprodukten, Produkten mit Acetamidstruktur oder zu Dimeren. Neben der Strukturaufklärung der mikrobiell gebildeten Produkte wurden die einzelnen Transformationswege für beide Bakterienstämme näher charakterisiert. Hierfür wurden u.a. die Produkte als Transformationssubstrate eingesetzt, der Einfluss der Kultivierung und Inkubationsmedien auf die Biotransformation untersucht sowie Proteomanalysen durchgeführt. Die Bildung von hydrophileren Transformationsprodukten durch die Bakterienstämme führte zur Detoxifizierung und Reduktion der östrogenen Aktivität der hydrophoben Bisphenole.
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.
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.
The introduction of two-dimensional polyacrylamide gel electrophoresis (2-D PAGE) enabled the separation and visualization of a substantial fraction of an organism’s entire proteome, and when mass spectrometry entered protein science, these proteins became even amenable to identification on a grand scale. Nevertheless, important classes of proteins elude a separation on classical 2 D gels, as the ones showing extremes in isoelectric point or molecular weight, and foremost very hydrophobic proteins naturally embedded in lipid membranes. This thesis aimed at the establishment and adaptation of alternatives to 2-D PAGE. New techniques allowing for an identification and quantification of critical protein classes were designed and adopted to physiological questions in the Gram-positive bacteria Bacillus subtilis and Staphylococcus aureus. In a comprehensive study on cytoplasmic proteins of S. aureus COL the number of proteins identified by a 2-D gel based approach could be extended by 650 proteins employing gel free technologies. Application of these complementary methods resulted in the establishment of a comprehensive reference map of the cytosolic proteome in growing and non-growing S. aureus cells which can serve as basis for further physiological investigations. Gel free separation of complex protein digests was likewise used in a quantitative study on heat stress in B. subtilis. By implementation of the iTRAQ® technology four different physiological states could be relatively quantified in one experiment. A parallel generation of 2-D gel based data enabled the depiction of strengths and weaknesses of protein quantitation by both, spot intensities on 2-D gels and iTRAQ® signal intensities in MS/MS spectra. Furthermore, new insights into heat sensitivity of pivotal enzymes involved in amino acid biosynthesis could be delivered. The institution of gel free approaches and advancements in 2-D PAGE provide the tools to penetrate into yet unamenable scopes of proteomes. A review on proteome coverage in B. subtilis gives an overview on the strategies which have been explored for most comprehensive protein identification in various sub-proteomes. Although more than one third of B. subtilis’ open reading frames could be demonstrated on protein level, one has to be aware of the fact that it still is a long way to achieve complete coverage of its proteome. Integral membrane proteins make up about one quarter of the entirety of proteins in a cell. Despite their large portion they are clearly understudied due to the intricacy of identification. Their low abundance and non-accessibility of membrane-spanning domains represent major experimental difficulties. The establishment of a protocol efficiently depleting cytosolic proteins by membrane shaving and targeting trans-membrane peptides by novel digestion strategies essentially facilitated identification of highly hydrophobic integral membrane proteins. This protocol was not only successfully applied to the membrane proteome of growing S. aureus cells, but was shown to be applicable in B. subtilis as well. Both studies displayed the novel membrane shaving approach to be highly complementary to a previously established separation of membrane proteins via 1 D PAGE. A combination of the two techniques resulted in identification of about half of the theoretical membrane proteome in both bacteria, and hence layed the foundation for advanced and quantitative analyses. In this regard, 14N/15N metabolically labeled membrane samples of growing and non-growing cells of S. aureus COL were relatively quantified revealing a significant difference in amount for more than one third of the proteins. A corresponding experimental setup was used to compare the membrane proteomes of S. aureus SA113 and its mutant deficient in the lysylphosphatidylglycerol synthetase MprF. Interesting quantitative differences were obtained for proteins most likely involved in the regulation of cellular surface net charge as well as for virulence-associated proteins.
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.
