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Understanding of the regulatory mechanisms controlling stress gene expression of S.aureus in response to environmental stress is very essential in studying its fitness and virulence. In this work, the changes in protein expression profiles as well as the gene transcription of S.aureus after heat exposure, osmotic stress and in response to the antibiotic puromycin were studied in order to provide detailed insights into the response of S.aureus to various kinds of environmental stress under in vitro conditions, namely: (1) to investigate the global response of S.aureus to heat stress conditions using transcriptomic and proteomic analyses. (2) to study the transcriptome and proteome of S.aureus in response to antibiotic substance puromycin. (3) to define the proteome signatures of S.aureus under NaCl stress condition. (4) to complete the proteome map of cytoplasmic proteins of S.aureus by identifying proteins exclusively synthesized during the exposure to stress. Firstly, the high resolution 2-D protein gel electrophoresis technique combined with MALDI-TOF-MS and a DNA array approach were used to investigate the cellular response of S.aureus to heat stress. A switch from normal growth temperature to high temperature condition revealed complex changes in the protein expression pattern as well as the genes expression profile. The effect of puromycin stress on S.aureus cells was analyzed, using a gel-based proteomic approach and transcriptomic analyses with DNA microarrays. We compared the protein synthesis pattern as well as the transcription data of S.aureus in response to puromycin stress with that in response to heat shock. The results demonstrated that both stress conditions induced specific, overlapping and general responses. Finally, the protein expression profile of S.aureus in response to NaCl stress was analyzed with 2D gel based proteomic approach. Our proteome analyses revealed the repression of the synthesis of many enzymes belong to different metabolism pathways . In summary, the signatures for stress or starvation stimuli can be used as diagnostic tools for the prediction of the mode of action of new antibiotics or for studying the physiological state of cells grown. Expression of the respective genes under in vivo conditions could provide some ideas on the environmental signals that specifically influence the survival of S.aureus within and outside the host.
In the post genomic era, novel “Omics” technologies like genomics and proteomics can be used in powerful screening approaches to provide unbiased lists of candidate genes and proteins and thus facilitate a comprehensive analysis of complex diseases such as cancer, which would not have been possible applying traditional genetic and biochemical approaches alone. During my PhD tenure I applied functional genomics screening technologies including proteomics in combination with traditional biochemical and cell biology approaches in two disease oriented projects: 1. Characterization of the role of BCL11b in Human T cell lymphomas (and) 2. Elucidation of the mechanism of pathophysiology of Johanson Blizzard Syndrome using UBR1 knockout mice and JBS patients’ lymphoblasts cell lines.
1.Characterization of the role of BCL11b in Human T cell lymphomas
: The Bcl11b protein belongs to the C2H2-family of Krueppel-like zinc finger proteins and thus is a member of the largest family of transcription factors in eukaryotes. It was shown to be important for a variety of functions such as T cell differentiation, normal development of central nervous system and DNA damage response. Malignant T cells undergo apoptotic cell death upon BCL11B down-regulation. However, the detailed mechanism of this cell death is not fully understood. Two dimensional difference in-gel electrophoresis (2D-DIGE), mass spectrometry and cell biological experiments were employed to investigate the functional impact of knock down of BCL11B in malignant T cell lines such as Jurkat and huT78. To further confirm the findings of these experiments, changes in protein patterns were also recorded after down-regulation of BCL11B expression in Jurkat cells over expressing BcL-xL and in Jurkat cells over expressing BCL11B. These experiments provide evidence for the involvement of the mitochondrial apoptotic pathway and increased levels of cleavage fragments of known caspase targets such as myosin, spectrin and vimentin were observed after BCL11B knockdown. The findings suggest an involvement of ERM proteins, which were up-regulated and phosphorylated upon BCL11B down-regulation. Besides ERM proteins, PDCD5, a key regulator of apoptosis, was also found at increased levels upon down regulation of BCL11B. Moreover, the levels of several proteins implicated in cell cycle entry, including DUT-N, UCK2, MAT1, CDK6, MCM4 and MCM6 were elevated, which might lead to uncontrolled cell cycle progression, uracil misincorporation and cell death. Interestingly, an inverse regulation pattern, i.e. decreased levels of ERM proteins, DUT-N, UCK2 and PDCD5 was seen upon over expression of BCL11B in Jurkat cells. In summary, proteome analyses revealed several previously unidentified mechanisms which could significantly contribute to the cell death following BCL11B knockdown.
