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1	Novel anti-infectives against pathogenic bacteria / Neue Anti-infectiva gegen pathogene Bakterien Balasubramanian, Srikkanth January 2018 (has links) (PDF) Marine sponge-associated actinomycetes are reservoirs of diverse natural products with novel biological activities. Their antibiotic potential has been well explored against a range of Gram positive and negative bacteria. However, not much is known about their anti-infective or anti-virulence potential against human pathogens. This Ph.D. project aimed to investigate the anti-infective (anti-Shiga toxin and anti-biofilm) potential of sponge-derived actinobacteria through identification and isolation of their bioactive metabolites produced and characterizing their mechanism of action by transcriptomics. This thesis is divided into three studies with the overall objective of exploring the anti-infective efficacy of actinomycetes-derived extracts and compound(s) that could possibly be used as future therapeutics. The first study deals with investigation on the anti-Shiga toxin effects of sponge-associated actinomycetes. Diarrheal infections pose a huge burden in several developing and developed countries. Diarrheal outbreaks caused by Enterohemorrhagic Escherichia coli (EHEC) could lead to life-threatening complications like gastroenteritis and haemolytic uremic syndrome (HUS) if left untreated. Shiga toxin (Stx) produced by EHEC is a major virulence factor that negatively affects the human cells, leading them to death via apoptosis. Antibiotics are not prescribed against EHEC infections since they may enhance the risk of development of HUS by inducing the production and release of Stx from disintegrating bacteria and thereby, worsening the complications. Therefore, an effective drug that blocks the Stx production without affecting the growth needs to be urgently developed. In this study, the inhibitory effects of 194 extracts and several compounds originating from a collection of marine sponge-derived actinomycetes were evaluated against the Stx production in EHEC strain EDL933 with the aid of Ridascreen® Verotoxin ELISA assay kit. It was found that treatment with the extracts did not lead to significant reduction in Stx production. However, strepthonium A isolated from the culture of Streptomyces sp. SBT345 (previously cultivated from the Mediterranean sponge Agelas oroides) reduced the Stx production (at 80 μM concentration) in EHEC strain EDL933 without affecting the bacterial growth. The structure of strepthonium A was resolved by spectroscopic analyses including 1D and 2D-NMR, as well as ESI-HRMS and ESI-HRMS2 experiments. This demonstrated the possible application of strepthonium A in restraining EHEC infections. VI In the second study, the effect of marine sponge-associated actinomycetes on biofilm formation of staphylococci was assessed. Medical devices such as contact lenses, metallic implants, catheters, pacemakers etc. are ideal ecological niches for formation of bacterial biofilms, which thereby lead to device-related infections. Bacteria in biofilms are multiple fold more tolerant to the host immune responses and conventional antibiotics, and hence are hard-to-treat. Here, the anti-biofilm potential of an organic extract derived from liquid fermentation of Streptomyces sp. SBT343 (previously cultivated from the Mediterranean sponge Petrosia ficiformis) was reported. Results obtained in vitro demonstrated its anti-biofilm (against staphylococci) and non-toxic nature (against mouse macrophage (J774.1), fibroblast (NIH/3T3) and human corneal epithelial cell lines). Interestingly, SBT343 extract could inhibit staphylococcal biofilm formation on polystyrene, glass and contact lens surfaces without affecting the bacterial growth. High Resolution Fourier Transform Mass Spectrometry (HR-MS) analysis indicated the complexity and the chemical diversity of components present in the extract. Preliminary physio-chemical characterization unmasked the heat stable and non-proteinaceous nature of the active component(s) in the extract. Finally, fractionation experiments revealed that the biological activity was due to synergistic effects of multiple components present in the extract. In the third study, anti-biofilm screening of 50 organic extracts generated from solid and liquid fermentation of 25 different previously characterized sponge-derived actinomycetes was carried out. This led to identification of the anti-biofilm organic extract derived from the solid culture of Streptomyces sp. SBT348 (previously cultivated from the Mediterranean sponge Petrosia ficiformis). Bioassay-guided fractionation was employed to identify the active fraction Fr 7 in the SBT348 crude extract. Further purification with semi-preparative HPLC led to isolation of the bioactive SKC1, SKC2, SKC3, SKC4 and SKC5 sub-fractions. The most active sub-fraction SKC3 