Staphylococcus aureus ist einer der bedeutendsten Erreger von Infektionen der Milchdrüse (Mastitis). In dieser Arbeit wurden 16 S. aureus-Isolate aus bovinen Mastitisinfektionen unterschiedlicher geografischer Herkunft umfassend charakterisiert, um tiefere Einblicke in die Wirtsspezifität von S. aureus zu erlangen. Das bovine Mastitisisolat S. aureus RF122, dessen Genomsequenz seit kurzem verfügbar ist, wurde zum Vergleich in die Studien einbezogen. Mittels Multilocus Sequence Typing wurde die klonale Verwandtschaft der Stämme analysiert und ihre Zugehörigkeit zu bestimmten Sequenztypen bzw. klonalen Komplexen ermittelt, von denen einige unter bovinen S. aureus-Isolaten weltweit sehr verbreitet sind.Zum Nachweis von virulenz- und resistenzassoziierten Genen, sowie regulatorischen und speziesspezifischen Markergenen wurde ein diagnostischer DNA-Microarray eingesetzt. Es konnte gezeigt werden, dass das individuelle Profil der Isolate sehr stark variierte und sich selbst Stämme mit dem gleichen Sequenztyp in ihrem variablen Genom teilweise erheblich unterschieden. Nur 43 Gene, die u.a. für Hämolysine, Proteasen, Leukocidine kodieren, waren in allen Stämmen konserviert. Es wurde auch die Existenz einiger als bovin-spezifisch angesehener Gene, bzw. die Abwesenheit humanspezifischer Gene nachgewiesen. Zusätzlich wurde die Expression von Virulenzfaktoren mittels 2D-Gelelektrophorese und massenspektrometrischer Identifizierung analysiert. Wie erwartet unterschieden sich die extrazellulären Proteommuster der einzelnen Stämme stark. Nur zwölf sekretierte Proteine wurden (in unterschiedlicher Menge) von mindestens 80 % der bovinen Isolate gebildet, und bilden das sogenannte „Core-Exoproteom“. Auch Isolate mit nahezu identischer genetischer Zusammensetzung unterschieden sich z.T. erheblich in ihrem Exoproteom, was sehr gut mit der Transkription des Virulenzgenregulators RNAIII korrelierte. Weiterhin wurde die mitogene Wirkung der Kulturüberstände auf humane und bovine PBMC (mononukleäre Zellen aus peripherem Blut) untersucht. Dabei fiel auf, dass zwei Isolate, welche Gene der bovinen Pathogenitätsinsel SaPIbov trugen, bovine T-Zellen stärker als humane stimulierten, was auf wirtsspezifische Unterschiede in der Aktivität dieser Superantigene hindeutet. Schließlich konnten durch den Vergleich mit S. aureus-Isolaten aus humanen Infektionen bestimmte Proteine ermittelt werden, die häufiger mit einem bestimmten Wirt assoziiert sind. Die Variabilität in der Expressionshäufigkeit dieser Proteine könnte mit der Wirtsspezifität von S. aureus im Zusammenhang stehen. Als pathogener Mikroorganismus ist S. aureus hohen Konzentrationen an reaktiven Sauerstoff- und Stickstoffspezies (ROS und RNS) ausgesetzt, die im Rahmen der unspezifischen Wirts-Immunantwort gebildet werden. Um das Verständnis über seine Anpassungsstrategien zu erweitern, wurden vier Substanzen, die oxidativen bzw. nitrosativen Stress verursachen, eingesetzt: Wasserstoffperoxid (H2O2), eine Vorstufe des stark toxischen Hydroxylradikals; Diamid, ein spezifisches Thiol-Oxidationsmittel, die Superoxidanion-generierende Substanz Paraquat, sowie der NO-Donor MAHMA NONOate. Für jeden Stressor wurden Proteomsignaturen durch Auftrennung der cytoplasmatischen Proteine mittels 2D-Proteingelelektrophorese und anschließender massenspektrometrischer Identifizierung erstellt. Die zu verschiedenen Zeitpunkten nach Stressauslösung neu synthetisierten Proteine wurden mittels L-[35S]-Methionin radioaktiv markiert und quantifiziert. Mindestens zweifach induzierte Proteine wurden als Markerproteine für einen bestimmten Stressor definiert. Durch Zugabe von 10 mM H2O2 wurden verstärkt Proteine synthetisiert, die an Synthese, Reparatur oder Schutz von Nukleinsäuren oder DNA beteiligt sind, was bestätigt, dass die DNA ein Hauptziel H2O2-induzierter Schädigung ist. Unter Einfluss von 10 nM Paraquat wurden Proteine mit sehr unterschiedlichen biologischen Funktionen, wie z.B. Aminosäuresyntheseenzyme und Cofaktoren, induziert. Der durch 1 mM Diamid induzierte Thiolstress führte wie erwartet zur verstärkten Neusynthese CtsR und HrcA-kontrollierter Chaperone und Proteasen, was auf die Akkumulation fehlgefalteter Proteine hindeutet, die höchstwahrscheinlich durch nichtnative Disulfidbrücken an den Thiolgruppen der Cysteinreste entstanden sind. Die Induktion von Peroxiredoxinen und einer Thioredoxinreduktase lassen auf ein gestörtes Redoxgleichgewicht in der Zelle schließen. Die Effekte von NO ähnelten denen, die auch unter Sauerstofflimitation beobachteten wurden. Viele Markerproteine sind in Glykolyse und Fermentation involviert und durch Nachweis der entsprechenden Fermentationsprodukte konnte eine höhere Aktivität fermentativer Stoffwechselwege bestätigt werden. Die Fähigkeit, unter Einfluss von NO auf anaeroben Metabolismus umzuschalten, könnte ein entscheidender Vorteil von S. aureus und essentiell für seine höhere Resistenz gegenüber NO sein.
A physiological proteomic approach to address infection-related issues of Gram-positive bacteria
(2012)
Trotz der vielen wissenschaftlichen Fortschritten sind Infektionskrankheiten auch heute noch die Haupttodesursache weltweit. Sie haben nicht nur heute, sondern werden auch in der Zukunft eine große epidemiologische Bedeutung haben. Die komplexe Infektionsthematik sollte unter zwei Gesichtspunkten betrachtet werden: der Prävention und der Behandlung. Zur Prävention von Infektionen zählen neben der Dekontamination und Sterilisation auch die Impfungen sowie die Hygiene- und Gesundheitsaufklärung. Bei der Behandlung von Infektionen kann auf Antibiotika zurückgegriffen werden, wenn das humane Immunsystem die Infektionen nicht auf natürliche Weise bekämpfen kann. Zwischen 1969 und 2000 wurde kein neues Antibiotikum den bereits vorhandenen Antibiotikaklassen hinzugefügt. Parallel zu dieser schwindenden Antibiotikaforschung, verbreiten sich