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Genome sequence analysis A combination of genome analysis application has been established here during this project. This offers an efficient platform to interactively compare similar genome regions and reveal loci differences. The genes and operons can be rapidly analyzed and local collinear blocks (LCBs) categorized according to their function. The features of interests are parsed, recognized, and clustered into reports. Phylogenetic relationships can be readily examined such as the evolution of critical factors or a certain highly-conserved region. The resulting platform-independent software packages (GENOVA and inGeno), have been proven to be efficient and easy to handle in a number of projects. The capabilities of the software allowed the investigation of virulence factors, e.g., rsbU, strains’ biological design, and in particular pathogenicity feature storage and management. We have successfully investigated the genomes of Staphylococcus aureus strains (COL, N315, 8325, RN1HG, Newman), Listeria spp. (welshimeri, innocua and monocytogenes), E.coli strains (O157:H7 and MG1655) and Vaccinia strains (WR, Copenhagen, Lister, LIVP, GLV-1h68 and parental strains). Metabolic network analysis Our YANAsquare package offers a workbench to rapidly establish the metabolic network of such as Staphylococcous aureus bacteria in genome-scale size as well as metabolic networks of interest such as the murine phagosome lipid signalling network. YANAsquare recruits reactions from online databases using an integrated KEGG browser. This reduces the efforts in building large metabolic networks. The involved calculation routines (METATOOL-derived wrapper or native Java implementation) readily obtain all possible flux modes (EM/EP) for metabolite fluxes within the network. Advanced layout algorithms visualize the topological structure of the network. In addition, the generated structure can be dynamically modified in the graphic interface. The generated network as well as the manipulated layout can be validated and stored (XML file: scheme of SBML level-2). This format can be further parsed and analyzed by other systems biology software, such as CellDesigner. Moreover, the integrated robustness-evaluation routine is able to examine the synthesis rates affected by each single mutation throughout the whole network. We have successfully applied the method to simulate single and multiple gene knockouts, and the affected fluxes are comprehensively revealed. Recently we applied the method to proteomic data and extra-cellular metabolite data of Staphylococci, the physiological changes regarding the flux distribution are studied. Calculations at different time points, including different conditions such as hypoxia or stress, show a good fit to experimental data. Moreover, using the proteomic data (enzyme amounts) calculated from 2D-Gel-EP experiments our study provides a way to compare the fluxome and the enzyme expression. Oncolytic vaccinia virus (VACV) We investigated the genetic differences between the de novo sequence of the recombinant oncolytic GLV-1h68 and other related VACVs, including function predictions for all found genome differences. Our phylogenetic analysis indicates that GLV-1h68 is closest to Lister strains but has lost several ORFs present in its parental LIVP strain, including genes encoding CrmE and a viral Golgi anti-apoptotic protein, v-GAAP. Functions of viral genes were either strain-specific, tissue-specific or host-specific comparing viral genes in the Lister, WR and COP strains. This helps to rationally design more optimized oncolytic virus strains to benefit cancer therapy in human patients. Identified differences from the comparison in open reading frames (ORFs) include genes for host-range selection, virulence and immune modulation proteins, e.g. ankyrin-like proteins, serine proteinase inhibitor SPI-2/CrmA, tumor necrosis factor (TNF) receptor homolog CrmC, semaphorin-like and interleukin-1 receptor homolog proteins. The contribution of foreign gene expression cassettes in the therapeutic and oncolytic virus GLV-1h68 was studied, including the F14.5L, J2R and A56R loci. The contribution of F14.5L inactivation to the reduced virulence is demonstrated by comparing the virulence data of GLV-1h68 with its F14.5L-null and revertant viruses. The comparison suggests that insertion of a foreign gene expression cassette in a nonessential locus in the viral genome is a practical way to attenuate VACVs, especially if the nonessential locus itself contains a virulence gene. This reduces the virulence of the virus without compromising too much the replication competency of the virus, the key to its oncolytic activity. The reduced pathogenicity of GLV-1h68 was confirmed by our experimental collaboration partners in male mice bearing C6 rat glioma and in immunocompetent mice bearing B16-F10 murine melanoma. In conclusion, bioinformatics and experimental data show that GLV-1h68 is a promising engineered VACV variant for anticancer therapy with tumor-specific replication, reduced pathogenicity and benign tissue tropism.
