1989
DOI: 10.1128/jb.171.1.353-359.1989
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virG, a plasmid-coded virulence gene of Shigella flexneri: identification of the virG protein and determination of the complete coding sequence

Abstract: On the 230-kilobase-pair (kb) virulence plasmid of Shigella flexneri 2a strain YSH6000, at least seven separate genetic determinants have been identified. One of them, an approximately 4-kb region, virG, that is required for the Sereny reaction, was extensively studied to examine the role of the virG region. The phenotype of a VirG-mutant (M94) of YSH6000 in the cytoplasm of cultured MK cels was characterized by a kinetic study of the invading shigellae. The observed phenotype of M94 in the cytoplasm indicated… Show more

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Cited by 235 publications
(204 citation statements)
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“…Forty-five mutants that were invasive but were defective in plaque formation, indicating mutations affecting intracellular multiplication or spread to adjacent cells, were selected for further study. The DNA sequences adjacent to the TnphoA inserts were analysed in the mutants and among these were icsA (virG ), a gene previously shown to be required for plaque formation (Bernardini et al, 1989;Lett et al, 1989), and a number of genes associated with LPS synthesis (Table 1). The S. flexneri LPS O-antigen-synthesis genes identified in this screen included rfbA, -B, -C, -F, and -G. These genes are involved in different steps in synthesis of the O-antigen repeating unit and are encoded on the S. flexneri chromosome (Macpherson et al, 1994;Morona et al, 1994) (Fig.…”
Section: Isolation Of Strains With Chromosomal Lps-synthesis Gene Mutmentioning
confidence: 99%
“…Forty-five mutants that were invasive but were defective in plaque formation, indicating mutations affecting intracellular multiplication or spread to adjacent cells, were selected for further study. The DNA sequences adjacent to the TnphoA inserts were analysed in the mutants and among these were icsA (virG ), a gene previously shown to be required for plaque formation (Bernardini et al, 1989;Lett et al, 1989), and a number of genes associated with LPS synthesis (Table 1). The S. flexneri LPS O-antigen-synthesis genes identified in this screen included rfbA, -B, -C, -F, and -G. These genes are involved in different steps in synthesis of the O-antigen repeating unit and are encoded on the S. flexneri chromosome (Macpherson et al, 1994;Morona et al, 1994) (Fig.…”
Section: Isolation Of Strains With Chromosomal Lps-synthesis Gene Mutmentioning
confidence: 99%
“…VirG is a surface-exposed outer membrane protein of bacterium, composed of 1102 amino acids, which contains three distinctive domains: the Nterminal signal sequence (residues 1-52), the surfaceexposed 706-amino-acid a-domain (residues 53-758) and the membrane-embedded 344-amino-acid C-terminal b-core (residues 759-1102) (Lett et al, 1989;Goldberg et al, 1993;Suzuki et al, 1995). The N-terminal two-thirds of the VirG a-domain, which contains six glycine-rich repeats, is essential for mediating actin assembly of Shigella in host cells, as the a-domain is involved in interacting with host proteins such as vinculin and neural Wiskott-Aldrich syndrome protein (N-WASP) (Suzuki et al, 1996;Egile et al, 1999;Suzuki and Sasakawa, 2001).…”
Section: Introductionmentioning
confidence: 99%
“…The virulence plasmid-encoded protein product of the icsA (virG) gene is necessary and sufficient for actinbased motility (Makino et al, 1986;Bernardini et al, 1989;Lett et al, 1989;Goldberg and Theriot, 1995;Kocks et al, 1995). IcsA, a 120 kDa outer membrane protein, is located at a single pole on the surface of the bacterium, at the junction with the actin tail (Goldberg et al, 1993).…”
Section: Introductionmentioning
confidence: 99%