was found to be a pure compound having BIC90 and MIC values of 3.95 μg/ml and 31.25 μg/ml against S. epidermidis RP62A. SKC3 had no apparent toxicity in vitro on cell lines and in vivo on the greater wax moth Galleria melonella larvae. SKC3 was stable to heat and enzymatic treatments indicating its non-proteinaceous nature. HR-MS analysis revealed the mass of SKC3 to be 1258.3 Da. Structure elucidation of SKC3 with the aid of 1D and 2D-NMR data is currently under investigation. Further, to obtain insights into the mode of action of SKC3 on S. epidermidis RP62A, RNA sequencing was done. Transcriptome data revealed that SKC3 was recognized by RP62A at 20 min and SKC3 negatively interfered with the central metabolism of staphylococci at 3 h. Taken VII together, these findings suggest that SKC3 could be a lead structure for development of new anti-staphylococcal drugs. Overall, the results obtained from this work underscore the anti-infective attributes of actinomycetes consortia associated with marine sponges, and their applications in natural product drug discovery programs. / Meeresschwamm-assoziierte Actinomyceten stellen ein Reservoir für verschiedene natürliche Produkte mit neuartigen biologischen Aktivitäten dar. Ihr antibiotisches Potenzial gegenüber einer Reihe von Gram-negativen und -positiven Bakterien ist bereits intensiv erforscht worden. Wenig ist allerdings über ihre antiinfektive und antivirulente Wirksamkeit gegenüber menschlichen Pathogenen bekannt. Ziel dieser Doktorarbeit war es, die antiinfektiven Fähigkeiten (anti-Shiga-Toxin und anti-Biofilm) der aus Schwämmen isolierten Actinobakterien zu untersuchen. Hierfür wurden bioaktive Metabolite der Actinobakterien identifiziert und isoliert und abschließend wurde ihr Wirkmechanismus mit Hilfe einer Transkriptomanalyse charakterisiert. Diese Arbeit ist in drei Studien gegliedert, welche alle zum Ziel hatten die antiinfektive Wirksamkeit von aus Actinomyceten gewonnenen Extrakten und Komponente(n), welche möglicherweise als zukünftige Therapeutika dienen könnten, zu untersuchen. Die erste Studie befasst sich mit den anti-Shiga-Toxin Effekten der Meeresschwamm- assoziierten Actinomyceten. Durchfallinfektionen stellen in vielen Entwicklungsländern aber auch in Industrieländern eine große Gefahr dar. Durchfallerkrankungen die durch enterohämorrhagische Escherichia coli (EHEC) hervorgerufen werden, können sich zu lebensbedrohlichen Komplikationen wie Gastroenteritis oder dem hämolytisch urenischen Syndrom (HUS) weiterentwickeln. Das von den EHEC Stämmen produzierte Shiga-Toxin (Stx) stellt hierbei den Haupt Virulenz Faktor dar, welcher die eukaryotische Proteinsynthese menschlicher Zellen negativ beeinflusst, was wiederum den Zelltod durch Apoptose zur Folge hat. Die Behandlung der EHEC-Patienten mit Antibiotika wird nicht empfohlen, da dies zu einem Anstieg von freigesetztem Stx der zersetzen Bakterien führen könnte, wodurch das Risiko für die Entwicklung des HUS ansteigt. Aus diesem Grund werden effektive Medikamente dringen benötigt, welche die Stx Produktion blockieren ohne das Wachstum der Bakterien zu beeinflussen. In dieser Studie wurden 194 Extrakte und einige isolierte Komponenten von aus Schwämmen gewonnenen Actinomyceten auf ihren negativen Einfluss auf die Stx Produktion des EHEC Stammes EDL933 mit der Hilfe des Ridascreen® Verotoxin ELISA Kits untersucht. Es konnte gezeigt werden, dass die Zugabe der Extrakte keinen signifikanten Einfluss auf die Stx Produktion hatte. Strepthonium A auf der anderen Seite, welches aus Streptomyces sp. SBT345 isoliert wurde (vom mediterranen Schwamm Agelas oroides) konnte die Stx Produktion von EDL933 bei einer Konzentration von 80 µM reduzieren ohne das Wachstum des EHEC Stammes zu beeinflussen. Die Struktur von Strepthonium A wurde mittels spektroskopischer Analyse (1D- und 2D-NMR), sowie mittels ESI-HRMS und ESI-HRMS2 Experimenten entschlüsselt. Basierend auf diesen Ergebnissen könnte Strepthonium A eine mögliche Alternative oder Zusatz in der Behandlung einer EHEC Infektion darstellen. In der zweiten Studie wurde der Einfluss der Meeresschwamm-assoziierten Actinomyceten auf die Biofilmbildung von Staphylokokken bewertet. Medizinische Produkte wie Kontakt Linsen, metallische Implantate, Katheter, Herzschrittmacher, usw. stellen optimale ökologische Nischen für die Ausbildung von bakteriellen Biofilmen dar, wodurch Infektionen im Menschen hervorgerufen werden können. Bakterien in einem Biofilm sind deutlich toleranter gegenüber der Immunantwort ihres Wirtes sowie gegenüber konventionellen Antibiotika und sind daher schwer zu bekämpfen. In dieser Studie wurde das anti-Biofilm Potential eines organischen Extrakts der flüssigen Fermentation von Streptomyces sp. SBT343 (vom mediterranen Schwamm Petrosia ficiformis) ermittelt. In vitro Ergebnisse zeigten, dass das organische Extrakt anti-Biofilm (gegenüber Staphylococci) Fähigkeiten besitzt