Rhodopsins are membrane-embedded photoreceptors found in all major taxonomic kingdoms using retinal as their chromophore. They play well-known functions in different biological systems, but their roles in fungi remain unknown. The filamentous fungus Fusarium fujikuroi contains two putative rhodopsins, CarO and OpsA. The gene carO is light-regulated, and the predicted polypeptide contains all conserved residues required for proton pumping. We aimed to elucidate the expression and cellular location of the fungal rhodopsin CarO, its presumed proton-pumping activity and the possible effect of such function on F. fujikuroi growth. In electrophysiology experiments we confirmed that CarO is a green-light driven proton pump. Visualization of fluorescent CarO-YFP expressed in F. fujikuroi under control of its native promoter revealed higher accumulation in spores (conidia) produced by light-exposed mycelia. Germination analyses of conidia from carO\(^{-}\) mutant and carO\(^{+}\) control strains showed a faster development of light-exposed carO-germlings. In conclusion, CarO is an active proton pump, abundant in light-formed conidia, whose activity slows down early hyphal development under light. Interestingly, CarO-related rhodopsins are typically found in plant-associated fungi, where green light dominates the phyllosphere. Our data provide the first reliable clue on a possible biological role of a fungal rhodopsin.
Enteric pathogens often cycle between virulent and saprophytic lifestyles. To endure these frequent changes in nutrient availability and composition bacteria possess an arsenal of regulatory and metabolic genes allowing rapid adaptation and high flexibility. While numerous proteins have been characterized with regard to metabolic control in pathogenic bacteria, small non-coding RNAs have emerged as additional regulators of metabolism. Recent advances in sequencing technology have vastly increased the number of candidate regulatory RNAs and several of them have been found to act at the interface of bacterial metabolism and virulence factor expression. Importantly, studying these riboregulators has not only provided insight into their metabolic control functions but also revealed new mechanisms of post-transcriptional gene control. This review will focus on the recent advances in this area of host-microbe interaction and discuss how regulatory small RNAs may help coordinate metabolism and virulence of enteric pathogens.
Two lineages of Salmonella enterica serovar Typhimurium (S. Typhimurium) of multi-locus sequence type ST313 have been linked with the emergence of invasive Salmonella disease across sub-Saharan Africa. The expansion of these lineages has a temporal association with the HIV pandemic and antibiotic usage. We analysed the whole genome sequence of 129 ST313 isolates representative of the two lineages and found evidence of lineage-specific genome degradation, with some similarities to that observed in S. Typhi. Individual ST313 S. Typhimurium isolates exhibit a distinct metabolic signature and modified enteropathogenesis in both a murine and cattle model of colitis, compared to S. Typhimurium outside of the ST313 lineages. These data define phenotypes that distinguish ST313 isolates from other S. Typhimurium and may represent adaptation to a distinct pathogenesis and lifestyle linked to an-immuno-compromised human population.
The human-pathogenic bacterium Salmonella enterica adjusts and adapts to different environments while attempting colonization. In the course of infection nutrient availabilities change drastically. New techniques, “-omics” data and subsequent integration by systems biology improve our understanding of these changes. We review changes in metabolism focusing on amino acid and carbohydrate metabolism. Furthermore, the adaptation process is associated with the activation of genes of the Salmonella pathogenicity islands (SPIs). Anti-infective strategies have to take these insights into account and include metabolic and other strategies. Salmonella infections will remain a challenge for infection biology.
The infectious intracellular lifestyle of Salmonella enterica relies on the adaptation to nutritional conditions within the Salmonella-containing vacuole (SCV) in host cells. We summarize latest results on metabolic requirements for Salmonella during infection. This includes intracellular phenotypes of mutant strains based on metabolic modeling and experimental tests, isotopolog profiling using (13)C-compounds in intracellular Salmonella, and complementation of metabolic defects for attenuated mutant strains towards a comprehensive understanding of the metabolic requirements of the intracellular lifestyle of Salmonella. Helpful for this are also genomic comparisons. We outline further recent studies and which analyses of intracellular phenotypes and improved metabolic simulations were done and comment on technical required steps as well as progress involved in the iterative refinement of metabolic flux models, analyses of mutant phenotypes, and isotopolog analyses. Salmonella lifestyle is well-adapted to the SCV and its specific metabolic requirements. Salmonella metabolism adapts rapidly to SCV conditions, the metabolic generalist Salmonella is quite successful in host infection.
