A genomewide mutagenesis screen identifies multiple genes contributing to Vi capsular expression in Salmonella enterica serovar typhi

Derek Pickard; Robert A Kingsley; Christine Hale; Keith Turner; Karthikeyan Sivaraman; Michael Wetter; Gemma C. Langridge; Gordon Dougan

doi:10.1128/JB.01632-12

A genomewide mutagenesis screen identifies multiple genes contributing to Vi capsular expression in Salmonella enterica serovar typhi

Derek Pickard, Robert A Kingsley, Christine Hale, Keith Turner, Karthikeyan Sivaraman, Michael Wetter, Gemma C. Langridge, Gordon Dougan

Research output: Contribution to journal › Article › Research › peer-review

25 Citations (Scopus)

Abstract

A transposon-based, genomewide mutagenesis screen exploiting the killing activity of a lytic ViII bacteriophage was used to identify Salmonella enterica serovar Typhi genes that contribute to Vi polysaccharide capsule expression. Genes enriched in the screen included those within the viaB locus (tviABCDE and vexABCDE) as well as oxyR, barA/sirA, and yrfF, which have not previously been associated with Vi expression. The role of these genes in Vi expression was confirmed by constructing defined null mutant derivatives of S. Typhi, and these were negative for Vi expression as determined by agglutination assays with Vi-specific sera or susceptibility to Vi-targeting bacteriophages. Transcriptome analysis confirmed a reduction in expression from the viaB locus in these S. Typhi mutant derivatives and defined regulatory networks associated with Vi expression.

Original language	English
Pages (from-to)	1320-1326
Number of pages	7
Journal	Journal of Bacteriology
Volume	195
Issue number	6
DOIs	https://doi.org/10.1128/JB.01632-12
Publication status	Published - Mar 2013
Externally published	Yes

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title = "A genomewide mutagenesis screen identifies multiple genes contributing to Vi capsular expression in Salmonella enterica serovar typhi",

abstract = "A transposon-based, genomewide mutagenesis screen exploiting the killing activity of a lytic ViII bacteriophage was used to identify Salmonella enterica serovar Typhi genes that contribute to Vi polysaccharide capsule expression. Genes enriched in the screen included those within the viaB locus (tviABCDE and vexABCDE) as well as oxyR, barA/sirA, and yrfF, which have not previously been associated with Vi expression. The role of these genes in Vi expression was confirmed by constructing defined null mutant derivatives of S. Typhi, and these were negative for Vi expression as determined by agglutination assays with Vi-specific sera or susceptibility to Vi-targeting bacteriophages. Transcriptome analysis confirmed a reduction in expression from the viaB locus in these S. Typhi mutant derivatives and defined regulatory networks associated with Vi expression.",

author = "Derek Pickard and Kingsley, \{Robert A\} and Christine Hale and Keith Turner and Karthikeyan Sivaraman and Michael Wetter and Langridge, \{Gemma C.\} and Gordon Dougan",

year = "2013",

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doi = "10.1128/JB.01632-12",

language = "English",

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T1 - A genomewide mutagenesis screen identifies multiple genes contributing to Vi capsular expression in Salmonella enterica serovar typhi

AU - Pickard, Derek

AU - Kingsley, Robert A

AU - Hale, Christine

AU - Turner, Keith

AU - Sivaraman, Karthikeyan

AU - Wetter, Michael

AU - Langridge, Gemma C.

AU - Dougan, Gordon

PY - 2013/3

Y1 - 2013/3

N2 - A transposon-based, genomewide mutagenesis screen exploiting the killing activity of a lytic ViII bacteriophage was used to identify Salmonella enterica serovar Typhi genes that contribute to Vi polysaccharide capsule expression. Genes enriched in the screen included those within the viaB locus (tviABCDE and vexABCDE) as well as oxyR, barA/sirA, and yrfF, which have not previously been associated with Vi expression. The role of these genes in Vi expression was confirmed by constructing defined null mutant derivatives of S. Typhi, and these were negative for Vi expression as determined by agglutination assays with Vi-specific sera or susceptibility to Vi-targeting bacteriophages. Transcriptome analysis confirmed a reduction in expression from the viaB locus in these S. Typhi mutant derivatives and defined regulatory networks associated with Vi expression.

AB - A transposon-based, genomewide mutagenesis screen exploiting the killing activity of a lytic ViII bacteriophage was used to identify Salmonella enterica serovar Typhi genes that contribute to Vi polysaccharide capsule expression. Genes enriched in the screen included those within the viaB locus (tviABCDE and vexABCDE) as well as oxyR, barA/sirA, and yrfF, which have not previously been associated with Vi expression. The role of these genes in Vi expression was confirmed by constructing defined null mutant derivatives of S. Typhi, and these were negative for Vi expression as determined by agglutination assays with Vi-specific sera or susceptibility to Vi-targeting bacteriophages. Transcriptome analysis confirmed a reduction in expression from the viaB locus in these S. Typhi mutant derivatives and defined regulatory networks associated with Vi expression.

UR - https://www.scopus.com/pages/publications/84874714760

U2 - 10.1128/JB.01632-12

DO - 10.1128/JB.01632-12

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SN - 0021-9193

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EP - 1326

JO - Journal of Bacteriology

JF - Journal of Bacteriology

IS - 6

ER -

A genomewide mutagenesis screen identifies multiple genes contributing to Vi capsular expression in Salmonella enterica serovar typhi

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