nosokomiale Infektionen und community-acquired (vor allem Methicillin-resistente) Infektionen rapide. Von besonderer Bedeutung ist die Grundlagenforschung an infektionsassoziierten Mikroorganismen, wie dem humanen Erreger Staphylococcus aureus. Im Zusammenhang mit Infektionen spielen Virulenzfaktoren eine entscheidende Rolle. Sie sind entweder an der Zelloberfläche platziert oder werden aktiv ins Medium sekretiert. Um das pathogene Potential von S. aureus besser zu verstehen und aufzuklären ist ein Verständnis über die Proteintransportwege essentiell. Momentan sind die Transportwege von Escherichia coli (Gram-negative) und Bacillus subtilis (Gram-positive) am besten charakterisiert. Viele Transportwegekomponenten wurden mittels Transkriptions und Proteomeanalysen auch in S. aureus konserviert gefunden und ermöglichten dadurch einen ersten Einblick in die Sekretionsmaschinerie. Das Verständnis, warum und wie Virulenzfaktoren Infektionen auslösen birgt ein großes Potential in der Suche nach verbesserter Infektionskontrolle und Behandlung. Kontaminierte medizinische Arbeitsmittel, wie zum Beispiel Katheter oder Endoskope können auch eine auslösende Quelle von Infektionen sein. Diese medizinischen Arbeitsmittel oder Geräte bestehen immer häufiger aus bio-kompatiblen Polymeren (z.B. Polyethylen (PE) oder Polyethylenterephthalat (PET). Diese thermosensitive Polymere können keinen hohen Temperaturen ausgesetzt werden, ohne dass sie beschädigt werden. Damit sind herkömmliche Sterilisationsverfahren (z.B. Autoklavieren) nicht anwendbar. Alternative chemische Verfahren (z.B. Ethylenoxid-Sterilisation) sind mit Nebenwirkungen und Risiken verbunden, die im medizinischen Bereich nicht akzeptabel sind. Alternative Dekontaminationsverfahren für diese thermosensitive Materialen sind also gefragt. Hierbei rückt das Niedertemperaturplasma (NTP) nicht nur bei den Physikern sondern auch bei den Biologen und Medizinern immer weiter in den Fokus der Forschung. NTP, welches unter atmosphärischen Druck erzeugt wird, ist aus einer Vielzahl von antimikrobiell aktiven Agentien und chemischen Produkten (z.B. atomarer Sauerstoff (O), Ozon (O3), Hydroxyl (OH), reaktive Sauerstoffspezies (ROS) und reaktive Stickstoffspezies (RNS)) zusammengesetzt und stellt damit ein wirksames Mittel für die mikrobielle Dekontamination dar. Seit einiger Zeit wird NTP auch erfolgreich bei der Wundbehandlung angewendet. Erste Studien zeigen ein großes Potential von NTP-Wundbehandlungen in Hinblick auf verbesserte Wundheilung. Die Anwendung von Plasma in der Medizin könnte ganz neue Perspektiven eröffnet- das ist zumindest die Vision. Auf der praktischen Seite gibt es allerdings noch eine Vielzahl von offenen Fragen: (i) welche Art von Plasma ist für welchen Zweck am besten geeignet; (ii) was sind die Vorteile von Plasma im Vergleich zu gängigen medizinischen Behandlungen; (iii) ist Plasma ein ökonomische Alternative im Vergleich zu gängigen Anwandelungen und Standards? Bevor Plasma sicher und routinemäßig in Krankenhäusern zu Einsatz kommen kann ist es zusätzlich von größter Wichtigkeit den Einfluss von Plasma auf Zellen zu klären. Erst wenn die Plasma-Zell-Interaktion (pro- und eukaryotische Zellen) grundsätzlich untersucht und verstanden ist kann eine sichere, erfolgreiche und vor allem akzeptierte Implementierung in den Krankenhausalltag stattfinden.
Die reverse Genetik ist ein wichtiges Werkzeug in der Grundlagenforschung und Impfstoffentwicklung der Influenza-A- und -B-Viren. Oft ist der limitierende Schritt für die Erstellung eines solchen Systems der reversen Genetik, bestehend aus mehreren Plasmiden für die einzelnen Gensegmente, die Klonierung der Virusgene in den Expressionsvektor. Für eine schnellere und einfachere Klonierung wurde in dieser Arbeit das LacZa-Fragment mittels modifizierter QuikChange-Reaktion in den Klonierungsvektor pHWSccdB inseriert. Mit dem so entstandenen Vektor pHWSccdBLacZa ist es nun möglich, zusätzlich eine Blau/Weiß-Selektion durchzuführen. Beider target-primed plasmid amplification zur Insertion des viralen Gensegmentes werden hierbei die beiden Selektionsmarker ccdB und LacZa durch das virale Gen ersetzt. Bakterienkolonien mit kloniertem Gensegment können von denen ohne komplettes Insert nun leichter und frühzeitiger durch eine nicht vorhandene Blaufärbung unterschieden werden. Schweine spielen in der Influenzavirus-Transmission eine besondere Rolle, da sie als sog. „mixing vessel“ gelten. Sie können z. B. Reassortanten aus aviären und porzinen Influenzaviren auf den Menschen übertragen, die sich bei einer zeitgleichen Infektion mit beiden Viren im Schwein bilden können. In dieser Arbeit wurden die seit 1979 in Europa zirkulierenden aviären H1N1- Schweineviren betrachtet. Sie sind Schweinestämme, deren Gene von einem aviären Vorläufervirus abstammen. Unter dem Ziel der Untersuchung der molekularen Determinanten des Wirts-Tropismus dieser aviären H1N1-Schweineviren wurden Reassortanten und Zufallsressortanten hergestellt unter Verwendung des aviären Virus A/Duck/Bavaria/1/77 (H1N1) (DkBav) und des aviären Schweinevirus A/Swine/Belgium/1/79 (H1N1) (SwBelg). Zunächst wurde die Replikationseffizienz von DkBav, SwBelg und den hergestellten Reassortanten auf einer aviären und einer porzinen Zelllinie untersucht. Hierbei wurde festgestellt, dass für das aviäre Virus