und nicht toxisch für Maus Makrophagen (J774.1), Fibroblasten (NIH/3T3) und humane korneale Epithelzellen ist. Zudem konnte gezeigt werden, dass das SBT343 Extrakt die Ausbildung eines Biofilms von Staphylokokken auf den Oberflächen von Polystyrol, Glass und Kontaktlinsen unterbinden konnte ohne das bakterielle Wachstum zu beeinflussen. Die hochauflösende Fouriertransformation-Massenspektrometrie (HR-MS) Analyse konnte die Komplexität sowie die chemische Vielfalt an Komponenten im Extrakt aufzeigen. Eine vorläufige, physio-chemische Charakterisierung deutet darauf hin, dass die aktive Komponente im Extrakt hitzestabil und nicht proteinartiger Natur ist. Abschließend konnte durch Fraktionierungsexperimente gezeigt werden, dass die biologische Aktivität auf synergistischen Effekten mehrerer Komponenten im Extrakt beruht. In einer dritten Studie wurden 50 organische Extrakte, welche aus fester und flüssiger Fermentierung von 25 verschiedenen aus Meeresschwämmen isolierten Actinomyceten gewonnen wurden, auf anti-Biofilm-Aktivität untersucht. Hierbei wurde die anti-Biofilm Aktivität des organischen Extrakts der Festkultur von Streptomyces sp. SBT348 (vom mediterranen Schwamm Petrosia ficiformis) identifiziert. Eine Bioassay gestützte Fraktionierung führte zu der Identifikation der aktiven Fraktion Fr 7 im SBT348 Extrakt. Durch weitere Aufreinigung des Extrakts mit einer semipräparativen HPLC, konnten die bioaktiven Sub-Fraktionen SKC1, SKC2, SKC3, SKC4 und SKC5 isoliert werden. Die Sub- Fraktion SKC3 hatte den stärksten anti-Biofilm Effekt und bestand aus einer reinen Verbindung mit BIC90 und MIC Werten von 3,95 µg/ml und 31,25 µg/ml gegen S. epidermidis RP62A. SKC3 zeigte weder erkennbare Toxizität gegenüber Zelllinien in vitro noch gegenüber den Larven der großen Wachsmotte Galleria melonella in vivo. SKC3 war Hitze- und Enzym-resistent, was auf eine nicht proteinartige Natur hindeutet. Eine HR-MS Analyse ergab, dass die Masse von SKC3 1258,3 Da beträgt. Die Strukturanalyse von SKC3 durch 1D und 2D-NMR ist zurzeit in Bearbeitung. Um weiteres Verständnis über den anti-Biofilm Wirkmechanismus von SKC3 auf S. epidermidis RP62A zu erlangen, wurde eine RNA Sequenzierungsanalyse durchgeführt. Die Transkriptomanalyse zeigte, dass SKC3 von RP62A nach einer 20-minütigen Inkubationszeit erkannt wird und dass SKC3 den zentralen Metabolismus des Staphylokokken Stammes nach 3 h negativ beeinflusst. Zusammengenommen deuten die Ergebnisse darauf hin, dass SKC3 als Leitstruktur für die Entwicklung neuer anti- Staphylokokken Medikamente dienen könnte. Zusammenfassend heben die Ergebnisse dieser Arbeit die antiinfektiven Eigenschaften der Meeresschwamm-assoziierte Actinomyceten hervor und bieten eine Möglichkeit für die Nutzung dieser in Wirkstoffentwicklungsprogrammen. Marine sponges Streptomyces Staphylococci Enterohemorrhagic Escherichia coli Biofilm ddc:570
2	Evaluation of Escherichia coli probiotic candidates for combating EHEC in the food chain using competition analysis in bovine feces Stigers, Linnea January 2018 (has links) Enterohemorrhagic E. coli, EHEC, is a verotoxin producing, zoonotic pathogen, which causes diseases in humans such as bloody or watery diarrhea. Microorganisms compete for limited living space, nutrients and other resources and therefore other microorganisms are EHECs biggest competitors. To avoid outbreaks and infections with EHEC, one possible approach is to use harmless but competitive bacteria as probiotics. Therefore, the aim of this study was to evaluate three probiotic E. coli strains and their ability to outcompete EHEC in bovine feces. Ten different cattle fecal samples from three different farms were used to mix with the three probiotic and EHEC strains. The mixture was diluted and cultivated at 0 h as a control and then incubated for 48 h at 20°C and 37°C before dilution and cultivation on CT-SMaC. Colonies was counted and ratios between EHEC and probiotic E. coli before and after incubation were calculated. Kruskal-Wallis test with Dunn’s test as post hoc test were used to see if observed reductions of EHEC were significant or not. In 37°C, strain 10 was the only strain producing a significant reduction of EHEC. In contrast, no significant reduction was observed at 20°C in any of the strains. Future research studying other factors and performed on live cattle models are necessary to confirm the usefulness of the studied probiotic candidates. However, these results indicate probiotics can be a useful tool to avoid infections and big outbreaks of EHEC in the future. Enterohemorrhagic Escherichia coli clade 8 O157:H7 cattle VTEC Biomedical Laboratory Science/Technology