2.Elucidation of the mechanism of pathophysiology of Johanson Blizzard Syndrome using UBR1 knockout mice and JBS patients’ lymphoblasts cell lines
: Johanson-Blizzard syndrome (JBS; OMIM 243,800), which was first described in 1971, is a rare autosomal recessively inherited genetic disorder with a unique combination of congenital abnormalities. The most constant clinical feature of JBS is the loss of exocrine pancreatic function due to progressive destruction of pancreatic acini. Genome wide linkage analysis identified the disease associated locus in the 15q14-q21 chromosome region and high-throughput sequencing of this region revealed several truncated and some missense mutations in the UBR1 gene. UBR1 gene contains 47 exons and spans over 161 kilobases. The UBR1 protein belongs to the E3 ubiquitin ligase family and is an important component of the N-end rule pathway of ubiquitous protein degradation. It was hypothesized that stabilization of direct and unique substrates of UBR1 could be the main cause of the JBS pathophysiology. So far sequencing of the UBR1 gene is the only available diagnostic procedure. However, sequencing might not always allow precise prediction of residual UBR1 activity. Hence, this study was started to develop a protein based diagnostic assay for the detection of subclinical cases of JBS and to identify signalling pathways contributing to the pathophysiology of this complex disorder using a murine UBR1 knockout model. 2D-DIGE proteome analysis was carried out for a comparative evaluation of lymphoblast samples of 14 patients and 11 controls. Principal component Analysis (PCA) clearly discriminated JBS patients from controls. However, 4 JBS patients differed from the rest and resembled controls more closely. Western-blot analysis revealed residual UBR1 levels in these patients, which were linked to a milder phenotype. Hierarchical clustering of the three groups (controls, patients with residual UBR1 levels and patients without UBR1) showed group-specific characteristic differences in the abundance of differentially regulated proteins. Quantification of a panel of five selected protein spots encompassing Interferon-induced GTP binding protein, HLA class II histocompatibility antigen, Annexin A6, FK506-binding protein 4 and GRP78 permitted discrimination of controls and JBS patients with mild phenotypes. Of note, the molecular chaperones GRP78 (BiP) and FK506BP were consistently altered in level in JBS patients and probably constitute UBR1 dependent substrates. This suggested JBS as an ER-stress related disease also indicating a possible way of therapeutic intervention. Comparative proteome analysis of UBR1 knockout and wild type animals after caerulein treatment revealed a significant accumulation of pancreatic proteases such as chymotrypsin B, anionic trypsin and pancreatic elastase in animals lacking UBR1. Furthermore, an up-regulation of ER-stress proteins and inflammation related proteins was observed. Phenotypic characterisation revealed in UBR1 knockout animals significantly increased lipase levels, a significantly increased histological score and significantly increased elastase activity 8h after the onset of pancreatitis. In isolated pancreatic acini of UBR1 knockout animals we found a significant increase in intracellular elastase activation upon supramaximal CCK stimulation, which was associated with a significant rise in the rate of necrosis explaining the more severe phenotype in the UBR1 knock-out animals. A TUNEL assay showed that there was more apoptosis in wild type compared to UBR1 knockout mice. Another set of experiments was designed to identify physiologically important substrates of UBR1. Inhibition of such substrates might then in turn allow reversion or prevention of the severe form of pancreatitis in UBR1 knockout mice. However, using the trypsin specific and reversible inhibitor S-124 it was shown that impaired trypsin degradation and thereby prolonged activation of this protease did not critically influence the phenotype. Calcium analysis after physiological stimulation revealed an increase of pathological Ca2+ signalling events, i.e. significant decrease of spike number and significant increase of spike duration. Of the candidates potentially influencing Ca2+ signalling RGS4 turned out to be of particular importance. Pre-incubation of pancreatic acini of UBR1 knockout animals with a specific RGS4 inhibitor (CCG-4986, 10 µM) normalized Ca2+ patterns, did not affect trypsin activity itself but prevented Ca2+-triggered premature trypsin activation and thus acinar disintegration. In summary, using lymphoblasts samples of JBS patients we were able to deduce a protein panel which could be developed as a possible diagnostic tool for confirmation of JBS syndrome. Furthermore, using UBR1 knockout mice in an experimental model we were able to elucidate the vital function of UBR1 and its direct substrate RGS4 in the defense against pathologic pancreatic damage thereby manifesting JBS as an inflammatory disorder due to an inadequate UBR1 mediated defense.
Massenspektrometrie hat sich zur Methode der Wahl für die globale relative und absolute Proteinquantifizierung entwickelt. Da das vorhandene Methodenspektrum in der Anzahl der zu analysierenden Proben limitiert ist und bei der Vermeidung von Vorfraktionierungstechniken keine globale Analyse erlaubt, war es das Ziel dieser Dissertation das Methodenspektrum anhand von anschaulichen Beispielen zur physiologischen Proteomanalyse Gram positiver Bakterien zu erweitern. Dazu erstreckt sich diese Arbeit von der Erweiterung der Anwendungsmöglichkeiten der Isotopen markierten relativen Quantifizierungsmethode, über die Entwicklung eines globalen markierungsfreien relativen Quantifizierungsansatzes bis zur globalen absoluten Quantifizierung und weiter im speziellen der Stöchiometrie-Aufklärung eines Proteinkomplexes. Die Kombination aus 14N/15N metabolischer Markierung mit der GeLC-MS Technik erlaubt eine robuste relative Quantifizierung auf globaler Ebene. Durch die Verwendung eines internen 15N-markierten Referenzextraktes wurde eine bisher nicht erreichte zeitliche Auflösung von zehn Zeitpunkten bei der Untersuchung eines Nährstoffwechsels zwischen den bevorzugten Kohlenstoffquellen, Glukose und Malat, des Gram positiven Modellorganismus Bacillus subtilis erreicht. Dieses Experiment zeigte klar, dass die Anpassung an Malat als zweite Kohlenstoffquelle sehr schnell passiert. Im Gegensatz dazu findet die Anpassung an Glukose als zusätzliche Kohlenstoffquelle mit einer zeitlichen Verschiebung von ca. 45 Min. statt. Diese Ergebnisse legen den Schluss nahe, dass die Anpassung an Malat hauptsächlich auf post-transkriptioneller Ebene geschieht und die Anpassung an Glukose auf transkriptioneller Ebene stattfindet. Die geringe Reproduzierbarkeit von Vorfraktionierungstechniken beschränkt ihre Anwendung während einer markierungsfreien Quantifizierung. Die eingeschränkte Kombinationsmöglichkeit mit Vorfraktionierungstechniken führt zu einer geringeren Anzahl an identifizierten und quantifizierten