DkBav das HA von SwBelg ausreicht, um in porzinen Zellen das Wachstumsniveau von SwBelg zu erreichen. Das HA-Segment ist also entscheidend für den Wirtstropismus von DkBav in einer porzinen Zelllinie. Experimente im Schwein zeigten jedoch, dass DkBav nicht alleine durch das HA von SwBelg zu einem Schweinevirus wird. Für diese Experimente wurden Schweine intranasal mit den hergestellten Viren, SwBelg und DkBav infiziert. Um die Replikation im Schwein zu steigern, benötigt DkBav zusätzlich zum HA noch das NA von SwBelg und für die Transmission von Schwein zu Schwein das NP sowie eines oder mehrere der anderen Gensegmente von SwBelg. Für eine starke Virusvermehrung in der Lunge benötigt DkBav den Polymerasekomplex, HA und NA von SwBelg. Für die Transformation in ein Schweinevirus benötigt DkBav also kein bestimmtes Gensegment, sondern eine Kombination mehrerer Gensegmente. Für hochpathogene aviäre Influenzaviren ist die polybasische Spaltstelle des Oberflächenproteins HA der wichtigste Virulenzfaktor. Das HA ist u. a. für die Bindung und die Fusion der Endosomenmembran von Influenzaviren mit der Wirtszelle zuständig. Da eine polybasische HA-Spaltstelle alleine jedoch nicht ausreicht, um die Virulenz eines LPAIV deutlich zu erhöhen, wurde in dieser Arbeit nach weiteren Virulenzdeterminanten im HA des hochpathogenen Influenzavirus A/Swan/Germany/R65/2006 (H5N1) (R65wt) zusätzlich zur polybasischen Spaltstelle gesucht. Hierzu wurden von den Viren R65wt und A/Teal/Germany/Wv632/2005 (H5N1) mit eingesetzter polybasischer Spaltstelle (TG05poly) verschiedene HA-Chimären und -Mutanten hergestellt und diese in vitro und in vivo untersucht. Dabei wurde festgestellt, dass die eingefügten Mutationen nicht ausreichten, um TG05poly zu einem hochpathogenen Virus zu machen. Für das hochpathogene Virus R65wt wurden die Aminosäuren HA-R123 und HAI124 als weitere Virulenzdeterminanten identifiziert. Bei HA-Sequenz- und HAStrukturanalysen wurde festgestellt, dass die Aminosäuren HA-123 und HA-124 innerhalb des niedrigpathogenen bzw. des hochpathogenen Phänotyps hoch konserviert vorliegen. Mutationen an diesen Positionen verringern nicht nur HA-Aktivierungs-pH und Virus-Inaktivierungs-pH deutlich, sondern auch die Letalität des Virus um fast 50 % (HA-I124T) oder das Virus wurde sogar avirulent (HA-R123S). Im Falle einer polybasischen Spaltstelle ist also eine erhöhte pH-Stabilität des HA vermittelt durch die Aminosäure R123 essentiell für die Entstehung eines hochpathogenen aviären H5N1-Virus aus einem niedrigpathogenen Vorläufer.
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.
Introduction: Inhibition of androgen synthesis by abiraterone acetate (AA) entails enhanced overall survival rates and clinical benefit for patients with locally advanced and metastasized prostate cancer (PC). The expression of heat shock protein 27 (HSP27) is generally associated with cytoprotection and was demonstrated to mediate chemoresistance under cytostatic therapy, for instance, docetaxel treatment. In this study, we investigated the impact of AA treatment on HSP27 expression and PC cell growth. Materials and Methods: HSP27 expression levels in docetaxel and AA-treated PC cell lines LNCaP and PC-3 were determined by SDS PAGE and Western blot analysis. Proliferation assays were performed using a CASY Cell Counter and Analyzer Model TT (Roche Applied Science). Results: Despite significantly increased HSP27 expression in PC cells incubated with docetaxel, Western blot analysis implicated a significant reduction of the cytoprotective HSP27 in AA-treated PC cells. Notably, HSP27 stably overexpressed in PC-3-HSP27 cells did not appear as an HSP27-mediated proliferation benefit in the presence of AA as shown in docetaxel incubation studies. Conclusion: In contrast to repeatedly demonstrated HSP27-driven chemoresistance related to chemotherapeutics, our results may constitute a broader molecular mode of action of AA chemotherapy. AA efficacy may exert an HSP27 suppressive role that goes beyond the primarily assumed inhibition of androgen biosynthesis.
Im Rahmen der vorliegenden Arbeit wurden BVDV-Mutanten mit Deletionen, Insertionen oder Substitutionen in der E(rns)-kodierenden Genomregion ausgehend von den infektiösen cDNA-Klonen pA/BVDV und pA/BVDV/Ins- (Meyers et al., 1996) generiert. Die meisten Veränderungen verhinderten die Entstehung infektiöser Virionen, so dass nichtessentielle Regionen im E(rns)-Protein nicht identifiziert werden konnten. Eine Ausnahme stellen die Aminosäuren 105-108 dar, deren Substitution im Zusammenhang mit adaptiven Mutationen toleriert wurde. Mit Hilfe von Zelllinien, die die BVDV-Strukturproteine konstitutiv exprimieren, konnte eine Mutante mit einer kompletten E(rns)-Deletion und einer internen EMCV-IRES im Genom effizient trans-komplementiert und sogenannte DISC-Viren erhalten werden. Außerdem wurden Plasmide für die Expression der BVDV-Strukturproteine (C, E(rns), E1, E2) hergestellt, mit deren Hilfe erstmals ein nicht-prozessiertes E(rns)-E1-Protein mit 60-65 kDa identifiziert werden konnte, das für mindestens 3 h relativ stabil in transfizierten Zellen vorlag. Durch Mutation der P3-Position eines SPP-Motivs gelang es, sowohl in pCITE-2a(+)-Expressionsplasmiden als auch in BVDV-Vollängen-Mutanten die Spaltung dieses E(rns)-E1-Proteins zu verhindern. Dadurch