3	Cell stress markers during development of hemolytic uremic syndrome and acute kidney injury Motomochi, Amanda 22 January 2016 (has links) Enterohemorrhagic E. coli (EHEC) infections are a leading cause of foodborne illness in the United States. Shiga-like toxins are produced that can cause hemorrhagic colitis and can lead to dangerous complications, such as acute kidney injury and hemolytic uremic syndrome (HUS). There are currently no specific treatments for HUS, and therefore more research into EHEC and HUS needs to be done. Our study focuses on Shiga-like toxin induction of endoplasmic reticulum (ER) stress in in vitro and in vivo systems, using human monocyte-like THP-1 cells and a non-human primate model of HUS. We used qPCR to determine the levels of ER stress marker expression induced by both Shiga-like toxin 1 (Stx1) and Shiga-like toxin 2 (Stx2) challenges. We also looked at ER stress marker expression in non-human primates that survived a lethal Stx2 challenge after being given a Stx2 binding tetravalent peptide. We expected to see increased ER stress marker expression in THP-1 cells challenged with both Shiga-like toxins and in animals that received lethal doses of the toxins. Although results were inconclusive for THP-1 cell experiments, our preliminary non-human primate data suggest that the timing of ER stress marker production is important, and Shiga-like toxins may suppress the unfolded protein response (UPR) in some baboon tissues. We also show that the therapeutic peptide TVP may reverse this UPR suppression and relieve ER stress leading to animal survival. Our study, along with the current literature, shows that Shiga-like toxin induced ER stress is a promising area for future study. Pathology Enterohemorrhagic Escherichia coli Endoplasmic reticulum stress Hemolytic uremic syndrome Shiga-like toxins
4	Investigating the contributions of leukocyte responses and kidney cell stress on Shiga- toxin pathogenesis Parello, Caitlin Suzanne Leibowitz 12 March 2016 (has links) BACKGROUND: Shiga toxin (Stx)-producing enterohemorrhagic Escherichia coli (EHEC) are emerging food- and water- borne pathogens and a leading cause of acute renal failure in otherwise healthy children. Ribotoxic Shiga toxins are the primary virulence factors and are responsible for the potentially lethal EHEC complication of hemolytic uremic syndrome (HUS). HUS, defined clinically by microangiopathic hemolytic anemia, thrombocytopenia and thrombotic microangiopathy which contribute to acute kidney injury or renal failure, is associated with significant patient morbidity. No pathogen- or toxin- specific therapeutic exists, and antibiotic use is contraindicated. Understanding the molecular mechanisms of Stx toxicity could lead to the development of Stx specific therapies. HYPOTHESIS: Experimental evidence suggests a role for leukocytes in systemic Stx2 trafficking and in Stx2 mediated kidney pathology. Cell stress responses, such as the ER stress response and ribosomal stress response, are hypothesized to induce apoptosis, and ultimately cell death, contributing to kidney injury; however these processes have only been described in vitro. If leukocyte and kidney cell stress responses are playing significant roles in in vivo Stx2 kidney injury, then down-regulation of these processes may provide therapeutic benefit. RESULTS: Mice injected with Stx2 or infected with Stx2-producing bacteria developed lethal kidney injury as judged by biomarkers and histopathology. Experimentally induced leukopenia did not alter kidney injury in either model, but did cause striking increases in the intestinal bacterial colonization which was dependent on the presence of Stx2. No Stx binding capacity was observed for either murine or human leukocytes ex vivo. Transcriptional evidence of kidney ER stress and apoptotic biomarkers were observed in both models of Stx2-mediated kidney injury, but down-regulation of these processes did not yield therapeutic benefit. CONCLUSIONS: Contrary to the current disease paradigm, no major role for leukocytes in systemic Stx2 trafficking or kidney injury was observed in vivo, but a novel role for host immune responses to Stx2 in the control of intestinal colonization by Stx2-producing bacteria was identified. Cell stress and apoptosis is induced by Stx2 in vivo but prevention of these is not sufficient to appreciably alter organ injury or survival in the murine models. Pathology Cell stress Enterohemorrhagic Escherichia coli Kidney injury Shiga toxin Hemolytic uremic syndrome