Proteinen, was durch den Einsatz von Ausschlusslisten mit optimierten Messparametern in wiederholten Messungen mit einer eindimensionalen Chromatographie ausgeglichen wurde. Im Vergleich zu einer einfachen Wiederholung der Messung konnte die Anzahl an identifizierten Peptiden um 32 % gesteigert werden. Der Ausschlusslistenansatz konnte anschließend erfolgreich für eine markierungsfreie globale Proteinquantifizierung der Stickstoffmonoxid (NO) Stressantwort des humanpathogenen Stapylococcus aureus eingesetzt werden. Die Ergebnisse wurden mittels paralleler Quantifizierung mit 14N/15N metabolischen Markierung verifiziert. Mit dem Ansatz wurden fast 50 % des gesamten Proteoms identifiziert und 70 % davon konnten mit einem zu dem Markierungsexperiment vergleichbaren Ergebnis quantifiziert werden. Die Proteomsignatur der NO-Stressantwort zeigte eine hohe Ähnlichkeit zu der von Antibiotika, die wie NO zu DNA-Strangbrüchen führen. Auch bei der absoluten Proteinquantifizierung kann nicht ohne Weiteres eine Vorfraktionierung eingesetzt werden. Durch die Verwendung einer „multiplexed LC-MS“ (LC-MSE) Methode wurde fast die Hälfte aller zytosolischen Proteine von B. subtilis mit einer hohen durchschnittlichen Sequenzabdeckung von 40 % identifiziert. Die Hi3-Methode ermögliche zusätzlich die absolute Quantifizierung fast aller identifizierten Proteine, die über fast vier Größenordnungen nachgewiesen werden konnten. Die Zuverlässigkeit des Ansatzes wurde für sechs Proteine mit der gut etablierten AQUA-Technik bestätigt. Mit der Hi3-Methode wurden zum einen absolute Proteomsignaturen für unterschiedliche Nährstoffsituationen erstellt, was auch Einblicke in die Regulation der Expression von Aminosäure-Biosynthese und –abbau-Enzyme ermöglichte. Zum anderen konnte gezeigt werden, dass die intrazelluläre Konzentration von ribosomalen und weiteren Wachstumsraten-abhängig benötigten Proteinen sich bei niedrigen Wachstumsraten nicht unterscheidet und erst ab einer Wachstumsrate von 0,8 Std.-1 linear ansteigt. Die vergleichsweise hohe Standardabweichung der Hi3-Methode (~30 %) erschwert ihre Anwendung bei der Bestimmung von nicht gradzahligen Protein-Komplex-Stöchiometrien. Deswegen wurde zur Analyse des RNA-Polymerase-Komplexes von B. subtilis der AQUA-Ansatz gewählt, der sich durch eine sehr geringe Standardabweichung auszeichnet (< 10 %). Dazu wurde ein Protokoll entwickelt, welches auf einer mTRAQ-Markierung der Referenzpeptide und des verdauten Komplexes beruhte. Es war so möglich die bekannte Stöchiometrie des Kernkomplexes RpoA:RpoB:RpoC 2:1:1 zu bestätigen und zusätzlich die zwei ω-Unterheiten und die σ-Faktoren σA und σB absolut zu bestimmen. Die Menge an σB im Komplex nahm nach Glukose-Hunger und Ethanol-Stress auf bis zu 5 % zu und es konnte gezeigt werden, dass sich die Menge einer ω-Unterheit (YloH) sich im gleichen Maße im Komplex ändert, wie die Menge an σA.
Rich knowledge about global nutrient cycles and functional interactions can be gained from the perspective of complex microbial proteomes. In this thesis, the application of environmental proteomics allowed for a direct in situ analysis of habitat-specific proteomes expressed by respective microbial communities from two different marine ecosystems. In the first part of this thesis, unculturable symbiont populations from tubeworms that colonize hydrothermal vents of the Pacific deep sea became accessible by use of community proteomics. This branch of environmental proteomics is generally employed to ascertain simple microbial assemblages derived from in situ samples. The proteome study was aimed at analyzing adaptations of seemingly monospecific symbionts to different hosts, the tubeworms Tevnia jerichonana und Riftia pachyptila. A comparison of the newly sequenced genomes of symbiont populations from both hosts confirmed that both symbioses involve the same bacterial species. Also the proteome analysis by 2D-PAGE showed a high physiological homogeneity for symbionts from both worm species, although the hosts are exposed to different geochemical conditions. Thus, the hosts provide their symbionts with a relatively stable internal environment by attenuation of external influences. Only minor variations in the symbionts proteomes reflected the differential environmental conditions outside the worms. Hence, the symbionts were able to fine-tune major metabolic pathways and oxidative stress in response to only minor chemical changes within their hosts. Moreover, new components of important physiological processes of the bacterial symbionts, like the sulfide oxidation and carbon fixation, were identified by in-depth proteomics of the Riftia symbiosis model system. The in situ protein samples showed as well that, in contrast to an earlier hypothesis, nitrate is used as an alternative electron acceptor. In the second part of this thesis, another branch of environmental proteomics called metaproteomics was applied to investigate the response of a bacterioplankton community to a spring phytoplankton bloom in the North Sea. Recurrent plankton blooms are a common phenomen of coastal areas, which however has only been investigated with limited resolution in biodiversity. Based on large-scale proteomic data sets it was found that specialized populations of Bacteroidetes, Gammaproteobacteria and Alphaproteobacteria exhibited differential protein expression patterns. These involved oligomer transporters, glycoside hydrolases and phosphate acquisition proteins. A successive utilization of algal organic matter by microbes indicated a series of ecological niches occupied by the heterotrophic picoplankton. Key proteins, identified by metaproteomics, were further investigated by studying a model bacterium to define their specificities regarding the utilization of algal glycans. By isotope labeling of proteins, quantitative proteomics of the North Sea isolate Gramella forsetii KT0803, a Bacteroidetes representative could be conducted. The adaptation to the algal polysaccharides alginate and laminarin in comparison with glucose was analyzed. G. forsetii proved to be a specialist for the chosen algal polymers, in particular for glucans like laminarin. Primarily comprehensive clusters, the so-called polysaccharide utilization loci (PULs) were activated. The results of this model study complemented the basic concepts obtained by the metaproteomic approach about carbon cycling in coastal systems. The accessibility of numerous unculturable marine microbes by environmental proteomics allows to improve our understanding of interactions that drive symbioses or complex communities. Adaptations to environmental parameters, such as the abundance of substrates, can be analyzed and associated with respective populations. Thus statements can be made for functional groups of microorganisms, their ability for the creation of niches and their flexibility to respond to varying environmental impacts. The increasing number of marine model bacteria enables targeted analysis of specificities and adaptations and hence to support the environmental proteomics approach.