konnte gezeigt werden, dass die E(rns)-E1-Spaltung essentiell für die Bildung infektiöser Viren ist. Bicistronische Mutanten wurden genutzt, um zu zeigen, dass das E(rns)-E1-Protein selbst jedoch nicht notwendig, aber förderlich für Entstehung infektiöser Virionen ist. Weiterhin konnte mittels eines im Rahmen dieser Arbeit generierten polyklonalen Bungowannah Virus-E(rns)-spezifischen Kaninchenserums, das E(rns)-Protein des atypischen Pestivirus Bungowannah Virus in Western Blot-Analysen mit etwa 38 kDa detektiert werden. Da jedoch kein Bungowannah Virus-E(rns)-E1-Protein nachgewiesen werden konnte, spielt E(rns)-E1 möglicherweise keine oder eine untergeordnete Rolle im Bungowannah Virus-Replikationszyklus. BVDV-E(rns)-Deletionen im CP7-Hintergrund konnten erfolgreich mit Bungowannah Virus-E(rns) komplementiert werden, wenn Bungowannah Virus-E(rns) und BVDV-E1 unabhängig von einer E(rns)-E1-Spaltung exprimiert wurden. Ein weiterer Schwerpunkt dieser Arbeit war es schließlich, eine effiziente Methode zur Konzentrierung und Reinigung infektiöser BVDV aus infizierten Zellen zu etablieren. Zum ersten Mal wurden BVDV-Mutanten mit FLAG-markierten E(rns)- und E2-Proteinen generiert, so dass erstmalig BVDV mittels Affinitätschromatografie gereinigt und elektronenmikroskopisch untersucht werden konnten. Mittels Negativkontrast-Elektronenmikroskopie wurden sphärische Partikel mit Durchmessern von 43-58 nm dargestellt. Sowohl durch affinitätschromatografische Virusreinigung als auch durch immunelektronenmikroskopische Untersuchungen konnte eine Assoziation von E(rns)- und E2-Proteinen mit der BVD-Virushülle demonstriert werden. Die in dieser Arbeit vorgestellte Methode kann als Basis für weiterführende Untersuchungen zur Morphogenese von Pestiviren genutzt werden.
The impact of summer drought on peat soil microbiome structure and function-A multi-proxy-comparison
(2022)
Different proxies for changes in structure and/or function of microbiomes have been developed, allowing assessing microbiome dynamics at multiple levels. However, the lack and differences in understanding the microbiome dynamics are due to the differences in the choice of proxies in different studies and the limitations of proxies themselves. Here, using both amplicon and metatranscriptomic sequencings, we compared four different proxies (16/18S rRNA genes, 16/18S rRNA transcripts, mRNA taxonomy and mRNA function) to reveal the impact of a severe summer drought in 2018 on prokaryotic and eukaryotic microbiome structures and functions in two rewetted fen peatlands in northern Germany. We found that both prokaryotic and eukaryotic microbiome compositions were significantly different between dry and wet months. Interestingly, mRNA proxies showed stronger and more significant impacts of drought for prokaryotes, while 18S rRNA transcript and mRNA taxonomy showed stronger drought impacts for eukaryotes. Accordingly, by comparing the accuracy of microbiome changes in predicting dry and wet months under different proxies, we found that mRNA proxies performed better for prokaryotes, while 18S rRNA transcript and mRNA taxonomy performed better for eukaryotes. In both cases, rRNA gene proxies showed much lower to the lowest accuracy, suggesting the drawback of DNA based approaches. To our knowledge, this is the first study comparing all these proxies to reveal the dynamics of both prokaryotic and eukaryotic microbiomes in soils. This study shows that microbiomes are sensitive to (extreme) weather changes in rewetted fens, and the associated microbial changes might contribute to ecological consequences.
Innerhalb der vorliegenden Arbeit wurden verschiedene Bakterien- und Hefestämme der Stammsammlung Biologie des Institutes für Mikrobiologie der Ernst-Moritz-Arndt-Universität Greifswald (SBUG) auf einen Umsatz von 9H-Carbazol untersucht. Neben Ralstonia spec. SBUG 290, Rhodococcus erythropolis SBUG 271 sowie den zwei im Rahmen dieser Arbeit als Pseudomonas putida identifizierten Stämmen SBUG 272 und SBUG 295 zählten zu den Bakterienstämmen 22 weitere noch nicht abschließend charakterisierte Isolate. Die geprüften Hefestämme umfassten neben 7 Vertretern der Gattung Trichosporon auch 19 nicht identifizierte Stämme. Basierend auf der für diese Mikroorganismen bereits nachgewiesenen Verwertung von Biphenyl beziehungsweise Dibenzofuran bestand die Hypothese, dass diese Stämme aufgrund von Strukturanalogien der Substrate auch in der Lage sind, weitere Heterozyklen zu transformieren. Angesichts des sehr breiten pharmakologischen Wirkungs- und Anwendungsspektrums von Carbazol-Derivaten wurde primär geprüft, inwieweit sich mit Hilfe dieser spezialisierten Mikroorganismen hydroxylierte Carbazol-Derivate als Ausgangssubstanzen für spätere Synthesen herstellen lassen. Da die verwendeten Bakterien im Gegensatz zu den Hefen zu einer Transformation von 9H-Carbazol befähigt waren, wurden mit diesen Stämmen Untersuchungen zur mikrobiellen Transformation von insgesamt 9 zusätzlichen stickstoffhaltigen Biarylverbindungen (2,3,4,9-Tetrahydro-1H-carbazol, 9-Methyl-9H-carbazol, Carbazol-9-yl-methanol, Carbazol-9-yl-essigsäure, 3-Carbazol-9-yl-propionsäure, 2-Carbazol-9-yl-ethanol, Acridin, 10H-Acridin-9-on, Phenazin) durchgeführt. Aufgrund der im Unterschied zu bisherigen Publikationen zum Umsatz von Biarylen festgestellten