5	Functional Elements of EspF<sub>u</sub>, an Enterohemorrhagic <em>E. coli</em> Effector that Stimulates Actin Assembly: A Dissertation Skehan, Brian M. 17 June 2009 (has links) Enterohemorrhagic Escherichia coli O157:H7 (EHEC) is an attaching and effacing pathogen that upon attachment to host cells, induce characteristic attaching and effacing lesions and formation of F-actin rich pedestals beneath sites of bacterial attachment. EHEC harbors a Type III secretion system through which it delivers dozens of effectors into the host cell. The two secreted effectors critical for EHEC-mediated actin pedestal formation are the translocated intimin receptor (Tir) and EspFU. EspFU consists of an N-terminal secretion signal and a C-terminus containing six tandem 47-residue proline-rich repeats, each of which can bind and activate the actin nucleation promoting factor N-WASP. Structural and functional analyses described here have identified the mechanism of N-WASP activation by EspFU and the minimal domains and specific residues required for this activity. While EspFU and Tir are the only bacterial effectors required for F-actin pedestal formation, recruitment of EspFU to Tir is mediated by an unidentified putative host factor. To identify the host factor responsible for linking these two effectors, a combination of in vitro and functional assays were used to identify the host factor, IRTKS and the residues required for these interactions were defined. Further, the presence of at least two 47-residue repeats in all characterized clinical isolates of canonical EHEC strains led us to address the minimal requirements for EspFU functional domains to promote recruitment to Tir and N-WASP activation. Here we show that two proline-rich elements of EspFU are required for recruitment of EspFU by IRTKS to sites of bacterial attachment. Furthermore, once artificially clustered at the membrane, a single N-WASP binding element of EspFU can induce actin pedestal formation. Enterohemorrhagic Escherichia coli Escherichia coli Proteins Microfilament Proteins Actins Carrier Proteins Receptors Cell Surface Amino Acids, Peptides, and Proteins Bacteria Macromolecular Substances
6	EspFU, an Enterohemorrhagic E. Coli Secreted Effector, Hijacks Mammalian Actin Assembly Proteins by Molecular Mimicry and Repetition: A Dissertation Lai, YuShuan (Cindy) 25 April 2014 (has links) Enterohemorrhagic E. coli (EHEC) is a major cause of food borne diarrheal illness worldwide. While disease symptoms are usually self-resolving and limited to severe gastroenteritis with bloody diarrhea, EHEC infection can lead to a life threatening complication known as Hemolytic Uremic Syndrome (HUS), which strikes children disproportionately and is the leading cause of kidney failure in children. Upon infection of gut epithelia, EHEC produces characteristic lesions called actin pedestals. These striking formations involve dramatic rearrangement of host cytoskeletal proteins. EHEC hijacks mammalian signaling pathways to cause destruction of microvilli and rebuilds the actin cytoskeleton underneath sites of bacterial attachment. Here, we present a brief study on a host factor, Calpain, involved in microvilli effacement, and an in depth investigation on a bacterial factor, EspFU, required for actin pedestal formation in intestinal cell models. Calpain is activated by both EHEC and the related pathogen, enteropathogenic E. coli (EPEC), during infection and facilitates microvilli disassembly by cleavage of a key membrane-cytoskeleton anchoring substrate, Ezrin. Actin pedestal formation is facilitated by the injection of two bacterial effectors, Tir and EspFU, into host cells, which work in concert to manipulate the host actin nucleators N-WASP and Arp2/3. EspFU hijacks key host signaling proteins N-WASP and IRTKS by mimetic displacement and has evolved to outcompete mammalian host ligands. Multiple repeats of key functional domains of EspFU are essential for actin pedestal activity through proper localization and competition against the an abundant host factor Eps8 for binding to IRTKS. Actin Cytoskeleton Actins Calpain Cytoskeletal Proteins Enterohemorrhagic Escherichia coli Escherichia coli Infections Escherichia coli Proteins Microvilli Dissertations, UMMS Bacterial Infections and Mycoses Bacteriology Cellular and Molecular Physiology Microbial Physiology
7	Influence du microbiote intestinal sur le métabolisme et la virulence des Escherichia coli entérohémorragiques Le Bihan, Guillaume 01 1900 (has links) No description available. Escherichia coli entérohémorragique Enterohemorrhagic Escherichia coli Microbiote intestinal Intestinal microbiota Adaptation Métabolisme Metabolism Virulence Régulation Regulation
8	Survie et pathogénicité des EHEC dans l'environnement digestif : Interactions avec le microbiote et l'épithélium intestinal. : Influence de l'administration de levures probiotiques. / Survival and Pathogenicity of Enterohemorrhagic Escherichia Coli in Digestive Environment : Interactions with the Microbiota and Intestinal Epithelium. : Influence of the Administration of Probiotic Yeasts. Cordonnier, Charlotte 18 December 2015 (has links) Les Escherichia coli entérohémorragiques (EHEC) sont des pathogènes majeurs pour l’homme responsables de toxi-infections alimentaires pouvant évoluer vers des complications potentiellement mortelles. La pathogénicité de ces souches est essentiellement due à la production de Shiga-toxines (Stx), même si d’autres facteurs semblent jouer un rôle important dans la virulence, comme