Global ETD Search

81	Rôle de Paa dans la pathogénicité des Escherichia coli attachants et effaçants (AEEC) Destable, Élodie January 2008 (has links) Mémoire numérisé par la Division de la gestion de documents et des archives de l'Université de Montréal. Escherichia coli entéropathogène Escherichia coli entérohémorragique Lésions attachantes et effaçantes Système de sécrétion de type III Paa Enteropathogenic Escherichia coli Enterohemorragic Escherichia coli Paa
82	Caractérisation moléculaire du système de sécrétion de type II de la bactérie phytopathogène Dickeya dadantii : études structurales et fonctionnelles sur l’interaction entre OutC et OutD / Molecular characterization of the type II secretion system of the phytopathogenic bacterium Dickeya dadantii : structural and functional studies of the interaction of OutC and OutD Wang, Xiaohui 10 February 2012 (has links) Le système de sécrétion de type II (T2SS) est largement exploité par les bactéries à Gram négatif pour sécréter divers facteurs de virulence depuis le périplasme vers le milieu extra-cellulaire. La bactérie phytopathogène Dickeya dadanti (ex. Erwinia chrysanthemi) utilise ce système, appelé Out, pour la sécrétion de pectinases responsable de la maladie de la pourriture molle chez de nombreuses plantes. Les deux composants essentiels du système Out, la protéine de membrane interne OutC et la sécrétine OutD, formant un pore dans la membrane externe, sont impliqués dans la spécificité de sécrétion. L'interaction entre OutC et OutD pourrait assurer l’intégrité structurelle et fonctionnelle du système de sécrétion en reliant les deux membranes. Nous avons entrepris une étude structure-fonction de ces deux composants afin d’identifier et caractériser leurs sites d’interaction et de mieux comprendre leurs rôles. Nous avons appliqué une approche intégrative impliquant une analyse in vivo par cystéine-scanning et pontage disulfure, une analyse in vitro par GST pull down et une analyse structurale d’OutC et OutD et de leurs interactions par RMN. Nos résultats indiquent la présence d'au moins trois sites d'interaction entre les régions périplasmiques d’OutC et d’OutD et suggèrent que ces interactions s’établissent par un mécanisme d’addition des brins β. Nous avons démontré qu’un site situé sur le domaine HR d’OutC pouvait interagir avec deux sites distincts d’OutD suggérant un mode d’interaction alternatif. La présence d’exoprotéines et/ou des composants de membrane interne du système OutE-L-M, modifie différemment l’affinité de ces trois sites d'interaction entre OutC et OutD. Nous proposons que ces interactions alternatives entre divers sites d’OutC et OutD pourraient refléter une succession d’étapes fonctionnelles lors du processus de sécrétion. Pour étudier le mécanisme d’adressage et d’assemblage de la sécrétine OutD dans la membrane externe, nous avons exploité les interactions entre OutD et deux composants auxiliaires du T2SS, la protéine de la membrane interne OutB et la lipoprotéine de la membrane externe OutS. Nous avons montré une interaction directe entre le domaine périplasmique d’OutB et le domaine N0 d’OutD. Une analyse structure-fonction du complexe OutS-OutD a révélé que la pilotine OutS interagit fortement avec 18 résidus à l’extrémité C-terminale de la sécrétine, entraînant la structuration sous forme hélicoïdale de cette région initialement non structurée. Ce travail nous permet de mieux comprendre le mécanisme d’assemblage et de fonctionnement du système de sécrétion de type II. / The type II secretion system (T2SS) is widely exploited by Gram-negative bacteria to secrete diverse virulence factors from the periplasm into the extra-cellular milieu. The phytopathogenic bacterium Dickeya dadanti (ex. Erwinia chrysanthemi) uses this system, named Out, to secrete several cell-wall degrading enzymes that cause soft-rot disease of many plants. The two core components of the Out system, the inner membrane protein OutC and the secretin OutD, which forms a secretion pore in the outer membrane, are involved in secretion specificity. The interaction between OutC and OutD could assure the structural and functional integrity of the secretion system by connecting the two membranes. To understand structure-function relationships between these two components and characterize their interaction sites, we applied an integrative approach involving in vivo cysteine scanning and disulfide cross-linking analysis, truncation analysis of OutC and OutD combined with in vitro GST pull-down, and structural analysis of these proteins and of their interactions by NMR. Our results indicate the presence of at least three interacting sites between the periplasmic regions of OutC and OutD and suggest a β-strand addition mechanism for these interactions. We demonstrated that one site of the HR domain of OutC can interact with two distinct sites of OutD suggesting an alternative mode of their interactions. The presence of exoproteins or/and the inner membrane components of the system OutE-L-M differently alters the affinity of the three OutC-OutD interacting sites. We suggest that successive interactions between these distinct regions of OutC and OutD may have functional importance in switching the secretion machinery between different functional states. To study the mechanism of the targeting and assembly of the secretin OutD into the outer membrane, we exploited the interactions between OutD and two auxiliary proteins, i.e., the inner membrane protein OutB and the outer membrane lipoprotein OutS. We showed a direct interaction between the periplasmic domain of OutB and the N0 domain of OutD. Structure-function analysis of OutS-OutD complex shows that the pilotin OutS binds tightly to 18 residues close to the C-terminus of the secretin subunit causing this unstructured region to become helical on forming the complex. This work allows us to better understand the assembly and function mechanism of the type II secretion system. Biosciences Microbiologie Métabolisme Caractérisation moléculaire Système de sécrétion de type II Secrétine Biosciences Microbiology Metabolism Molecular characterization Type II secretion system Secretin 579.307 2