abweichenden Produktbildung bei Inkubation mit 9H-Carbazol wurden die Bakterienstämme für vergleichende Analysen ebenfalls auf die Transformation von Dibenzothiophen sowie 9H-Fluoren geprüft. Insgesamt wurden bei der Transformation der getesteten Biarylverbindungen 55 Produkte untersucht, von denen 34 bislang für Bakterien noch nicht beschrieben wurden. Basierend auf GCMS-, LCMS- und NMR-Analysen konnten insgesamt 29 Verbindungen identifiziert und für 14 Transformationsprodukte anhand der erhaltenen Daten vorläufige Strukturvorschläge unterbreitet werden. Zusätzlich wurde im Rahmen dieser Arbeit für weitere 8 der in den Versuchen gebildeten Produkte bereits eine erste strukturanalytische Charakterisierung vorgenommen. In weiterführenden Versuchen wurden die durch die Bakterienstämme gebildeten Produkte als Substrate eingesetzt, um zu analysieren auf welche Weise die über primäre Hydroxylierungsreaktionen hinausgehenden Transformationen dieser Substanzen erfolgen. Dazu wurden, in erster Linie am Beispiel von Ralstonia spec. SBUG 290, insgesamt 28 der gebildeten Produkte auf einen weiteren Umsatz geprüft, darunter 14 Substanzen, die kommerziell nicht verfügbar sind und daher zuvor in größeren Mengen aus den Transformationsansätzen gereinigt wurden. Basierend auf diesen Untersuchungen konnten schließlich anhand der nachgewiesenen Produkte Aussagen zu den durch die Stämme katalysierten Transformationswegen abgeleitet werden. In Versuchen mit dem rekombinanten Stamm Escherichia coli DH5alpha SBUG 1575, der die Gene bphA1–A3 der Biphenyl-2,3-dioxygenase aus Ralstonia spec. SBUG 290 trägt, wurde die Beteiligung dieses Enzyms am Umsatz der eingesetzten Biarylverbindungen untersucht.
Streptococcus pneumoniaeinfections lead to high morbidity and mortality rates worldwide.Pneumococcal polysaccharide conjugate vaccines significantly reduce the burden of disease but havea limited range of protection, which encourages the development of a broadly protective protein-basedalternative. We and others have shown that immunization with pneumococcal lipoproteins that lackthe lipid anchor protects against colonization. Since immunity againstS. pneumoniaeis mediatedthrough Toll-like receptor 2 signaling induced by lipidated proteins, we investigated the effects ofa lipid modification on the induced immune responses in either intranasally or subcutaneouslyvaccinated mice. Here, we demonstrate that lipidation of recombinant lipoproteins DacB and PnrAstrongly improves their immunogenicity. Mice immunized with lipidated proteins showed enhancedantibody concentrations and different induction kinetics. The induced humoral immune responsewas modulated by lipidation, indicated by increased IgG2/IgG1 subclass ratios related to Th1-typeimmunity. In a mouse model of colonization, immunization with lipidated antigens led to a moderatebut consistent reduction of pneumococcal colonization as compared to the non-lipidated proteins,indicating that protein lipidation can improve the protective capacity of the coupled antigen. Thus,protein lipidation represents a promising approach for the development of a serotype-independentpneumococcal vaccine.
Permafrost-affected soil stores a significant amount of organic carbon. Identifying the biological constraints of soil organic matter transformation, e.g., the interaction of major soil microbial soil organic matter decomposers, is crucial for predicting carbon vulnerability in permafrost-affected soil. Fungi are important players in the decomposition of soil organic matter and often interact in various mutualistic relationships during this process. We investigated four different soil horizon types (including specific horizons of cryoturbated soil organic matter (cryoOM)) across different types of permafrost-affected soil in the Western Canadian Arctic, determined the composition of fungal communities by sequencing (Illumina MPS) the fungal internal transcribed spacer region, assigned fungal lifestyles, and by determining the co-occurrence of fungal network properties, identified the topological role of keystone fungal taxa. Compositional analysis revealed a significantly higher relative proportion of the litter saprotroph Lachnum and root-associated saprotroph Phialocephala in the topsoil and the ectomycorrhizal close-contact exploring Russula in cryoOM, whereas Sites 1 and 2 had a significantly higher mean proportion of plant pathogens and lichenized trophic modes. Co-occurrence network analysis revealed the lowest modularity and average path length, and highest clustering coefficient in cryoOM, which suggested a lower network resistance to environmental perturbation. Zi-Pi plot analysis suggested that some keystone taxa changed their role from generalist to specialist, depending on the specific horizon concerned, Cladophialophora in topsoil, saprotrophic Mortierella in cryoOM, and Penicillium in subsoil were classified as generalists for the respective horizons but specialists elsewhere. The litter saprotrophic taxon Cadophora finlandica played a role as a generalist in Site 1 and specialist in the rest of the sites. Overall, these results suggested that fungal communities within cryoOM were more susceptible to environmental change and some taxa may shift their role, which may lead to changes in carbon storage in permafrost-affected soil.