Die chronische Herzinsuffizienz (HI) bezeichnet das Unvermögen des Herzens, die vom Körper benötigte Blutmenge bedarfsgerecht zu befördern und stellt in der Allgemeinbevölkerung das Endstadium vieler Herzerkrankungen dar. Trotz großer Fortschritte in der medikamentösen Therapie ist die Prognose der HI auch heute noch schlecht. Der progrediente Verlauf erstreckt sich von einer kompensierten Herzhypertrophie mit aufrechterhaltener Pumpfunktion bis hin zu einer massiven Ventrikeldilatation mit stark eingeschränkter Herzfunktion und weist dementsprechend eine schlechte Prognose auf. Die zellulären Veränderungen auf Protein- und Genexpressionsebene während der Progression einer HI sind sehr komplex und trotz ausgiebiger wissenschaftlicher Arbeiten nicht ausreichend geklärt. Dabei ist es von entscheidender Bedeutung, in welcher Phase der Erkrankung spezifische Änderungen in der Genregulation entstehen und inwiefern sich diese auf den Phänotyp auswirken. Auf Grund dessen beschäftigt sich die vorliegende Arbeit mit den zeitabhängigen Veränderungen auf mRNA-und Proteinebene während der Progression der HI. Um alle Stadien beginnend von einer subklinischen Organschädigung bis hin zur Ausbildung einer HI experimentell untersuchen zu können, wurde zunächst ein Mausmodell etabliert, welches durch eine chronische Nachlasterhöhung mittels Einengung des Aortenlumens eine Myokardschädigung durch eine arterielle Hypertonie simuliert (transverse aortic constriction, TAC). Die Herzfunktion der Mäuse wurde an den postoperativen Tagen 4, 14, 21, 28, 42, und 56 durch Messungen im Kleintier-MRT (Magnetresonanztomografie) evaluiert. Dabei konnte gezeigt werden, dass sich die linksventrikuläre Ejektionsfraktion (LVEF) TAC-operierter Mäuse vom postoperativen Tag 4 zu 14 verschlechtert, bis Tag 42 auf einem konstanten Niveau hält und bis Tag 56 nochmals stark absinkt. Im Gegensatz dazu zeigten Sham-operierte Mäuse über den gesamten Zeitraum eine stabile LVEF. Ein vergleichbarer stufenartiger Verlauf konnte bei den Parametern der linksventrikulären Masse und den endsystolischen bzw. enddiastolischen Volumina beobachtet werden. Zusätzlich konnte durch histologische Untersuchungen zu den verschiedenen postoperativen Zeitpunkten eine verstärkte Fibrosierung des Herzgewebes nach der TAC-OP aufgezeigt werden. Für die longitudinalen Transkriptom- und Proteomuntersuchungen wurden die Herzen (jeweils linke und rechte Ventrikel) nach den MRT-Messungen entnommen, gruppen- und zeitpunktspezifisch gepoolt und einer Microarray- bzw. massenspektrometrischen Analyse unterzogen. Auf Transkriptomebene zeigten sich vor allem an den Tagen 4 und 56 starke TAC-induzierte Veränderungen im Expressionsmuster, wohingegen der Zeitraum zwischen 14 und 42 Tagen weniger differenziell exprimierte Gene aufwies. Der Verlauf der Erkrankung konnte anhand bereits bekannter Hypertrophie- und HI-marker sehr gut charakterisiert werden. So zeigten Nppa (ANP) und Nppb (BNP) im linken Ventrikel bereits kurz nach Aortenstenose stark erhöhte Expressionslevel, die über die gesamte Versuchsdauer erhalten blieben. Weiterhin wurde die Expression von Genen reguliert, die an kardialen Remodelingprozessen maßgeblich beteiligt sind, wie beispielsweise Acta1 (a-Aktin), Myh7 (b-Myosin Heavy Chain) und Postn (Periostin). Im Vergleich beider Ventrikel zeigte der rechte Ventrikel bezüglich der Anzahl der regulierten Gene als auch bei der Expression HI-assoziierter Gene eine verzögerte und weniger stark ausgeprägte Reaktion. In den linken Ventrikeln wurden vor allem die Gene reguliert, deren Genprodukte der extrazelluären Matrix angehören. Eine Validierung der Microarray-Ergebnisse mittels realtime-PCR konnte die Richtigkeit der Analysemethode sehr präzise bestätigen. Da diese anhand ausgewählter Gene auf Einzeltierebene durchgeführt wurde, konnte zusätzlich auf Korrelation zwischen mRNA-Expression und den kardialen Funktionsparametern getestet werden. Wie erwartet spiegelten die Epressionslevel der HI-assozierten Markergene Nppa (ANP), Nppb (BNP) und Myh7 (b-Myosin Heavy Chain) die progressive Verschlechterung der Herzfunktion wider. Zusätzlich konnten durch die Validierung und Korrelationsanalysen weitere interessante Kandidatengene, wie beispielsweise Sfrp2 (Secreted frizzled-related protein 2) und Wisp2 (WNT1-inducible signaling pathway protein 2) für weiterführende Studien identifiziert werden. Auch auf Proteomebene konnten vergleichbare Ergebnisse erzielt werden. Auch hier zeigte der linke Ventrikel eine deutlich ausgeprägtere Reaktion auf die Drucküberlastung, der rechte Ventrikel antwortete deutlich schwächer und verzögert. Änderungen im Proteinmuster nach TAC waren in den linken Ventrikeln vor allem an den Tagen 14, 21 und 28 stark ausgeprägt. Ingenuity Pathway Analysen der veränderten Proteine weisen auf Veränderungen im Kalzium-, Rho A- und PKA-Signaling vor allem zu den frühen Zeitpunkten hin, wohingegen zu späteren Zeitpunkten hauptsächlich metabolische Prozesse betroffen waren.