83	Déterminants protéiques de la voie de sécrétion Sec impliqués dans la formation de biofilm chez Listeria monocytogenes / Protein determinants of the Sec secretion pathway involved in Listeria monocytogenes biofilm formation Renier, Sandra Anne Angèle 07 December 2012 (has links) Listeria monocytogenes est une bactérie pathogène impliquée dans la toxi-infection alimentaire à l’origine de la listeriose, une maladie peu fréquente mais avec un taux de mortalité de 25 % chez l’homme. Cette bactérie est capable de former un biofilm lui permettant de mieux résister aux stress environnementaux ainsi qu’aux traitements de décontamination. Une nouvelle stratégie d’analyse génomique a été développée et a permis de cibler des systèmes de sécrétion et des protéines potentiellement impliqués dans la formation de biofilm. L’inactivation de la voie SecA2 entraîne la formation d’un biofilm aérien et par conséquent fragile. Ce morphotype est capable de croître de façon sessile à 20°C sur du polystyrène alors que ce n’est pas le cas pour la souche sauvage. De nouvelles protéines sécrétées de façon SecA2 dépendante ont été identifiées par l’étude de l’exoprotéome du mutant ΔsecA2 en comparaison avec celui de la souche sauvage. Le rôle des lipoprotéines dans la formation de biofilm ainsi que leur maturation par les peptidases signal de type II, LspA et LspB, a également été abordé. La combinaison d'une analyse de l’expression des gènes codant les lipoprotéines au cours de la formation de biofilm avec l’analyse génomique basé sur le sécrétome a permis de cibler trois lipoprotéines, dont LpeA qui serait impliquée dans les phases tardives de formation de biofilm. Enfin, l’importance majeure de LspA dans la maturation des lipoprotéines, a été mise en évidence par l’étude de l’exoprotéome des doubles mutant ΔlgtΔlspA et ΔlgtΔlspB en comparaison avec celui de Δlgt. / Listeria monocytogenes is a foodborne pathogenic bacteria responsible for listeriosis, a rare but high mortality rate disease in humans (25 %). This bacterium can form biofilm allowing a better resistance to environmental stresses as well as decontamination treatments. A new strategy for genomic analysis was developed and allowed to target secretion systems and proteins potentially involved in biofilm formation. Inactivation of the SecA2 pathway leads to the formation of an aerial and fragile biofilm. This morphotype is able to grow in a sessile mode at 20 °C on polystyrene whereas this is not the case for the wild type strain. New proteins secreted in a SecA2 manner were identified by comparing the ΔsecA2 exoproteome to the one of the wild type. The role of lipoproteins in biofilm formation and their maturation by the signal peptidase II, LpsA and LspB, was also tackled. Combining expression analysis of genes encoding lipoproteins during biofilm formation with genomic analysis based on the secretome allowed targeting three lipoproteins, including LpeA, which appeared to be involved in the later stages of biofilm formation. Finally, the importance of LspA in the maturation of lipoproteins,was highlighted by comparing of the double mutant ΔlgtΔlspA and ΔlgtΔlspB exoproteomes to the one of Δlgt. Listeria monocytogenes Biofilm Système de sécrétion SecA2 MurA CwhA Lipoprotéines Peptidases signal Exoprotéome Listeria monocytogenes Biofilm Secretion system SecA2 MurA CwhA Lipoproteins Signal peptidases Exoproteome
84	La machinerie de sécrétion de type II Xcp de Pseudomonas aeruginosa : relations structure-fonction et interactome Douzi, Badreddine 28 October 2011 (has links) Les bactéries à Gram négatif sont entourées par une enveloppe cellulaire qui, contrairement aux bactéries à Gram positif, possèdent une organisation membranaire complexe composée d’une membrane interne appelée généralement membrane cytoplasmique, un espace périplasmique contenant une matrice de peptidoglycane et une membrane externe asymétrique constituée d’une monocouche de phospholipides surmontée d’une assise de lipopolysaccharide (LPS). Afin de franchir cette barrière, les bactéries à Gram négatif ont développé différentes voies de sécrétions spécifiques dédiées à l’export des protéines (effecteurs) du milieu intracellulaire vers le milieu extracellulaire. Jusqu'à présent, six systèmes de sécrétion ont été identifiés chez ces bactéries. Chez Pseudomonas aeruginosa, une bactérie pathogène opportuniste, le système de sécrétion de type II appelé aussi sécréton Xcp constitue l’un des facteurs principales de sa virulence. Le sécréton Xcp est un complexe macromoléculaire formé par 12 protéines, nommées XcpAO et XcpPC-XcpZM. Ce complexe macromoléculaire est organisé en trois sous-complexes : i) une plateforme d’assemblage ancrée dans la membrane interne formé par les protéines XcpRESFYLZM ii) un pore de sécrétion localisé dans la membrane externe formé par l’oligomérisation d’une protéine appelé la sécrétine XcpQD. Le pore de sécrétion est connecté à la plateforme de la membrane interne par une protéine appelée XcpPC iii) un pseudopilus périplasmique sous forme de fibre hélicoïdale qui est formé par la multimérisation d’une protéine appelée la pseudopiline majeure XcpTG. D’autres protéines appelées les pseudopilines mineures XcpUH-VI-WJ-XK intègrent le pseudopilus. La première partie du travail effectué au cours de cette thèse a eu pour but d’étudier et de comprendre par des approches structurales, biochimiques et biophysiques le mécanisme