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dc.contributor.authorPickard, Derek-
dc.contributor.authorWain, John-
dc.contributor.authorBaker, Stephen-
dc.contributor.authorLine, Alexandra-
dc.contributor.authorChohan, Sonia-
dc.contributor.authorFookes, Maria-
dc.contributor.authorBarron, Andrew-
dc.contributor.authorGaora, Peadar O-
dc.contributor.authorChabalgoity, José A.-
dc.contributor.authorThanky, Niren-
dc.contributor.authorScholes, Christoph-
dc.contributor.authorThomson, Nicholas-
dc.contributor.authorQuail, Michael-
dc.contributor.authorParkhill, Julian-
dc.contributor.authorDougan, Gordon-
dc.date.accessioned2026-06-15T17:49:45Z-
dc.date.available2026-06-15T17:49:45Z-
dc.date.issued2003-
dc.identifier.citationPICKARD, D., WAIN, J., BAKER, S., y otros. Composition, Acquisition, and Distribution of the Vi Exopolysaccharide-Encoding Salmonella enterica Pathogenicity Island SPI-7. J Bacteriol [en línea] 2003, 185(17). DOI: 10.1128/JB.185.17.5055–5065.2003es
dc.identifier.urihttps://hdl.handle.net/20.500.12008/55519-
dc.description.abstractVi capsular polysaccharide production is encoded by the viaB locus, which has a limited distribution in Salmonella enterica serovars. In S. enterica serovar Typhi, viaB is encoded on a 134-kb pathogenicity island known as SPI-7 that is located between partially duplicated tRNApheU sites. Functional and bioinformatic analysis suggests that SPI-7 has a mosaic structure and may have evolved as a consequence of several independent insertion events. Analysis of viaB-associated DNA in Vi-positive S. enterica serovar Paratyphi C and S. enterica serovar Dublin isolates revealed the presence of similar SPI-7 islands. In S. enterica serovars Paratyphi C and Dublin, the SopE bacteriophage and a 15-kb fragment adjacent to the intact tRNApheU site were absent. In S. enterica serovar Paratyphi C only, a region encoding a type IV pilus involved in the adherence of S. enterica serovar Typhi to host cells was missing. The remainder of the SPI-7 islands investigated exhibited over 99% DNA sequence identity in the three serovars. Of 30 other Salmonella serovars examined, 24 contained no insertions at the equivalent tRNApheU site, 2 had a 3.7-kb insertion, and 4 showed sequence variation at the tRNApheU-phoN junction, which was not analyzed further. Sequence analysis of the SPI-7 region from S. enterica serovar Typhi strain CT18 revealed significant synteny with clusters of genes from a variety of saprophytic bacteria and phytobacteria, including Pseudomonas aeruginosa and Xanthomonas axonopodis pv. citri. This analysis suggested that SPI-7 may be a mobile element, such as a conjugative transposon or an integrated plasmid remnant.es
dc.format.mimetypeapplication/pdfes
dc.language.isoenes
dc.relation.ispartofJ Bacteriol. 185(17), 2003es
dc.rightsLas obras depositadas en el Repositorio se rigen por la Ordenanza de los Derechos de la Propiedad Intelectual de la Universidad de la República.(Res. Nº 91 de C.D.C. de 8/III/1994 – D.O. 7/IV/1994) y por la Ordenanza del Repositorio Abierto de la Universidad de la República (Res. Nº 16 de C.D.C. de 07/10/2014)es
dc.subject.otherSALMONELLA ENTERICAes
dc.subject.otherSPI-7es
dc.titleComposition, Acquisition, and Distribution of the Vi Exopolysaccharide-Encoding Salmonella enterica Pathogenicity Island SPI-7es
dc.typeArtículoes
dc.contributor.filiacionPickard Derek, Imperial College (Reino Unido). Department of Biological Sciences. Centre for Molecular Microbiology and Infection-
dc.contributor.filiacionWain John, Imperial College (Reino Unido). Department of Infectious Diseases and Microbiology-
dc.contributor.filiacionBaker Stephen, Imperial College (Reino Unido). Department of Biological Sciences. Centre for Molecular Microbiology and Infection-
dc.contributor.filiacionLine Alexandra, Wellcome Trust Genome Campus (Reino Unido). The Sanger Institute-
dc.contributor.filiacionChohan Sonia, Wellcome Trust Genome Campus (Reino Unido). The Sanger Institute-
dc.contributor.filiacionFookes Maria, Wellcome Trust Genome Campus (Reino Unido). The Sanger Institute-
dc.contributor.filiacionBarron Andrew, Wellcome Trust Genome Campus (Reino Unido). The Sanger Institute-
dc.contributor.filiacionGaora Peadar O, Imperial College (Reino Unido). Department of Biological Sciences. Centre for Molecular Microbiology and Infection-
dc.contributor.filiacionChabalgoity José A., Universidad de la República (Uruguay). Facultad de Medicina. Instituto de Higiene. Unidad Académica Desarrollo Biotecnológico-
dc.contributor.filiacionThanky Niren, Imperial College (Reino Unido). Department of Biological Sciences. Centre for Molecular Microbiology and Infection-
dc.contributor.filiacionScholes Christoph, Imperial College (Reino Unido). Department of Biological Sciences. Centre for Molecular Microbiology and Infection-
dc.contributor.filiacionThomson Nicholas, Wellcome Trust Genome Campus (Reino Unido). The Sanger Institute-
dc.contributor.filiacionQuail Michael, Wellcome Trust Genome Campus (Reino Unido). The Sanger Institute-
dc.contributor.filiacionParkhill Julian, Wellcome Trust Genome Campus (Reino Unido). The Sanger Institute-
dc.contributor.filiacionDougan Gordon, Imperial College (Reino Unido). Department of Biological Sciences. Centre for Molecular Microbiology and Infection-
dc.rights.licenceLicencia Creative Commons Atribución (CC - By 4.0)es
dc.identifier.doi10.1128/JB.185.17.5055–5065.2003-
Aparece en las colecciones: Artículos - Instituto de Higiene

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