Staphylococcus aureus is a commensal that colonizes the skin and mucosa of 20-30% of the human population without leading to symptoms of diseases. However, it is also the most important cause of nosocomial infections. Those range from minor skin infections to life-threatening diseases such as pneumonia, endocarditis or septicaemia. Development of strains with resistance against many antibiotics complicates the situation further. The variety of strains with their various properties is one reason why no successful vaccine has been introduced to the market, yet. Therefore, efficient strategies for prevention and therapy of these dangerous infections are urgently needed. To accomplish these goals, the understanding of molecular interactions between host and pathogen is indispensable. Within this dissertation, several internalization experiments were performed aiming to investigate the interaction of S. aureus HG001 and human cell lines upon infection on the protein level. In order to obtain sufficient amounts of proteins for comprehensive physiological interpretations, it is necessary to enrich bacteria, secreted bacterial proteins or infected host cells upon internalization. In the framework of this thesis, bacteria which continuously produce green fluorescent protein (GFP) were employed. With that it was possible to sort bacteria from lysed host cells by flow cytometry or to separate host cells carrying bacteria after contact from those which did not. Subsequently, the proteins were proteolytically digested and peptides were analyzed by mass spectrometry in a gel-free proteomics approach. To allow such analyses also for staphylococci which do not produce GFP, such as clinical isolates, an additional protocol was developed. Prior to the infection, bacteria were labeled with fluorescent or para-magnetic nanoparticles. Afterwards bacteria could be separated from host cell debris by fluorescence-based cell sorting or with the help of a strong magnet. In order to cover also important secreted virulence factors of S. aureus HG001, phagosomes and engulfed bacteria and secreted proteins were isolated from infected host cells. Further steps of protocol optimization included improved bacterial cell counting by fluorescence-based flow cytometry, enhanced data analysis by combination of different search algorithms, and comprehensive functional annotation of proteins of the applied strain by sequence comparison with other strains and organisms. First, the proteome adaptation of internalized S. aureus HG001 and the infected A549 host cells was investigated during the first hours of infection. It became clear, that the bacteria replicate inside the host during the first 6.5 h. After internalization the levels of bacterial enzymes involved in protein biosynthesis decreased. Furthermore, bacteria adapted their proteome to the harsh intracellular conditions such as oxygen limitation, cell wall stress, host defense in terms of oxidative stress, and nutrient limitation. After contact to S. aureus HG001, A549 cells produced increased amounts of cytokines (e.g. IL-8, IFN-γ) in comparison to non-treated A549 cells. In addition, activation of the immunoproteasome and hints of early apoptosis activity were observed. Afterwards, the response of S. aureus HG001 to internalization by A549, S9 or HEK 293 cells was compared on the proteome level. It was obvious, that the adaptation to stress and the reduced protein synthesis are conserved mechanisms. Host dependent differences were detected especially in the energy metabolism and the synthesis of some amino acids. Additionally, bacteria showed different intracellular replication patterns depending on the host cell line. A higher percentage of extracellular bacterial proteins was found in isolated phagosomes compared to the sorted samples. Selected low abundant virulence factors could be quantified at two points in time after infection with the help of the sensitive single reaction monitoring (SRM) method. Further, a heterogeneous mixture of several phagosomal maturation steps was present during the first 6.5 h after infection. Finally, the gel-free proteome analyses could be applied to investigate Bordetella pertussis, the cause of whooping cough, during iron limitation and after internalization, and the results were compared to the S. aureus HG001 data.