d’assemblage des pseudopilines en pseudopilus. La deuxième partie de ce travail a porté sur l’étude des réseaux d’interactions entre les substrats sécrétés et les composants de la machinerie Xcp. Durant cette thèse, nous avons ainsi i) identifier grâce à l’étude des interactions protéine-protéine l’existence d’un complexe quaternaire entre les pseudopilines mineures XcpUH-VI-WJ-XK localisées au sommet du pseudopilus ii) déterminer les structures de la pseudopiline majeure XcpTG par RMN et de la pseudopiline mineure XcpWJ par cristallographie aux rayons X iii) déterminer les différents éléments du sécréton qui interagissent avec les exoprotéines du sécréton. Ce réseau d’interaction nous a permis de proposer un modèle de fonctionnement du sécréton qui élucide le cheminement des exoprotéines dans le sécréton afin qu’elles soient exportées vers le milieu extracellulaire. / Gram-negative bacteria are characterized by a complex organization of their cell envelope composed by the inner membrane (IM) called cytoplasmic membrane, the periplasmic space containing a peptidoglycan layer and the outer membrane (OM) covered by the lipopolysaccharide matrix. Gram-negative bacteria have evolved several specialized machines called secretion systems to export their effectors from the intracellular medium to the extracellular milieu or to the host cells. Up to now, at least six secretion systems have been identified. In the opportunistic pathogen Pseudomonas aeruginosa, the type II secretion system called the Xcp secreton is the major pathway for the release of virulence factors. The Xcp secreton is a macromolecular complex composed by 12 proteins called XcpAO, XcpPC-XcpZM. This machinery is organized in 3 sub-complexes: i) the assembly platform localized in the IM implicating XcpRESFYLZM proteins ii) the OM pore composed by the oligomerization of the secretin XcpQD. The connection between the assembly platform and the secretin is performed by XcpPC anchored in the IM iii) a periplasmic pseudopilus consisting of the multimerization of the so-called major pseudopilin XcpTG. The pseudopilus is a helicoidally filament spanning the periplasmic area and pushing the substrate into the secretin pore. Four other proteins, the minor pseudopilins XcpUH-VI-WJ-XK, were found in the pseudopilus. In the present work we first focused on the study of the pseudopilus components by biochemical, biophysical and structural strategies to understand their assembly. Secondly, we investigate the protein interactome between periplasmic secreton component and secreted substrates. Thus, we revealed the presence of a quaternary complex composed by XcpUH-VI-WJ-XK located at the tip of the pseudopilus. To understand at atomic scale the regulation of the pseudopilus, we determined the structure of two components of the pseudopilus XcpTG by NMR and XcpWJ by X-ray crystallography. Using systematic protein-protein interaction studies between secreton components and purified exoproteins of Pseudomonas aeruginosa, we identified 5 proteins of the secreton able to interact with exoproteins. This interaction network allowed us to propose a model for the secretion process including the sequential steps followed by exoproteins inside the secreton to leave the cell envelop. Sécrétion Système de sécrétion de type II Pseudopilus Reconnaissance substrat-machinerie BIAcore Interaction protéine-protéine Secretion Type II secretion system Pseudopilus Substrate-machinery recognition BIAcore Protein-protein interaction
85	Characterization of structure, dynamics, function and interactions of components from the type IV secretion system of Xanthomonas citri by solution nuclear magnetic resonance / Caracterização da estrutura, dinâmica, interações e função de componentes do sistema de secreção tipo IV de Xanthomonas citri por ressonância magnética nuclear em solução Oliveira, Luciana Coutinho de 01 February 2016 (has links) Bacteria use specialized systems, called secretion systems, in order to translocate substrates to the environment or to other cells, or even to uptake molecules from the exterior environment. Six different secretion systems have been described in Gram-negative bacteria. The Type IV Secretion System (T4SS) is involved in translocation of virulence factors, bacterial conjugation, uptake and release of DNA, and in the secretion of antibacterial toxins. The T4SS channel corresponds to a toroidal upramolecular complex consisting of 14 repetitions of the VirB7-VirB9-VirB10 heterotrimer. This channel, also called \"core complex\", is divided in two layers, an outer layer consisting of the VirB7 lipoprotein in complex with the C-terminal domains of VirB9 (VirB9CT) and VirB10 (VirB10CT), and an inner layer composed by the N-terminal domains of VirB9 (VirB9NT) and VirB10 (VirB10NT). Xanthomonas citri pv. citri (Xac) is a gram-negative bacterium that infects citrus plants causing a disease called \"citrus canker\". Although not directly involved in causing the disease, the chromosomally encoded T4SS is responsible for the secretion of toxins, working as a bacterial killing machine (Souza et al., 2015). The three-dimensional structure of Xac\'s VirB7 obtained by Nuclear Magnetic Resonance (NMR) spectroscopy (PDB 2L4W) revealed that, unlike the canonical VirB7, Xac\'s VirB7 consists of a flexible N-terminal domain followed by a C-terminal globular domain. The flexible N-terminal tail is involved in interaction with VirB9CT. In this thesis, the NMR structure of the complex formed between VirB9CT and a peptide derived from the N-terminal tail of Xac-VirB7 (VirB7NT) was solved. This complex is stabilized by hydrophobic interactions involving the side chains of particular amino acid residues such as Phe30, Trp34 and Val37 in VirB7, and Arg250, Tyr167 and Tyr169 in VirB9. Mutations of