The human-pathogenic bacterium Salmonella enterica adjusts and adapts to different environments while attempting colonization. In the course of infection nutrient availabilities change drastically. New techniques, "-omics" data and subsequent integration by systems biology improve our understanding of these changes. We review changes in metabolism focusing on amino acid and carbohydrate metabolism. Furthermore, the adaptation process is associated with the activation of genes of the Salmonella pathogenicity islands (SPIs). Anti-infective strategies have to take these insights into account and include metabolic and other strategies. Salmonella infections will remain a challenge for infection biology.
RNAseq analysis of Aspergillus fumigatus in blood reveals a just wait and see resting stage behavior
(2015)
Background:
Invasive aspergillosis is started after germination of Aspergillus fumigatus conidia that are inhaled by susceptible individuals. Fungal hyphae can grow in the lung through the epithelial tissue and disseminate hematogenously to invade into other organs. Low fungaemia indicates that fungal elements do not reside in the bloodstream for long.
Results:
We analyzed whether blood represents a hostile environment to which the physiology of A. fumigatus has to adapt. An in vitro model of A. fumigatus infection was established by incubating mycelium in blood. Our model allowed to discern the changes of the gene expression profile of A. fumigatus at various stages of the infection. The majority of described virulence factors that are connected to pulmonary infections appeared not to be activated during the blood phase. Three active processes were identified that presumably help the fungus to survive the blood environment in an advanced phase of the infection: iron homeostasis, secondary metabolism, and the formation of detoxifying enzymes.
Conclusions:
We propose that A. fumigatus is hardly able to propagate in blood. After an early stage of sensing the environment, virtually all uptake mechanisms and energy-consuming metabolic pathways are shut-down. The fungus appears to adapt by trans-differentiation into a resting mycelial stage. This might reflect the harsh conditions in blood where A. fumigatus cannot take up sufficient nutrients to establish self-defense mechanisms combined with significant growth.
Vergleichende Proteomanalyse eines avirulenten und virulenten Stammes von Legionella pneumophila Sg1 Subgruppe OLDA unter Anwendung der zweidimensionalen Gelelektrophorese. Die Stämme unterliegen einer spontanen LPS-Phasenvariation und unterscheiden sich phänotypisch in multiplen Eigenschaften. Es zeigten sich different exprimierte Proteine der Membranoberfläche, der LPS-Biosynthese und des Bakterienstoffwechsels.
Staphylococcus aureus ist ein bedeutender opportunistischer Krankheitserreger, der eine Vielzahl von Infektionen in Menschen und Tieren hervorrufen kann. Das Krankheitsbild reicht von leichten Hautinfektionen bis hin zu lebensbedrohlichen Infektionen wie Endokarditis, Sepsis oder Pneumonien. S. aureus ist ein Haupterreger nosokomialer Infektionen. Besonders die Antibiotikaresistenzentwicklung von S. aureus–Stämmen ist problematisch. Als wirksame Antibiotika können zur Zeit oft nur noch Vancomycin, Synercid oder Linezolid zur Therapie eingesetzt werden. Die alarmierende Resistenzentwicklung in S. aureus verdeutlicht, dass die Entwicklung neuer Antibiotika und die Identifizierung neuer bakterieller Angriffsstrukturen dringend erforderlich ist. Gängige antiinfektive Therapeutika sind gegen die bakterielle Zellwandsynthese, den DNA- und RNA-Stoffwechsel oder die Proteinbiosynthese gerichtet. In dieser Arbeit sollten Virulenz-relevante Zielstrukturen für die Entwicklung neuer Antibiotika