Ziel der Dissertation war die Untersuchung der physiologischen Adaptation von Staphylococcus aureus an Vancomycin und Linezolid mit Hilfe der Proteom-Analytik und die Entwicklung neuer Methoden für Proteom-Untersuchungen. Für die Untersuchung der Vancomycinstress-Antwort im ersten Teil der Doktorarbeit wurden alle vier Subproteome mit insgesamt sechs verschiedenen Methoden untersucht. Es konnte mehr als die Hälfte des theoretischen Proteoms quantifiziert werden, die Arbeit ist damit eine der umfassendsten Proteom-Studien, die bisher in S. aureus durchgeführt wurden. Es wurden verschiedene Enzyme der Biosynthese von Aminosäuren, die im Peptidoglykan-Vorläufer-Pentapeptid vorkommen, nach Vancomycin-Stress in signifikant erhöhter Menge nachgewiesen. Das ist ein Hinweis auf eine erhöhte Peptidoglykan-Synthese, wie sie auch in S. aureus Stämmen mit verminderter Vancomycin-Sensitivität beobachtet werden kann. Die Abundanz SaeRS-kontrollierter Virulenzfaktoren war nach Vancomycin-Stress vermindert. In der Vancomycin-Studie wurden extrazelluläre Proteine mit einer Trichloressigsäure (TCE)-Fällung gefällt, diese Methode ist in der Proteom-Analytik weit verbreitet. Die TCE-Fällung hat verschiedene Nachteile. Nach der Fällung muss das entstandene Pellet mehrfach gewaschen werden, hierbei kommt es zu Verlusten und die Reproduzierbarkeit sinkt. Aufgrund dieser Nachteile wurde im zweiten Teil der Dissertation ein neues Protokoll zur Anreicherung verdünnter Proteine entwickelt. Grundlage war das kommerziell erhältliche Festphasenextraktions-System StrataClean, das ursprünglich zur Entfernung von Proteinen aus PCR-Ansätzen entwickelt wurde. Im Rahmen der Doktorarbeit wurde die StrataClean-Extraktion für die gel-freie Proteom-Analytik optimiert. Der wichtigste Schritt war eine Präinkubation der StrataClean-Partikel in Salzsäure, um Kontaminationen an den Partikeln quantitativ abzubauen. Mit dem optimierten Protokoll konnten Proteine auch aus sehr stark verdünnten Lösungen (20 µg Protein in 200 ml Flüssigkeit) mit hoher Effizienz reproduzierbar angereichert werden. Diese hoch-effiziente Anreicherung ist mit keinem anderen etablierten Protokoll möglich. Zudem konnte gezeigt werden, dass die StrataClean Fällung Proteine unabhängig von ihren biophysikalischen Eigenschaften anreichert. Daher ist die StrataClean-Aufreinigung auch für absolute Quantifizierungsansätze interessant. Als weitere Anwendung können StrataClean-gebundene Proteine für mehr als 10 Tage bei Raumtemperatur gelagert werden. Das ermöglicht den Versand von Proteinproben auf dem normalen Postweg ohne aufwendige Kühlsysteme. Im dritten Teil der Doktorarbeit wurde die Linezolid-Adaptation von S. aureus USA300 analysiert. In Wachstumsversuchen konnte gezeigt werden, dass nach Linezolid-Zugabe zu exponentiell wachsenden Zellen bei OD 0.5 die Wachstumsrate sofort abnahm. Bei OD 1.6 – 2 trat ein temporärer Wachstumsarrest auf, dessen Dauer von der zugegebenen Linezolid-Konzentration abhing. Nach diesem Wachstumsarrest, der bis zu 15 Stunden anhielt, fingen die Zellen wieder an sich zu teilen. Es konnte gezeigt werden, dass die Linezolid-Konzentration im Medium während des kompletten Versuches konstant blieb. Die Hauptanpassung an Linezolid war eine verstärkte Expression der Gene ribosomaler Proteine und eine daraus folgende erhöhte Akkumulation der ribosomalen Proteine. Zudem konnte eine generelle Abnahme der Menge integraler Membranproteine und sekretierter Proteine festgestellt werden, auch wenn die Expression der codierenden Gene zunahm. Mittels elektronenmikroskopischer Analysen konnte gezeigt werden, dass die Zellen nach Linezolid-Zugabe deutlich größer wurden. Als weitere morphologische Auswirkung von Linezolid-Stress war die Dicke der Zellwand um den Faktor vier erhöht und es wurden Defekte in der Zellteilung beobachtet. Insbesondere nach Wiederaufnahme des Wachstums gab es zahlreiche zelluläre Strukturen, die mehrere, zum Teil falsch positionierte, Septen hatten. Mit Fluoreszenz-Mikroskopie wurde bewiesen, dass sich das Chromosom, das im normalen Wachstum das Cytosol ausfüllt, nach Linezolid-Zugabe komprimierte und den Kontakt zur Membran verlor. Eine Verbindung zwischen Chromosom und Membran wird durch Transertions-Komplexe gebildet. Transertion bezeichnet die simultane Transkription, Translation und Translokation integraler Membranproteine, dabei werden Komplexe aus Chromosom, mRNA, Ribosom, dem entstehendem Protein und den membranständigen SEC-Proteintransportern gebildet. Aus der Kombination der Ergebnisse wurde geschlossen, dass durch die Linezolid ausgelöste Translations-Hemmung die Transertionskomplexe aufgelöst werden und dadurch die Protein-Translokation vermindert wird. Auch die Defekte in der Zellteilung können so erklärt werden, da so das Chromosom eine Struktur-gebende Funktion für die Zellteilung verliert. Bisher war nicht vollständig bekannt, wie die strukturelle Ordnung in der Zellteilung von Staphylokokken entsteht.