such amino acids affect not only the stability of the VirB9:VirB7 complex in vitro, but also reduce the T4SS activity and impairs its assembly in vivo. Furthermore, the ability of forming VirB7:VirB7 oligomers is essential for a functional T4SS, although it is not required for assembling the complex. The structural propensity and flexibility of a fragment derived from the proline-rich region (PRR) of the N-terminal tail of VirB10 (VirB10NT - residues 85 to 182) were studied. Measurements of the {1H}-15N heteronuclear NOE showed that VirB10NT is highly flexible on a sub-nanosecond time scale. Analysis of chemical shifts and NOEs showed that the ensemble and time average conformation of VirB10NT consists of a short alpha helix between residues 151-163, and that this helix is involved in interactions with VirB9NT. These findings provide the first compelling evidence for the interaction between the N-terminal domains of VirB9 and VirB10, and for the existence of significant flexibility within Xacs T4SS. / Bactérias usam sistemas especializados, denominados sistemas de secreção, a fim de translocar substratos para o ambiente ou para outras células, ou até mesmo para capturar moléculas do meio externo. Seis diferentes sistemas de secreção foram descritos em bactérias gram-negativas. O Sistema de Secreção do Tipo IV (T4SS) está envolvido na translocação de fatores de virulência, conjugação bacteriana, absorção e liberação de DNA, e secreção de toxinas antibacterianas. O canal do T4SS (core complex) corresponde a um complexo formado por 14 repetições do heterotrimero VirB7-VirB9-VirB10. A camada externa deste canal é constituída por VirB7 em complexo com os domínios C-terminal de VirB9 (VirB9CT) e VirB10 (VirB10CT). Os domínios N-terminal de VirB9 (VirB9NT) e VirB10 (VirB10NT) formam a camada interna do core complex. Xanthomonas citri pv. citri (Xac) é uma bactéria gram-negativa que infecta plantas cítricas causando uma doença chamada \"cancro cítrico\". Embora não esteja diretamente envolvido na infecção, o T4SS cromossomal secreta toxinas capazes de matar outras bactérias gram-negativas. VirB7 de Xac possui uma cauda N-terminal flexível e um domínio globular C-terminal ausente em outras proteínas VirB7. VirB7 interage com VirB9CT através de sua cauda N-terminal. Nesta tese, a estrutura de RMN do complexo formado por VirB9CT e um peptídeo derivado do segmento N-terminal de VirB7 foi resolvida. O complexo é estabilizado, principalmente, por interações hidrofóbicas envolvendo as cadeias laterais de determinados resíduos de aminoácidos, particularmente a Phe30, o Trp34 e a Val37 em VirB7 e a Arg250, a Tyr167 e a Tyr169 em VirB9. A substituição de alguns destes aminoácidos por alanina afeta não só a constante de dissociação do complexo in vitro, como também a atividade e a montagem do T4SS in vivo. Além disso, resíduos específicos envolvidos em oligomerização de VirB7 são essenciais para a manutenção de um T4SS funcional, embora não sejam essenciais para a montagem do sistema. Estudos estruturais, de dinâmica e de interações de um fragmento derivado da região rica em prolinas (proline-rich region - PRR) contida no N-terminal de VirB10 (VirB10NT - resíduos 85-182) também foram realizados. Medidas de {1H}-15N NOE heteronuclear mostraram que VirB10NT é altamente flexível. Análises de deslocamentos químicos e NOEs mostrou que VirB10NT forma uma hélice curta entre os resíduos 151-163. Ensaios de interação por RMN indicaram que esta hélice está envolvida em interações com VirB9NT. Estes resultados são a primeira evidência convincente para a especificidade de interação entre os domínios N-terminal de VirB9 e VirB10. Estes dados apontam também para a existência de flexibilidade dentro do T4SS de Xac. Biologia estrutural Nuclear magnetic resonance Ressonância magnética nuclear Sistema de secreção do tipo IV Structural biology Type IV secretion system Xanthomonas citri Xanthomonas citri
86	Untersuchungen zum Aufbau, zur Funktion und zur Verbreitung von genomischen Inseln in der Gattung Legionella Lautner, Monika 25 February 2013 (has links) Der Austausch von genetischem Material über horizontalen Gentransfer, stellt einen wichtigen Mechanismus in der bakteriellen Evolution dar. Legionella pneumophila Stämme codieren für verschiedene Typ IV Sekretionssysteme (T4SS) und integrative konjugative Elemente, die zur genomischen Variabilität der intrazellulären Erreger beitragen. L. pneumophila Corby codiert auf der genomischen Insel Trb-1 für ein funktionelles Konjugations- und T4ASS. Trb-1 ist innerhalb des tRNAPro Gens integriert und kann in einer chromosomalen oder zirkulären episomalen Form existieren. Zusätzlich zu den trb/tra Genen sind auf der Insel eine Integrase (int-1) und die Gene lvrRABC der Legionella vir Region (lvr) lokalisiert. Durch die Deletion von int-1 konnte gezeigt werden, dass die Exzision von Trb-1 unter Beteiligung der Integrase erfolgt. Zudem wurde in dieser Arbeit zum ersten Mal demonstriert, dass die lvr-Region, vor allem der putative Phagen-Repressor LvrR an der Regulation der Exzision von Trb-1 beteiligt ist. Die Konjugation von Trb-1 in L. oakridgensis, hatte keinen Effekt auf die in vivo Fitness der Transkonjuganten in humanen Makrophagen. Die genomischen Inseln LpcGI-1 und LpcGI-2 codieren für ein neues putatives GI-T4SS. Für LpcGI-2 konnte erstmals gezeigt werden, dass das T4SS funktionell ist und die Konjugation der genomischen Insel in einen anderen L. pneumophila Stamm vermitteln kann. LpcGI-2 kann anschließend ortsspezifisch in das Genom der Transkonjuganten integriert werden. LpcGI-1 und LpcGI-2 werden vom tRNAThr bzw. tRNAMet Gen flankiert und können in verschiedenen chromosomalen und zirkulären, episomalen Formen existieren. Die Exzision von LpcGI-2 erfolgt ähnlich zu Trb-1, in Abhängigkeit einer