des facteurs d’adhésion. La survie et la régulation des facteurs de virulence des EHEC dans l’environnement digestif humain sont des facteurs clés dans la pathogénicité bactérienne, mais restent à ce jour mal décrits, essentiellement en raison d’un manque de modèles d’étude adaptés. De plus, l’absence de traitement spécifique a conduit à s’intéresser à des moyens préventifs et/ou curatifs alternatifs, comme l’utilisation de probiotiques. L’objectif de ce travail de thèse est (i) de mieux comprendre le comportement de la souche de référence EHEC O157:H7 EDL933 dans l’environnement digestif humain simulé, et en particulier ses interactions avec le microbiote résident et l’épithélium intestinal, et (ii) d’évaluer l’effet antagoniste d’une souche de levure probiotique vis-à-vis de la survie, la virulence et l’interaction du pathogène avec l’épithélium intestinal, à l’aide d’approches in vitro et in vivo complémentaires. En modèles digestifs in vitro, la souche EHEC survit dans l’estomac, voire se multiplie dans les parties distales de l’intestin grêle, alors qu’elle ne se maintient pas dans l’environnement colique. Les gènes de virulence codant les Stx et des adhésines majeurs (intimine et « Long Polar Fimbriae » ou Lpf) sont surexprimés dès les parties hautes du tractus digestifs, et ce, même en absence de cellules épithéliales. Les conditions rencontrées dans le tractus digestif supérieur de l’enfant, comparativement à celui de l’adulte, conduisent à une survie et un niveau d’expression des gènes codant les Stx et les Lpf plus élevés chez l’enfant, ce qui peut contribuer à expliquer la grande sensibilité de cette population aux infections à EHEC. Enfin, les Lpf semblent jouent un rôle clé dans le ciblage spécifique des cellules M et le tropisme des EHEC pour les plaques de Peyer, et ce, à la fois in vitro (cellules M en culture) et in vivo (anses iléales murines). Même si elle ne modifie pas la survie du pathogène dans l’environnement colique, la levure probiotique S. cerevisiae CNCM I-3856 a montré des propriétés antagonistes intéressantes vis-à-vis d’EHEC O157:H7 en (i) modulant favorablement l’activité fermentaire du microbiote intestinal, (ii) diminuant significativement l’expression des gènes codant les Stx et (iii) inhibant la translocation bactérienne au travers des plaques de Peyer et les lésions hémorragiques associées. Par ailleurs, l’effet du pathogène et des probiotiques sur le microbiote colique est individu dépendant, confortant l’hypothèse que des facteurs associés à l’hôte, comme le microbiote, pourraient conditionner l’évolution clinique des infections à EHEC et l’efficacité d’une stratégie probiotique.Ce travail de thèse contribue à une meilleure compréhension du comportement des EHEC dans l’environnement digestif humain et confirme l’intérêt d’une stratégie probiotique dans la lutte contre le pathogène. Une étude plus approfondie du transcriptome du pathogène dans l’environnement digestif et une analyse par des méthodes haut débit du microbiote intestinal permettraient de continuer à mieux décrire la physiopathologie des infections à EHEC et comprendre les mécanismes associés à l’effet antagoniste des probiotiques. / The enterohemorrhagic Escherichia coli (EHEC) are major zoonotic pathogens responsible for food-borne infectionwhich leads to life-threatening complications in humans. The main virulence determinant of EHEC is the production of Shigatoxins (Stx), even if other factors seem to play an important role in virulence, such as adhesion factors. Survival and virulenceof EHEC strains in the human digestive environment are a key factor in bacterial pathogenesis but remains unclear owing tolack of relevant model. Moreover, no specific treatment has led to interest in preventative and / or curative alternatives, suchas using probiotics. The objective of this study is to better understand the behavior of the reference strain EHEC O157:H7EDL933 in the entire digestive tract, and in particular its interaction with the resident microbiota and the intestinal epithelium,and to evaluate the antagonistic effect of the probiotic yeast, Saccharomyces cerevisiae CNCM I-3856, using in vitro and in vivo complementary approaches.In vitro, bacterial mortality was noticed in the stomach, whereas bacterial growth resumption was observed in thedistal parts of the small intestine and the pathogen was not able to maintain in the human colonic conditions. Virulence genesencoding Stx and adhesins (intimin and “Long polar fimbriae”) are upregulated in the upper parts of the digestive tract. A ten-time higher amount of cells was found in the ileal effluents of infant compared to adult. stx genes were over-expressed (up to25-fold) in infant conditions compared to the adult ones. This results show that differences in digestive physicochemicalparameters of the upper gastrointestinal tract may partially explain why infants are more susceptible to