Staphylococcus aureus can be a harmless colonizer of the human body, which colonizes about 20-30% of the population. If S. aureus overcomes the outer physical barrier of the body, comprised of the skin and mucous surfaces, it can also cause severe diseases such as endocarditis, pneumonia, or sepsis. S. aureus possesses a variety of secreted and surface bound virulence factors to mediate attachment and invasion into the host, to disseminate an infection and to modulate and evade the immune system. But not only the huge amount of virulence factors turn S. aureus into a dangerous human pathogen, also its resistances to a broad spectrum of commonly used antibiotics make infections hard to treat. During the last years it became apparent that S. aureus can be internalized by as well as replicate and persist in professional and non-professional phagocytic cells. It is suggested that the intracellular compartment protects S. aureus from antibiotic treatment and the immune system. To accomplish the adaptation to the intracellular compartment, S. aureus needs to regulate its gene expression by regulatory systems. One of these regulators is the alternative sigma factor SigB, which directly and indirectly regulates the expression of about 200 genes in vitro. However, the stimuli leading to the activation of SigB in S. aureus are barely known and also its role during an infection varies, depending on the S. aureus strain and infection model used. Therefore, the importance of SigB during the early adaption of S. aureus to the intracellular environment should be elucidated using a cell culture infection model. First, the existing cell culture infection workflow had to be modified to improve the data analysis and to increase the yield of identified proteins to comparatively monitor the adaption reaction of S. aureus HG001 and its isogenic ΔsigB mutant to the intracellular milieu of S9 human bronchial epithelial cells. The proteome analysis in conjunction with RT-qPCR analysis of the wild type and the ΔsigB mutant revealed a fast and transient activation of SigB directly after internalization. Quantitative analysis of the intracellular bacterial titer demonstrated a requirement of SigB for intracellular replication. Differences in the proteome composition of the ΔsigB mutant in comparison to the wild type after internalization reflected the different growth rates, resistance to antibiotics and toxic compounds, adaptation to oxidative stress, and protein quality control mechanisms. The accessory gene regulator (Agr) is like SigB also a global regulator of gene expression in S. aureus. To elucidate possible benefits in the intracellular survival of the co-occurrence of S. aureus wild type and Δagr mutant cells, like it can be found in sites of an infection, a co-infection assay was established. With the co-infection assay the simultaneous and competitive intracellular survival in comparison to the individual intracellular survival was followed for three days post-infection (p.i.). The single and the co-infection revealed that the wild type was able to replicate more efficiently during the first hours p.i. than the Δagr mutant, but the mutant was able to survive more efficiently. The extracellular proteome of S. aureus represents the key compartment for virulence factors. Virulence factors are secreted or bound to the surface of the S. aureus cell. With the infection workflow applied in this study, secreted proteins are lost during the enrichment of the intracellular bacteria for proteome analysis. Therefore, no information about the levels or the regulation of virulence factor expression can be acquired in the cell culture infection model using cell sorting approaches. Hence, the extracellular proteome of S. aureus was analyzed in vitro from shake flask experiments. To get a comprehensive overview of the regulatory impact of different global regulators onto the secretome, S. aureus LS1 mutants lacking the global regulators Agr, SarA and SigB were compared to the respective wild type. Additionally the protein level of the secretome of the well characterized and frequently used S. aureus strains 6850, CowanI, HG001, LS1, SH1000, and USA300 was comparatively analyzed. This project was performed in collaboration with the group of Prof. Löffler from the Institute of Medical Microbiology in Jena. The data of the extracellular proteome generated in this thesis were combined with phenotypic and toxicity data to explain strain differences in invasiveness, cytotoxicity, phagosomal escape, and intracellular persistence in infection experiments.
Members of the species Bacillus pumilus get more and more in focus of the biotechnological industry as potential new production strains. Based on secretome analysis, Bacillus pumilus strain Jo2, possessing high secretion capability, was chosen for an omics based investigation. The physiology of Bacillus pumilus cells growing either in minimal or complex medium was analyzed by a combination of proteomic and metabolomic methods. Master gels of the cytosolic and the secreted proteome covering major parts of the main metabolic pathways were created by means of 2D gel electrophoresis. Quantification of 2D gels allowed displaying the most abundant proteins in these sub-proteomes. Application of the GeLC-MS/MS technique tripled the number of identified proteins and enabled detection of many intrinsic membrane proteins. In total, 1542 proteins were identified in growing B. pumilus cells, among them 1182 cytosolic proteins, 297 membrane and lipoproteins and 63 secreted proteins. This accounts for about 43 % of the 3616 proteins encoded in the B. pumilus Jo2 genome sequence. By using GC-MS, IP-LC/MS and H-NMR methods numerous metabolites were analyzed and assigned to the reconstructed metabolic pathways. Our data indicate that applying a combination of proteomic and metabolomic techniques a comprehensive view of the physiology of growing B. pumilus cells can be gained. In addition, selected production-relevant genome features such as the restriction modification system, NRPS clusters and the secretory system of B. pumilus Jo2 are discussed. In their natural habitat, the soil, B. pumilus cells are often exposed to growth limiting conditions due to the lack of sufficient amounts of nutrients. Such limitations can also occur during fermentation conditions and will negatively influence the efficiency of the process. Glucose is the main carbon and energy source of B. pumilus. Thus, a deficiency of glucose has an enormous impact on cell growth. A 1D LC-MS/MS approach was performed to quantify the proteins using an N14/N15 labeling and to analyze the changes in the protein equipment when B. pumilus cells stop their exponential growth and become stationary due to limitation of glucose. 1033 proteins in the cytosolic fraction of B. pumilus cells were quantified and 272 of them appeared to be upregulated when the cells experience glucose starvation. 2D-PAGE was used to analyze the exoproteome of those cells. Glucose starving B. pumilus cells seemed to focus on usage of proteins and peptides as alternative carbon and energy sources instead of other carbohydrates. Especially the exoproteome of glucose starving cells is dominated by proteases and peptidases. Furthermore, cells used fatty acids as carbon source indicated by upregulation of enzymes involved in β-oxidation and the methylcitrate pathway. Bacillus pumilus is characterized by a higher oxidative stress resistance than other comparable industrially relevant Bacilli such as B. subtilis or B. licheniformis. In this study the response of B. pumilus to oxidative stress was investigated during a treatment with high concentrations of hydrogen peroxide at the proteome, transcriptome and metabolome level. Genes/proteins belonging to regulons, which are known to have important functions in the oxidative stress response of other organisms, were found to be upregulated, such as the Fur, Spx, SOS or CtsR regulon. Strikingly, parts of the fundamental PerR regulon responding to peroxide stress in B. subtilis are not encoded in the B. pumilus genome. Thus, B. pumilus misses the catalase KatA, the DNA-protection protein MrgA or the alkyl hydroperoxide reductase AhpCF. Data of this study suggests that the catalase KatX2 takes over the function of the missing KatA in the oxidative stress response of B. pumilus. The genome-wide expression analysis revealed an induction of bacillithiol (Cys-GlcN-malate, BSH) relevant genes. An analysis of the intracellular metabolites detected high intracellular levels of this protective metabolite, which indicates the importance of bacillithiol in the peroxide stress resistance of B. pumilus. Using the physiological knowledge gained during our studies, we analyzed samples taken during an industrial fermentation process. Five samples were taken during the processes using a protease overexpressing B. pumilus strain and a non-overexpressing B. pumilus reference strain. 2D-PAGE was employed to analyze the samples. 448 proteins could be identified in the samples from the protease overexpressing stain as well as 453 proteins in the reference strain. The proteins were quantified relatively comparing the different growth phases of each strain as well as comparing the strains to each other. The physiological knowledge gained from the shake flask studies enabled us to interpret the findings. Both strains showed an induction of proteins involved in acquisition of alternative carbon sources and of proteins involved in degradation and usage of fatty acids, e.g. the methylcitrate pathway, when they stop exponential growth. This is comparable to the results gained from the analysis of B. pumilus cells under glucose limitation, indicating similar conditions during the processes. Especially in the late phases of the fermentation processes the cells were obviously exposed to severe stress conditions. Our results demonstrated that overexpressing cells showed a significantly stronger oxidative stress response at the end of the fermentation process compared to non-overexpressing cells, which indicated that not only the high cell densities but also the overproduction of the target protein might be responsible for these conditions.