ortsspezifischen Integrase. Im Genom von Lp Corby wurden zwei weitere genomische Inseln (LpcGI-Asn und LpcGI-Phe) identifiziert. In silico Analysen zeigten zudem, dass genomische Inseln mit einer Ähnlichkeit zu Trb-1, LpcGI-2 bzw. LpcGI-1 im Genus Legionella verbreitet sind. / Exchange of genetic information by horizontal gene transfer is an important mechanism for the evolution of bacterial genomes. Legionella pneumophila strains encode different type IV secretion systems and integrative conjugative elements contribute to the variability of the intracellular pathogen. The genomic island Trb-1 of L. pneumophila Corby encodes a functional conjugation and T4ASS. Trb-1 is integrated within the tRNAPro gene and can exist in a chromosomal or an episomal circular form. In addition to the trb/tra genes, a site-specific integrase (int-1) and a Legionella vir region (lvrRABC) are also localized on the genomic island. By deleting the int-1 gene, it could be demonstrated that the excision and of Trb-1 is integrase dependent. Furthermore, in this work it was shown for the first time that the lvr region and especially the putative phage repressor LvrR, is involved in the regulation of Trb-1 excision. Conjugation of Trb-1 in L. oakridgensis does not influence the in vivo fitness of the transconjugants in human macrophages. The genomic islands LpcGI-1 and LpcGI-2 encode a new putative T4SS. For the first time it could be demonstrated, that the T4SS localized on LpcGI-2 is functional. Although LpcGI-2 could be mobilized and transferred via conjugation to another L. pneumophila strain, followed by the site-specific integration into the genome of the transconjugants. LpcGI-1 and LpcGI-2 are flanked by the tRNAThr or tRNAMet gene respectively. Both islands can exist in different chromosomal and episomal forms. The excision of LpcGI-2 occurs similar to Trb-1 in an integrase dependent manner. Two additional genomic islands (LpcGI-Asn and LpcGI-Phe) could be identified in the genome of Lp Corby. Moreover, data of the in silico analysis demonstrated, that genomic islands similar to Trb-1, LpcGI-2 and LpcGI-1 are distributed within the genus Legionella. Legionella Typ IV Sekretionssystem Konjugation genomische Insel Integrase Legionella type IV secretion system conjugation genomic island integrase 570 Biowissenschaften, Biologie 32 Biologie XD 4987 ddc:570
87	Desenvolvimento de um banco de dados para classificação e análise de sistemas de secreção do tipo IV bacteriano / Development of a database for classification and analysis of type IV secretion systems Santos Netto, Diogo dos 31 October 2008 (has links) Made available in DSpace on 2015-03-04T18:51:16Z (GMT). No. of bitstreams: 1 Anexos-Final.pdf: 7146890 bytes, checksum: bb4f151b856a0b67e03a2261753fccfe (MD5) Previous issue date: 2008-10-31 / Coordenacao de Aperfeicoamento de Pessoal de Nivel Superior / The type IV secretion system can be classified as a large family of macromolecule transporters divided in three recognized sub-families involved in different bacterial functions. The major sub-family of T4SS is the conjugation system, which allows transfer of genetic material as a nucleoprotein via cell contact among bacteria. Analogously to bacterial conjugation, the T4SS can transfer genetic material from bacteria to eukaryotic cells; such is the case of T-DNA transfer of Agrobacterium tumefaciens to host plant cells. The system of effector proteins transport constitutes the second sub-family, being indispensable for infection processes of several mammalian and plants pathogens. The third sub-family corresponds to the DNA uptake/release system involved in genetic transformation competence, independently of cell contact, as it was described to the systems VirB/D4 from Campylobacter jejuni and ComB form Helicobacter pylori. Several essential features of T4SS are well known, but the knowledge in support of an uncomplicated classification or proper protein annotation of system subunits remains confusing, which in same cases can avoid making inferences about evolution of the system in bacterial species. The purpose of this work was to organize, classify and integrate the knowledge about T4SS through building a database devoted to this bacterial secretion system. The T4SS database was created using the SGBD MySQL and Perl programming language and with a web interface (HTML/CGI) that gives access to the database. Currently, this database hold genomic data from 43 bacteria and 10 plasmids acquired from the GenBank NCBI, these organisms comprise groups from Actionobacteria to Gram-negative Proteobacteria including symbiotic and pathogenic bacteria. By applying Bidirectional Best-Hits method was possible to get a core set of 75 clusters with 974 proteins involved in the T4SS. Also, during this procedure BlastP, Muscle e ClustalW algorithms were applied. The database was manually annotated supported by cross references built-in the T4SS annotation pages, such as the UniProtKB/Swiss-Prot, COG, InterPro and TCDB as well as by the methods for signal peptide and transmembrane regions prediction. All T4SS protein records scattered into 75 ortholog clusters were organized into five different classes of type IV secretion system proteins: (i) Type IVA Mpf/T4CP; (ii) Type IVA Dtr; (iii) F-type plasmid; (iv) IncP-1-type plasmid; (v) Type IVB Icm/Dot. All 974 proteins were annotated into 68 well-known families, which can be involved in conjugation, effector translocator, DNA uptake/release or even can be bifunctional proteins. Also, by using the Maximum Likelihood method were built 70 unrooted phylogenetic trees that represents just 70 clusters instead of 75, this is due to five clusters had only two protein sequences, five unrooted phylogenetic trees were built for each group of first hierarchical