Herpesviruses are a fascinating group of enveloped DNA viruses, which rely on membrane fusion for infectious entry and direct cell-to-cell spread. Compared with many other enveloped viruses, they utilize a remarkably complex fusion machinery. Three conserved virion proteins, the bona fide fusion protein gB, and the presumably gB activating gH/gL heterodimer constitute the conserved core fusion machinery and are believed to drive membrane fusion in a cascade-like fashion. Activation of this cascade in most alphaherpesviruses is proposed to be triggered by binding of gD to specific host cell receptors. The molecular details of this fusion process, however, remain largely elusive. Yet, a detailed mechanistic knowledge of this process would be greatly beneficial for the development of efficient countermeasures against a variety of diseases. In this thesis, the functional relevance of individual components of the essential gH/gL complex of the alphaherpesvirus PrV has been assessed by two different approaches: by reversion analysis (paper II) and site-directed mutagenesis (papers III-V). In contrast to other herpesviruses, gL-deleted PrV is able to perform limited cell-to-cell spread, providing the unique opportunity to passage the entry-deficient virus in cell culture to select for PrV revertants capable of infecting cells gL-independently. This approach already resulted in an infectious gL-negative PrV mutant (PrV-ΔgLPass), in which the function of gL was compensated by formation of a gDgH hybrid protein. Here, the requirements for gL-independent infectivity of a second independent revertant (PrV-ΔgLPassB4.1), were analyzed. Sequencing of the genes encoding for gB, gH and gD, revealed mutations in each of them. By means of a robust infection-free, transfection-based cell-cell fusion assay (paper I), we identified two amino acid substitutions in the gL-binding domain I of gHB4.1 (L70P, W103R) as sufficient to compensate for lack of gL. Two mutations in gB (G672R, ΔK883) were found to enhance fusogenicity, probably by lowering the energy, required for gB refolding from pre- to postfusion conformation. Coexpression of gHB4.1 and gBB4.1 led to an excess fusion, which was completely suppressed by gDB4.1 in the fusion assays. This was surprising since PrV gD is normally not required for in vitro fusion or direct viral cell-to-cell spread, clearly separating this process from fusion during entry, for which PrV gD is essential. The fusion inhibiting effect of gDB4.1 could be attributed to a single point mutation resulting in an amino acid substitution within the ectodomain (A106V). In conclusion, these results indicated that gL is not central to the fusion process, as its function can be compensated for. As found so far, gL-independent infectivity can be realized by compensatory mutations in gH (as in PrV-ΔgLPass) or in gH plus gB (as in PrV-ΔgLPassB4.1). Excessive fusion induced by gHB4.1 and gBB4.1 was counter-regulated by gDB4.1, indicating that the interplay between these proteins is precisely regulated and further implies that gL and gD, despite being not absolutely essential for the fusion process, have important regulatory functions on gH and/or gB.
Both PrV-ΔgLPass mutants had acquired compensatory mutations in gH affecting the predicted gL-binding domain I in gH. By construction of an artificial gH32/98, which lacked the predicted gL-binding domain and was similar to the recently crystallized gH-core fragment present in the gDgH hybrid protein, we identified the N-terminal part of PrV gH as essential for gH function during fusion (paper III). gH32/98 was unable to promote fusion of wild-type gB in fusion assays and led to a total loss of function in the viral context. These results indicated that the gD moiety, present in gDgH, is critical for proper function of the gH-core fragment. We hypothesize that the gD moiety may adopt a stabilizing or modulating influence on the gH structure, which is normally executed by gL and important for interaction of gH with wild-type gB. Remarkably, substitution of wild-type gB by gBB4.1 rescued function of gH32/98 in the cellular and viral contexts. These findings suggest that gBB4.1 has been selected for interaction with “gL-less” gH. In conclusion, these results demonstrated that gL and the gL-binding domain are not strictly required for membrane fusion during virus entry and spread but that compensatory mutations must be present in gB to restore a fully functional fusion machinery. These results strongly support the notion of a functional gH-gB interaction as a prerequisite for membrane fusion.
In addition to the N-terminal domain, we identified the transmembrane domain of PrV gH as an essential component of the fusion machinery, while the cytoplasmic domain was demonstrated to play a modulatory but nonessential role (paper IV). Whereas truncation or substitution of the PrV gH TMD by a gpi-anchor or the analogous sequence from PrV gD rendered gH non-functional, the HSV-1 gH TMD was found to functionally substitute for the PrV gH TMD in cell-cell fusion and complementation assays. Since residues in the TMD which are conserved between HSV and PrV gH but absent in PrV gD, are placed on one face of an α-helical wheel plot, we hypothesize that the gH TMD has an intrinsic property to interact with membrane components such as lipids or other molecules as a requirement for promoting membrane fusion.
In a final study focusing on the function of gH, we identified the N-glycosylation sites utilized by PrV gH, and determined their individual role in viral infection (paper V). PrV gH was found to be modified by N-glycans at five potential glycosylation sites. N-glycans at PrV specific N77 and the highly conserved site N627 were found to be critical for efficient membrane fusion in the fusion assays, and during viral entry and cell-to-cell spread. N627 was further shown to be crucial for proper gH transport and maturation. In contrast, inactivation of N604, conserved in the Varicellovirus genus, enhanced in vitro fusion activity and viral cell-to-cell spread. These findings demonstrated a role of the N-glycans in proper localization and function of PrV gH.
Linking transcriptional dynamics of CH4-cycling grassland soil microbiomes to seasonal gas fluxes
(2022)
Soil CH4 fluxes are driven by CH4-producing and -consuming microorganisms that determine whether soils are sources or sinks of this potent greenhouse gas. To date, a comprehensive understanding of underlying microbiome dynamics has rarely been obtained in situ. Using quantitative metatranscriptomics, we aimed to link CH4-cycling microbiomes to net surface CH4 fluxes throughout a year in two grassland soils. CH4 fluxes were highly dynamic: both soils were net CH4 sources in autumn and winter and sinks in spring and summer, respectively. Correspondingly, methanogen mRNA abundances per gram soil correlated well with CH4 fluxes. Methanotroph to methanogen mRNA ratios were higher in spring and summer, when the soils acted as net CH4 sinks. CH4 uptake was associated with an increased proportion of USCα and γ pmoA and pmoA2 transcripts. We assume that methanogen transcript abundance may be useful to approximate changes in net surface CH4 emissions from grassland soils. High methanotroph to methanogen ratios would indicate CH4 sink properties. Our study links for the first time the seasonal transcriptional dynamics of CH4-cycling soil microbiomes to gas fluxes in situ. It suggests mRNA transcript abundances as promising indicators of dynamic ecosystem-level processes.
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.