Heart Failure is currently the most common cardiac disorder and a major public health concern worldwide. The adult mammalian heart harbors a subpopulation of cardiac progenitor cells (CPC) that are capable of improving cardiac function. The scope of this study was to delineate the molecular phenotype of a subpopulation of CPCs characterized by the expression of the stem cells antigen-1 surface marker (Sca-1+) and to further identify molecular alterations occurring under heart failure conditions. In order to understand the underlying cellular mechanisms an integrated approach of proteomics and transcriptomics-based techniques were employed. The first step towards achieving this goal was to unravel the native Sca-1+ cell characteristics of freshly isolated progenitor cells derived from healthy adult murine hearts. The proteome map of Sca-1 cells was established using a gel-based mass-spectrometry (gel LC-MS/MS) approach. For better interpretation, a comparison with the protein profiles of cardiomyocytes and Sca-1- cells obtained under similar experimental conditions was performed. All three cell-types were morphologically different in size and structure, which was also evident from their protein expression profiles. We observed that Sca-1+ cells lack endothelial-like and cardiac contractile phenotypes, unlike Sca-1- cells and cardiomyocytes, respectively. Functional assessment of both protein and gene expression profiles revealed a possible role of Sca-1+ cells in cell adhesion, migration, and proliferation. CPC remain in a dormant state under physiological condition unless challenged by myocardial injury. Previous studies revealed that resident Sca-1+ cells home to the injured myocardium but not to the healthy heart and further differentiate into functional cardiomyocytes. We investigated the molecular background of this behavior of adult Sca-1+ cells under heart failure condition which might provide a better insight into their cardiogenic potential in a pathological milieu. The double transgenic α-myosin heavy chain (MHC)-cyclin T1/Gαq overexpressing mouse was chosen as a model for heart failure. Using the comparative gene expression profiling we could detect the differential regulation of 197 genes with at least a 2-fold difference. Among these BDNF mRNA levels were 5-fold higher in the Sca-1+ cells derived from transgenic mice (Cyc+) in comparison to that of wild-type controls (Wt+). This difference was also observed at protein level. The substantially higher expression of BDNF during heart failure prompted us to investigate its regulatory effect on Sca1+ cells. In this current study we were able to show that small amounts of exogenous BDNF stimulated the migratory potential of Cyc+ cells. This effect was not seen in treated Wt+ cells. Furthermore, pulsed SILAC was employed to monitor BDNF mediated changes following treatment. After BDNF treatment, 58 proteins were differentially regulated of which proteins related to cell proliferation were reduced in level in Cyc+ cells while they displayed increased levels in Wt+ cells. Findings from bromodeoxyuridine (BrdU) assays and immunoblotting indicated that BDNF might initiate a differentiation program by repressing cell proliferation in Cyc+ cells. Taken together, it could be shown that the BDNF effect on protein synthesis of Cyc+ and Wt+ cells varied considerably, suggesting an improvement of the cardiogenic potential of Sca-1+ cells under pathological conditions. Aldosterone levels are known to be elevated during heart failure. In this part of study it was hypothesized that endocrine factors associated with heart failure might influence the migration of CPC, thereby possibly restoring the cardiac function of diseased hearts. It could be shown that high concentrations of aldosterone, similar to those found in the plasma of heart failure patients, induced the migration of Sca-1+ cells by up to 60% when compared to control, while physiological levels had no significant influence. In addition, it could be demonstrated that the aldosterone stimulus led to the activation of the mineralocorticoid receptor (MR) expressed on Sca1+ cells, which in turn facilitated migration. This was supported by application of MR antagonist eplerenone, which significantly reduced the aldosterone-induced increase in cell migration while a glucocorticoid antagonist exhibited no inhibitory effect. Hence, the results support the potential role of aldosterone in the mobilization of CPC. It is currently believed that the beneficial effects of cell-based therapies on cardiac repair are imparted to a large degree via paracrine mechanisms. We therefore focused on understanding the influence of pathophysiological levels of aldosterone on the extracellular environment of Sca-1+ cells. MS-based secretome profiling of cells treated for 24h with aldosterone treatment revealed higher levels of proteins associated with extracellular matrix remodeling and IGF signaling. Additionally, galectin-1 and gelsolin were significantly increased in level under pathological conditions indicating a possible paracrine tissue repair of Sca-1+ cells. To conclude, the global proteome and transcriptome profiles generated here revealed the molecular phenotype of Sca-1+ cells which may be used for future reference. The comparative microarray study provided deeper insight into the endogenous changes in mRNA expression during heart failure and delineated the cardiogenic characteristics of Sca-1+ cells. Moreover, the data presented here shed new light on the potential role of BDNF in regulating the mobilization and proliferation of CPCs. Our study on the influence of aldosterone on the migration and the extracellular proteome of CPCs provided new insights on the beneficial effects of this mineralocorticoid on cardiac cells.