classification, one unrooted phylogenetic trees including proteins from archetype systems of all groups, one unrooted phylogenetic trees from 16S sequence of each organism and one rooted tree including a sequence from a Gram-positive bacteria as an external group. The phylogenetic analyses show that some proteins of T4SS are more divergent than others, which indicate that for a particular function few sequence mutations were needed, but other proteins required many sequence mutations to get another functions. Thus, these results proved that proteins belong to the same cluster show different functions: conjugation, DNA uptake/release or effector translocator. Consequently, it was possible verify that similar functions were grouped together within phylogenetic tree, which allowed to annotate a probable function of some uncharacterized proteins, that is possibly due to the sequence similarity may reveal a similar evolution to get the same function. Thus, the phylogenetic trees allowed confirming the protein annotation as well as inferring whether uncharacterized proteins would encompass a known function. The T4SS database will be an open access, given to the users searching and submission sequence tools, which will permit to get insights about classification and phylogeny of T4SS sequence of interest. T4SS Database is accessible at the URL http://www.t4ss.lncc.br. / O T4SS pode ser classificado como uma família de transportadores de macromoléculas envolvidos em diferentes funções bacterianas. A maior subfamília do T4SS é a do sistema de conjugação, o qual permite a transferência de material genético entre bactérias. Analogamente à conjugação, o sistema pode transferir material genético entre bactérias e eucariotos, tal como a transferência de T-DNA de Agrobacterium tumefaciens. O sistema de transporte de proteínas efetoras constitui uma segunda subfamília do T4SS, sendo indispensável nos processos de infecção de vários patógenos de mamíferos e plantas. A última subfamília corresponde ao sistema DNA-uptake/release" que funciona independente de contato com uma célula alvo, representado pelos sistemas VirB/D4 de Campylobacter jejuni e ComB de Helicobacter pylori. Muitas características básicas do T4SS são bem conhecidas, entretanto o conhecimento para a classificação simples e intuitiva ou a anotação apropriada das proteínas ainda não está claro, impedindo em alguns casos estabelecer correlações evolutivas deste sistema em bactérias. O objetivo deste trabalho foi o de organizar, classificar e integrar o conhecimento do T4SS através da construção de um banco de dados especializado para este sistema secretório bacteriano. O banco de dados T4SS foi criado utilizando o SGBD MySQL e a linguagem de programação Perl e com uma interface web (HTML/CGI) que fornece acesso ao banco. Este banco consta atualmente com 43 genomas bacterianos e 10 plasmídeos obtidos do GenBank NCBI, estes organismos vão desde Actinobactérias até Proteobactérias Gram-negativas, incluindo simbiontes e patogênicos. Foi utilizada a metodologia do Bidirectional Best-Hits", com a qual foi possível obter um conjunto mínimo de 75 clusters" com 974 proteínas envolvidas no T4SS. Também, durante este procedimento foram utilizados os algoritmos BlastP, Muscle e ClustalW. O banco foi anotado manualmente utilizando referências cruzadas incluídas nas páginas de anotação do T4SS, tais como UniProtKB/Swiss-Prot, COG, InterPro e TCDB e métodos para predição de regiões de peptídeos sinal e transmembrana. As análises do banco T4SS permitiram criar uma classificação hierárquica e funcional para as proteínas do T4SS, consistindo em cinco grupos: (i) Type IVA Mpf/T4CP; (ii) Type IVA Dtr; (iii) F-type plasmid; (iv) IncP-1-type plasmid; (v) Type IVB Icm/Dot). As 974 proteínas foram anotadas em 68 famílias conhecidas, as quais podem estar envolvidas em conjugação, transferência de T-DNA, transferência de proteínas efetoras, DNA-uptake/release" ou bem serem proteínas bifuncionais. Também, através do método de máxima verossimilhança foram geradas 70 árvores filogenéticas não enraizadas (NR) representando apenas 70 clusters, já que cinco clusters apresentaram apenas duas seqüências de proteínas, cinco árvores filogenéticas NR foram criadas para cada grupo da primeira categoria hierárquica, uma árvore NR com representantes de todos os grupos, uma árvore NR gerada a partir das seqüências 16S de cada organismo e uma árvore de um cluster incluindo uma seqüência de bactéria Gram-positiva como grupo externo. As análises filogenéticas mostram que determinadas proteínas do sistema são mais divergentes que outras, indicando que para uma determinada função poucas mutações de seqüências foram necessárias, já outras proteínas precisaram de maiores mutações para adquirir outras funções. Por isso, verifica-se que proteínas de um mesmo cluster apresentam diferentes funções: conjugação, DNA-uptake/release", traslocadores de proteínas efetoras. Conseqüentemente, foi possível verificar que funções semelhantes se agruparam juntas nas árvores filogenéticas, permitindo anotar uma função provável das proteínas ainda não caracterizadas ( unknown"), isto possivelmente devido a que em virtude de sua semelhança de seqüências, possivelmente evoluíram para realizar a mesma função. Assim, as arvores possuíram a finalidade de confirmar a anotação e contribuíram permitindo inferir se os unknown" ou probable" podem ser de uma determinada classificação funcional. O banco T4SS será de uso público, oferecendo ao usuário ferramentas de buscas e submissão de seqüências, as quais permitirão inferir respostas sobre a classificação e filogenia da seqüência T4SS de interesse. O banco de dados T4SS pode ser acessado na URL: http://www.t4ss.lncc.br. Bioinformática Genômica Bioinformatics Genomics Database