untersucht werden. Insgesamt wurden sieben Gene analysiert, von denen vier zu Anfang dieser Arbeit in S. aureus noch nicht charakterisiert waren. Die Zielgene (clpP, purH, ssrA und smpB) in S. aureus sollten deletiert werden, um ihre Überlebensnotwendigkeit in vitro- und in vivo zu überprüfen. Eine Deletion gelang bei den Genen clpP und purH, die somit als nicht essenziell in S. aureus zu betrachten sind. Die bereits zuvor als nicht-essenziell charakterisierten Gene arlR, arlS und putP wurden deletiert und die Mutanten dclpP, darlR, darlS, dpurH und dputP wurden phänotypisch in Hinsicht auf ihren Einfluss auf die Pathogenität in S. aureus analysiert. Die differenzielle Genexpression der Mutanten dclpP und darlR wurde mit Hilfe von Microarray-Hybridisierungsexperimenten untersucht. Die ∆clpP-Mutante zeigte einen starken Wachstumsdefekt bei verschiedenen Temperaturen (30, 37, 42°C) und war nicht mehr in der Lage bei 20°C zu wachsen. Ebenso war das Wachstum unter anaeroben Bedingungen stark beeinträchtigt. Der Stamm dclpP wies eine verringerte hämolytische Aktivität sowie eine verminderte Adhärenz an Polystyren auf. Außerdem konnte eine stark erhöhte autolytische Aktivität in einem Triton X-100-Assay beobachtet werden. In einem Invasions-Zellkulturassay mit 293T-Epithelzellen konnte eine ~10-fach erhöhte Invasivität im Vergleich zu dem isogenen Wildtyp festgestellt werden. Die Komplementierung der ∆clpP-Mutante durch Einführung eines clpP-Expressionsvektors führte nahezu bei allen getesteten Bedingungen zur Wiederherstellung des wildtypischen Phänotyps. Die Transkriptomanalyse der dclpP-Mutante ergab eine deutliche Veränderung in der Genexpression (15 % aller Gene). Eine computerunterstützte Analyse der Upstreambereiche der deregulierten Gene führte zu der Identifizierung verschiedener Regulons, die bei der bakteriellen Antwort auf verschiedene Stressbedingungen eine Rolle spielen. Die clpP-Deletion betrifft besonders Regulatoren, deren Aktivität in Abhängigkeit zu veränderten Redox-Bedingungen reguliert wird, wie z. B. verschiedenen Stressbedingungen und Anaerobiose. Die Konstruktion der darlR- und darlS-Mutanten führte zu einer gesteigerten hämolytischen Aktivität, einer erhöhten Adhärenz an Polystyren sowie einer erhöhten autolytischen Aktivität in Triton X-100-Assays. Die Internalisierungsrate durch 293T-Epithelzellen war vermindert. Die darlR-Mutante wurde in einem Katheter-assoziierten Infektionsmodell in Ratten eingesetzt. Die kompetitive Infektion mit Mutante und Wildtyp ergab einen deutlichen Nachteil bei der Etablierung einer Infektion durch die Mutante. Die Transkriptomanalyse der 8325darlR-Mutante in der exponenziellen und in der stationären Phase unterstreicht den großen Einfluss des ArlRS-Zwei-Komponenten-Systems auf die Regulation der Genexpression in S. aureus. In der exponenziellen Phase wurden insgesamt 5 % und in der stationären Phase 15 % der Gene differenziell exprimiert. dpurH- und dputP-Mutanten wiesen in vitro keine Veränderungen im Wachstums-verhalten, der Biofilmbildung oder hämolytischen Aktivität auf. In einem Infektionsmodell in Ratten führte die Deletion von purH in dem S. aureus-Stamm MA12 zu einer signifikanten Verminderung der Virulenz. Die Herstellung von smpB- und ssrA-Deletionsmutanten verlief ohne Erfolg. Es wurde versucht, einen direkten Nachweis für den essenziellen Charakter dieser Gene durch den Einsatz konditional letaler Expressionssysteme zu erbringen. Weder der Austausch des wildtypischen durch einen regulierbaren Promotor noch eine Antisense-RNA-Strategie war für eine eindeutige Klärung dieser Frage ausreichend. Es konnte durch diese Arbeit jedoch gezeigt werden, dass die Antisense-RNA-Strategie eine Beeinträchtigung des Wachstums von S. aureus bewirkt.