EHEC infection thanadults. And finally, Lpf seem to play a key role in the interactions of EHEC with murine Peyer’s patches and are needed for anactive translocation of the pathogen across M cells, and both in vitro (M cells culture) and in vivo (murine ileal loops).S. cerevisiae had not effect on EHEC survival in the colonic environment but (i) favorably influenced gut microbiotaactivity through beneficial modulation of short chain fatty acid production, (ii) leading to significantly decrease stx expressionand (iii) significantly reduced EHEC translocation through M cells and inhibited in vivo interactions of the pathogen withPeyer’s patches and the associated hemorrhagic lesions. Probiotic had donor-dependent effect on the gut microbiota strengthenthe hypothesis that host-associated factors such as microbiota could influence the clinical evolution of EHEC infection and theeffectiveness of a probiotic strategy.This work contributes to a better understanding of the behavior of EHEC in the human digestive environment andconfirms the interest of probiotic strategy in controlling EHEC infections. Further transcriptome studies are warranted for thepathogen in the human digestive environment, with or without probiotics for the better understanding of the pathophysiologyof EHEC and so on the mechanisms involved in the antagonistic effect of probiotics. Escherichia coli enterohémorragique Système de digestion in vitro Microbiote Probiotiques Anses iléales murines Long Polar Fimbriae Enterohemorrhagic Escherichia coli Digestive in vitro model Gut microbiota Probiotics Murine ileal loops Long Polar Fimbriae 616.9
9	Colonisation de la viande par Escherichia coli O157∶H7 : caractérisation moléculaire, cellulaire et tissulaire des interactions / Meat colonisation by Escherichia coli O157∶H7 : molecular, cellular and tissue characterisation of the interactions Chagnot, Caroline 02 April 2014 (has links) Escherichia coli O157:H7 est le sérotype le plus souvent incriminé lors de toxi-infection alimentaire par les E. coli entérohémorragiques (EHEC). Il peut être associé, dans les cas les plus graves, à des colites hémorragiques mortelles et au syndrome hémolytique et urémique (SHU), touchant essentiellement les jeunes enfants. Le vecteur alimentaire le plus courant lors de ces contaminations est le boeuf haché. L’étape primaire de la contamination bactérienne se situe lors de l'abattage où les bactéries peuvent être transférées de la peau à la carcasse. Une gaine conjonctive entoure les muscles, sa composition protéique, similaire à la matrice extracellulaire (ECM), pourrait jouer un rôle dans l'adhésion bactérienne. Dans un premier temps, l’étude de l'adhésion et de la colonisation des bactéries aux protéines majeures de l’ECM musculaire, a révélé une forte influence des conditions de croissances sur l’adhésion, l'adhésion étant maximale à 25°C et pH7, en particulier aux collagènes I et III. Chez les EHEC, diverses protéines de surfaces peuvent être potentiellement impliquées dans l’adhésion à l’ECM. Le rôle d'un autotransporteur, l'antigène 43 (Ag43), dans l'autoagrégation, l'adhésion et la formation de biofilm, a été établit chez E. coli O157:H7 EDL933. Par la suite, les interactions entre E. coli O157:H7 et la viande ont été étudiées sur deux muscles modèles de types métabolique et contractile opposés (Soleus oxidatif lent et EDL, glycolytique rapide), caractérisés par microspectroscopie de fluorescence UV couplée au rayonnement synchrotron. Les différents types de fibres musculaires ainsi que l’effet d’une anoxie prolongée simulant la maturation des viandes ont été discriminés par leurs réponses spectrales après une excitation à 275 nm. Un tropisme bactérien plus élevé pour le muscle soleus que pour le muscle EDL a été clairement observé. Bien qu'E. coli O157:H7 adhère de manière similaire aux différents types de fibres musculaires, l'adhésion des bactéries se fait essentiellement au niveau de l'ECM, mettant en évidence le rôle clé de l'ECM et du tissu conjonctif musculaire dans l’adhésion des E. coli O157:H7 à la viande. Ces travaux de recherche sur l’adhésion bactérienne aux muscles squelettiques aux niveaux moléculaires, cellulaires et tissulaires fournissent les premières connaissances sur la physiologie des EHEC lors de la contamination de la viande et constituent un pré-requis indispensable au développement de pratiques et de stratégies innovantes afin de réduire le risque de contamination des viandes. / Escherichia coli O157:H7 is the most prevalent serotype involved in foodborne infection by enterohemorrhagic E. coli (EHEC). It is associated with life-threatening hemorrhagic colitis and the hemolyticuremic syndrome (HUS), which essentially affect young children. The major food vector of EHEC contamination is ground beef. The primary bacterial contamination occurs during the slaughter, essentially at dehiding stage where bacteria can be