88	Estudos estruturais e de interações proteína-proteína envolvendo componentes de um sistema de secreção do tipo IV de Xanthomonas axonopodis pv. citri / Structural and protein-protein interaction studies of type IV secretion system components from Xanthomonas axonopodis pv. citri Souza, Diorge Paulo de 25 May 2010 (has links) Xanthomonas axonopodis pv. citri (Xac) é o causador do cancro de plantas cítricas. Entre os potenciais fatores de virulência codificados por Xac, está o Sistema de Secreção do Tipo IV (T4SS), um grande complexo multiprotéico que atravessa o periplasma e as membranas interna e externa de bactérias Gram-negativas. O T4SS está envolvido com secreção de proteínas e/ou DNA para o meio extracelular ou diretamente no interior da célula do hospedeiro. Este Sistema requer tipicamente 12 proteínas para realizar suas funções: VirB1-VirB11 e VirD4. O T4SS codificado pelo cromossomo de Xac está aparentemente incompleto, devido a não codificar nenhuma proteína com similaridade de seqüência a VirB7. Os objetivos deste trabalho são estudar a estrutura, função e interações das proteínas do T4SS de Xanthomonas. Foram clonados 23 genes que codificam proteínas ou domínios relacionados ao T4SS, e os polipeptídeos foram produzidos de forma recombinante em E. coli. Treze deles foram purificados e submetidos a estudos estruturais, espectroscópicos e de interações proteína-proteína. A estrutura em solução de Xac262224-139 foi resolvida, apresentando uma região N-terminal desenovelada de aproximadamente 30 resíduos e um domínio globular. Este polipeptídeo oligomeriza em troca química rápida na escala de tempo de RMN e o seu N-terminal desenovelado reconhece o domínio C-terminal de VirB9 (VirB9154-255) em troca lenta. Análise de RMN demonstrou que VirB9154-255 possui uma estrutura flexível em solução, sofrendo uma marcante mudança conformacional na presença de Xac262224-139. Ambas proteínas se tornam rígidas após a interação. Xac2622 é o equivalente a VirB7 em Xanthomonas, baseado na localização do seu gene no lócus do T4SS, localização subcelular predita do polipeptídeo codificado e sua interação com VirB9. Porém, diferente de outras proteínas da família VirB7, Xac2622 possui um domínio globular adicional, com topologia e estrutura similares a domínios presentes apenas em proteínas associadas à membrana externa de bactérias Gram-negativas. Nocaute do gene xac2622, contudo, não afetou a virulência de Xac na infecção de plantas de laranja pêra. O domínio enovelado de Xac2622 foi cristalizado, e os cristais obtidos difrataram até uma resolução de 1,0 Å, pertencendo ao grupo espacial C2221. O modelo preliminar possui Rfactor de 0,121 e Rfree de 0,147. Foram obtidos cristais de outras 3 proteínas relacionadas ao T4SS de Xac, porém somente um deles difratou em alta resolução (2,0 Å, pertencendo ao grupo espacial C2). O potencial sinal de secreção pelo T4SS de Xanthomonas é um domínio C-terminal conservado de aproximadamente 115 resíduos, encontrado nos substratos putativos do T4SS. Caracterizamos um destes domínios, presente na proteína Xac2609, e ele é intrinsicamente desestruturado. Essa observação pode ter implicações funcionais, visto que os substratos são desenovelados antes de sua passagem pelo canal de secreção do T4SS / Xanthomonas axonopodis pv. citri (Xac) is a gram-negative bacterial phytopathogen that infects citrus. One possible virulence determinant is a chromosomally encoded Type IV Secretion System (T4SS), a multiprotein complex that spans the bacterial periplasm and both inner and outer membranes. The T4SS is used by some bacteria to secrete proteins and/or DNA to the extracellular milieu or the host interior. The model T4SS from Agrobacterium tumefaciens is made up of twelve structural proteins: VirB1-VirB11 and VirD4. The Xanthomonas T4SS is apparently incomplete because of the lack of a polypeptide with sequence similarity to VirB7. The aim of this project is the study of structure-function relationships in the Xanthomonas T4SS. Twenty-three T4SS protein-coding genes, including full-length proteins or domains, were cloned and the proteins were produced in different E. coli strains. Thirteen polypeptides were purified and some of them were submitted to structural, spectroscopic and protein-protein interaction studies. We used NMR to solve the solution structure of Xac262224-139 which consists of an unfolded N-terminal segment of ~30 residues followed by a globular domain. Xac262224-139 oligomerizes in fast exchange at the NMR time scale and interacts via its unfolded N-terminus with the VirB9 C-terminus (VirB9154-255) in slow exchange. NMR analysis showed that VirB9154-255 has a flexible structure in solution. However, this polypeptide undergoes a significant conformational modification in the presence of Xac2622,24-139 and both proteins become rigid upon interaction. Xac2622 is the Xanthomonas VirB7, based on the chromosomal localization of its gene, predicted subcellular localization and protein interaction analysis. But surprisingly, unlike other VirB7 proteins, Xac2622 has an extra C-terminal folded domain whose topology and structure are strikingly similar to that of periplasmic domains found in outer membrane proteins of many bacterial Secretion Systems. Knockout of the xac2622 gene, however, does not affect the Xac virulence in orange leaf infection assays. The Xac2622 folded domain was also crystallized, and these crystals diffracted up to 1.0 Å resolution and belong to the space group C2221. The preliminary refined model has Rfactor of 0.121 and Rfree of 0.147. Crystals of three other T4SS proteins have been obtained, but only one of them diffracted to high resolution (2.0 Å; space group C2). Xac2610 is a hypothetical protein whose gene is located in the T4SS locus, and its interactions were studied with VirB9, VirB11 and Xac2609, a putative T4SS substrate. The potential T4SS secretion signal is a conserved, approximately 115 residues, C-terminal domain found in the putative substrates of the Xanthomonas T4SS. This sequence mediates interactions with VirD4. We have characterized this domain from one substrate and it is mainly unfolded. This observation may have functional implications, as the substrates are unfolded before their secretion through the T4SS channel Biologia estrutural Cristalografia e difração de raios-X Nuclear magnetic resonance Ressonância magnética nuclear Sistema de secreção do tipo IV Structural biology Type IV secretion system X-ray crystallography Xanthomonas Xanthomonas