Degradation of branched chain aliphatic and aromatic petroleum hydrocarbons by microorganisms
(2008)
The overall aim of the work was to investigate the ability of several Gram-positive bacteria including Mycocbacterium neoaurum SBUG 109, Nocardia cyriacigeorgica SBUG 1472 and Rhodococcus ruber SBUG 82 and the yeast Trichosporon mucoides SBUG-Y 801 to degrade and transform branched chain hydrocarbons which occur in petroleum and its fraction products such as gasoline or gas oil and which are known as important and recalcitrant environmental pollutants. Pristane, iso-pentylbenzene and sec-octylbenzene were used in this work as model compounds. These compounds represent significant groups of petroleum constituents (branched chain alkanes and aromatic hydrocarbons). Three bacteria and the yeast T. mucoides SBUG-Y 801 were selected in a screen of 16 hydrocarbon-utilizing strains in the SBUG collection and from 21 isolated hydrocarbon-utilizing strains from oil-contaminated habitats of Saudi Arabian Desert and of Vietnam. The bacteria were identified in cooperation with DSZM (Deutsche Sammlung von Mikroorganismen und Zellkulturen) as M. neoaurum SBUG 109, N. cyriacigeorgica SBUG 1472, R. ruber SBUG 82. These bacterial and yeast strains were shown to possess high potential for degrading and transforming pristane, iso-pentylbenzene and sec-octylbenzene. The intermediates produced by these bacteria during incubation with pristane were analyzed by GC and GC/MS. The products 4-methyl pentanoic acid; methyl butanedioic acid; 2-methyl pentadioic acid; methyl propanedioic acid; 4-methyl heptanedioic acid and 2,6,10,14–tetramethyl-pentadecan–3–one were detected in M. neoaurum cultures. In R. ruber, methyl butanedioic acid; 2-methyl pentadioic acid; 4,8-dimethylnonanoic acid, 4-methyl heptanedioic acid; 2,6,10–trimethylundecanoic acid; 3,7-dimethyl decanedioic acid and 2,6,10,14–tetramethyl–pentadecan–3-one were identified. In N. cyriacigeorgica, 2-methylpentanedioic acid; 4,8-dimethylnonanedioic acid; 2,6-dimethylheptanedioic acid and pristanic acid were found. The detection of 11 intermediates during pristane degradation by the three Gram-positive bacteria provided sufficient information to elucidate in detail three degradative pathways of pristane involving mono-, di- and sub-terminal oxidations. The sub-terminal oxidation by M. neoaurum and R. ruber was demonstrated for the first time. This occurence of a sub-terminal oxidation in these strains was strengthened by further results of aromatic compounds transformation (see below). During this pathway, ketone mono-oxygenation reactions seem to be involved. Because of this it will be of interest to look more closely at the catalytic processes involved and their possible extension to the bio-degradation of other branched chain hydrocarbons. Since in the present study 59 %, 51 % and 84 % of pristane were degraded in 3 weeks by M. neoaurum, R. ruber and N. cyriacigeorgica, this illustrated that the degradation rates of this isoprenoid alkane were high. The bacteria we studied were not only effective degraders of multiple branched chain alkane but also useful transformers of aromatic hydrocarbons. The intermediates produced were analyzed by comparing the retention times and UV/Vis spectra of the HPLC elution profile as well as the retention times and mass spectra of the GC/MS with those of available standards. Using iso-pentylbenzene as a substrate, 8 metabolites were generated by M. neoaurum transformation including product A (phenylacetic acid), B (acetophenone), D (iso-valerophenone), E (succinic acid), F (benzoic acid), G [(2-hydroxy-phenyl)-acetic acid] and H (2-methyl-4-phenyl-butyric acid). We additionally identified an alkyl hydroxylated iso-pentylbenzene derivative as 2-methyl-4-phenyl-butan-2-ol or 2-methyl-4-phenyl-butan-1-ol. Two metabolites (C and D) were detected by N. cyriacigeorgica transformation and three metabolites (A, D and F) were identified by R. ruber transformation which led to the complete biotransformation of this substance. iso-Pentylbenzene transformation by M. neoaurum was initiated by attack on the alkyl side chain followed by ring cleavage. The appearance of iso-valeorophenone confirmed the occurrence of a sub-terminal oxidation mechanism in M. neoaurum and R. ruber. In addition to products A, C, D and G, the identification X-(3–methyl–butyl)-phenol (X means that position of the hydroxy group on the aromatic ring system, such as 2, 3 or 4 remained unclear) in T. mucoides cultivation demonstrated for the first time the capacity of alkyl side chain attack by this organism which was hitherto known only for its ability of ring cleavage. The detection of 15 degradation products of sec-octylbenzene (including 2-phenylpropionic acid, 3-phenylbutyric acid, ß-methylcinnamic acid, 5-phenylhexanoic acid, acetophenone, 2-hydroxy-acetophenone, 2,3-dihydroxy-benzoic acid, succinic acid, 7-phenyloctan-2-one, benzoic acid, phenylacetic acid, 7-phenyl-octan-2-ol, hydroxy-phenylacetic acid and 2-hydroxybenzoic acid), in the studied bacteria pointed to an effective sec-octylbenzene degradation pathway in which dehydrogenation of 3-phenylbutyric acid to form ß-methylcinnamic acid is a newly described option. The identification of 2-phenylpropionic acid and 3-phenylbutyric acid in sec-octylbenzene transformation experiments by T. mucoides confirmed the possibility of alkyl side chain attack by this yeast. Summarizing the results, we describe for the first time in detail the biotransformation of sec-octylbenzene by M. neoaurum, N. cyriacigeorgica, R. ruber and T. mucoides. Our results suggest that these microorganisms may be useful as potential strains for hydrocarbon degradation and it may be of interest to investigate their suitability to solve specific environmental pollutant problems associated with branched chain aliphatic and alkyl-branched compounds which contribute to the persistence of hydrocarbon fractions in the environment.