transferred from hides to carcasses. The connective tissue surrounding the muscle, highly similar to extracellular matrix (ECM) could potentially be a support for bacterial adhesion. When investigating the adhesion and colonization to the main muscle fibrous ECM proteins, the great influence of growth conditions on subsequent bacterial attachment was shown. Maximal adhesion to ECM proteins occurred at 25°C and pH 7, especially to collagens I and III. In EHEC, various surface-exposed protein determinants can be expressed and potentially involved in ECM adhesion. Investigating the autoaggregation, bacterial adhesion and biofilm formation, the involvement of Antigen 43 (Ag43), an autotransporter protein, was demonstrated in E. coli O157:H7 EDL933. Then, the attachment of E. coli O157:H7 to the meat was determined on two different model muscles, with different contractile and metabolic characteristic (Soleus oxidative, slow and EDL glycolytic, fast), previously characterized by UV microspectroscopy coupled to synchrotron radiation fluorescence. The different of muscle fiber types and the effect of a prolonged anoxia simulating maturing meat were discriminated by their spectral responses after excitation at 275 nm. It clearly appeared that bacteria displayed differential tropism as function of the muscle types, higher for the Soleus than the EDL muscles. While E. coli O157:H7 adhered similarly to the different types of muscle fibers, bacterial adherence essentially occurred at the ECM, pinpointing the key role of connective tissue for E. coli O157:H7 adhesion to meat. This first comprehensive investigation of bacterial adhesion to skeletal muscles at molecular, cellular and tissue levels provides new insight in the physiology of the colonization of meat by EHEC and constitutes a prerequisite for the development of innovative practices and strategies to minimize the risk of meat contamination. Escherichia coli entérohémorragiques Contamination alimentaire Adhésion bactérienne ECM Muscle squelettique Types de fibres Viande Microspectroscopie de fluorescence UV Enterohemorrhagic Escherichia coli Food contamination Bacterial adhesion ECM Skeletal muscle Fiber types Meat UV microspectroscopy
10	A New Murine Model For Enterohemorrhagic Escherichia coli Infection Reveals That Actin Pedestal Formation Facilitates Mucosal Colonization and Lethal Disease: A Dissertation Mallick, Emily M. 28 March 2012 (has links) Enterohemorrhagic Escherichia coli (EHEC) colonizes the intestine and produces the phage-encoded Shiga toxin (Stx) which is absorbed systemically and can lead to hemolytic uremic syndrome (HUS) characterized by hemolytic anemia, thrombocytopenia, and renal failure. EHEC, and two related pathogens, Enteropathogenic E. coli (EPEC), and the murine pathogen, Citrobacter rodentium, are attaching and effacing (AE) pathogens that intimately adhere to enterocytes and form actin “pedestals” beneath bound bacteria. The actin pedestal, because it is a unique characteristic of AE pathogens, has been the subject of intense study for over 20 years. Investigations into the mechanism of pedestal formation have revealed that to generate AE lesions, EHEC injects the type III effector, Tir, into mammalian cells, which functions as a receptor for the bacterial adhesin intimin. Tir-intimin binding then triggers a signaling cascade leading to pedestal formation. In spite of these mechanistic insights, the role of intimin and pedestal formation in EHEC disease remains unclear, in part because of the paucity of murine models for EHEC infection. We found that the pathogenic significance of EHEC Stx, Tir, and intimin, as well as the actin assembly triggered by the interaction of the latter two factors, could be productively assessed during murine infection by recombinant C. rodentium expressing EHEC virulence factors. Here we show that EHEC intimin was able to promote colonization of C. rodentium in conventional mice. Additionally, previous in vitro data indicates that intimin may have also function in a Tir-independent manner, and we revealed this function using streptomycin pre-treated mice. Lastly, using a toxigenic C. rodentium strain, we assessed the function of pedestal formation mediated by Tir-intimin interaction and found that Tir-mediated actin polymerization promoted mucosal colonization and a systemic Stx-mediated disease that shares several key features with human HUS. Enterohemorrhagic Escherichia coli Escherichia coli Infections Hemolytic-Uremic Syndrome Shiga-Toxigenic Escherichia coli Shiga Toxin Citrobacter rodentium Adhesins Bacterial Escherichia coli Proteins Amino Acids, Peptides, and Proteins Animal Experimentation and Research Bacteria Bacterial Infections and Mycoses Biological Factors Enzymes and Coenzymes Hemic and Lymphatic Diseases Immunology and Infectious Disease Male Urogenital Diseases

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