89	Déterminants génétiques et protéiques impliqués dans les processus d'adhésion de la bactérie commensale humaine Streptococcus salivarius / Genetic and protein determinants involved in adhesive processes of human commensal bacterium Streptococcus salivarius Couvigny, Benoît 09 December 2014 (has links) Afin de caractériser les mécanismes moléculaires sous-jacents au processus d’adhésion des bactéries commensales, nous avons utilisé Streptococcus salivarius comme modèle. Streptococcus salivarius est une bactérie pionière dans la colonisation des surfaces orales chez le nouveau né, et devient par la suite un composant majoritaire du microbiote oral de l'adulte avec un rôle écologique majeur. Nous avons développé une méthode pour identifier, par des tests de criblage phénotypique, les gènes impliqués dans l’adhésion de S. salivarius aux surfaces bactériennes ou de l’hôte. Notre approche a permis d’identifier un ensemble de gènes codant pour des protéines de surfaces, des glycosyltransférases, des transporteurs qui sont impliqués dans les phénomènes d’auto-agréation et / ou de co-agrégation avec d’autres espèces et / ou l’adhésion aux protéines de l’hôte.En particulier, nous avons montré que le système SecA2Y2, qui comprend des gènes codant pour des protéines dédiées à la glycosylation et l'export de protéines de surface riche en sérine (SRRPs), participe aux processus d’agrégation, de formation de biofilms, à l'adhésion in vitro aux protéines de l’hôte et in vivo à la colonisation du tractus digestif de souris. Alors que toutes les bactéries contenant un système similaire possèdent un substrat unique au système, une SRRP, le locus génétique secA2Y2 comprend trois SRRPs qui présentent des rôles complémentaires dans les phénotypes précédement cités. SrpB est spécifiquement impliquée dans la liaison aux cellules epitheliales, tandis que SrpC participe à l’adhésion aux protéines de la matrice extracellulaire et le mucus. De manière atypique, nous avons démontré que le processus de maturation des SRRPs est supporté par glycosyltransférases extra-cluster. Cette étude est le premier rapport indiquant la présence dans une bactérie de trois SRRPs, qui présentent des rôles complémentaires dans l'interaction bactéries-hôte. Bien que le système SecA2Y2 soit principalement associé à la virulence des bactéries pathogènes, il semble être clairement impliqué dans les caractères de commensalité de S. salivarius, tels que la colonisation de ses niches écologiques orales et intestinales. Ce travail offre de nouvelles perspectives sur les mécanismes de colonisation des bactéries commensales. / To characterize molecular mechanisms underlying adhesion of commensal bacteria, we used Streptococcus salivarius (SSAL) as a model. SSAL is among the most important pioneer colonizers of neonatal oral mucosal surfaces, and later becomes a predominant component of the human adult oral microbiota with pre-eminent ecological role. We developed a method to identified, through phenotypic screening assays, genes involved in SSAL adhesion to host or bacterial surfaces. In particular, we showed that the SecA2Y2 system, which comprises genes devoted to glycosylation and export of surface Serine Rich Repeat Proteins (SRRPs), participates to bacterial aggregation, biofilm formation, in vitro adhesion and colonization of mice. While all bacteria containing a similar system possess only one SRRP, the SSAL secA2Y2 locus comprises three SRRPs with complementary role in line with the previous phenotypes. Interestingly, SrpB is specifically involved in the binding to epithelial cells, while SrpC to the extracellular matrix and mucus proteins. We showed that these interactions require glycosylation of both bacterial SRPs and host surfaces. Surprisingly, we demonstrated that this essential process is shared by glycosyltransferases located in other genomic regions. This work is the first report showing the presence in a bacterium of three SRPs, which display complementary roles in bacterial-host interaction. While the SecA2Y2 system is mostly associated to virulence in pathogenic bacteria, it appears to be involved in the expression of commensal traits in SSAL, such as its colonization and its resilience to oral and intestinal niches. This work may offer new insights into the mechanisms of niche establishment (host, microbial communities) of commensal bacteria. Streptococcus salivarius Adhésion Agrégation Système de secretion accessoire Fibrils Serin-rich-repeat protein Streptococcus salivarius Adhesion Aggregation Saccessory secretion system Fibrils Serin-rich-repeat protein
90	Type III Secretion Mediated Translocation of Effector Exoenzymes by Pseudomonas aeruginosa / Injektion av gifter via typ III sekretionssystemet hos bakterien Pseudomonas aeruginosa Sundin, Charlotta January 2003 (has links) No description available. Cell and molecular biology Pseudomonas aeruginosa type III secretion system ExoS ExoT PcrV PcrG PopB PopD PopN type IV pili Cell- och molekylärbiologi Cell and molecular biology Cell- och molekylärbiologi

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