Cloning, characterization and sequencing of an accessory gene regulator (agr) in Staphylococcus aureus

H. L. Peng; R. P. Novick; B. Kreiswirth; J. Kornblum; P. Schlievert

doi:10.1128/jb.170.9.4365-4372.1988

Cloning, characterization and sequencing of an accessory gene regulator (agr) in Staphylococcus aureus

H. L. Peng, R. P. Novick, B. Kreiswirth, J. Kornblum, P. Schlievert

Public Health Research Institute, New York

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

438 Scopus citations

Abstract

We have previously identified a gene in Staphylococcus aureus, agr, whose activity is required for high-level post-exponential-phase expression of a series of secreted proteins. In this paper, we describe the cloning of this gene in Escherichia coli by using an inserted transposon (Tn551) as a cloning probe. The cloned gene, consisting of a 241-codon open reading frame containing the site of the transposon insertion, was recloned to an S. aureus vector, pSK265, and shown to be functional in S. aureus. Activity was evaluated by determinations of α-hemolysin, β-hemolysin, and toxic shock syndrome toxin-1 production in early-stationary-phase cultures. The cloned gene showed considerable variation with respect to different exoproteins and different host strains compared with the chromosomal agr determinant; this variation could not be attributed to the higher copy number of the cloned gene and probably reflects inapparent subtleties of the regulatory system.

Original language	English
Pages (from-to)	4365-4372
Number of pages	8
Journal	Journal of Bacteriology
Volume	170
Issue number	9
DOIs	https://doi.org/10.1128/jb.170.9.4365-4372.1988
State	Published - 1988
Externally published	Yes

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10.1128/jb.170.9.4365-4372.1988

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title = "Cloning, characterization and sequencing of an accessory gene regulator (agr) in Staphylococcus aureus",

abstract = "We have previously identified a gene in Staphylococcus aureus, agr, whose activity is required for high-level post-exponential-phase expression of a series of secreted proteins. In this paper, we describe the cloning of this gene in Escherichia coli by using an inserted transposon (Tn551) as a cloning probe. The cloned gene, consisting of a 241-codon open reading frame containing the site of the transposon insertion, was recloned to an S. aureus vector, pSK265, and shown to be functional in S. aureus. Activity was evaluated by determinations of α-hemolysin, β-hemolysin, and toxic shock syndrome toxin-1 production in early-stationary-phase cultures. The cloned gene showed considerable variation with respect to different exoproteins and different host strains compared with the chromosomal agr determinant; this variation could not be attributed to the higher copy number of the cloned gene and probably reflects inapparent subtleties of the regulatory system.",

author = "Peng, {H. L.} and Novick, {R. P.} and B. Kreiswirth and J. Kornblum and P. Schlievert",

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AU - Peng, H. L.

AU - Novick, R. P.

AU - Kreiswirth, B.

AU - Kornblum, J.

AU - Schlievert, P.

PY - 1988

Y1 - 1988

N2 - We have previously identified a gene in Staphylococcus aureus, agr, whose activity is required for high-level post-exponential-phase expression of a series of secreted proteins. In this paper, we describe the cloning of this gene in Escherichia coli by using an inserted transposon (Tn551) as a cloning probe. The cloned gene, consisting of a 241-codon open reading frame containing the site of the transposon insertion, was recloned to an S. aureus vector, pSK265, and shown to be functional in S. aureus. Activity was evaluated by determinations of α-hemolysin, β-hemolysin, and toxic shock syndrome toxin-1 production in early-stationary-phase cultures. The cloned gene showed considerable variation with respect to different exoproteins and different host strains compared with the chromosomal agr determinant; this variation could not be attributed to the higher copy number of the cloned gene and probably reflects inapparent subtleties of the regulatory system.

AB - We have previously identified a gene in Staphylococcus aureus, agr, whose activity is required for high-level post-exponential-phase expression of a series of secreted proteins. In this paper, we describe the cloning of this gene in Escherichia coli by using an inserted transposon (Tn551) as a cloning probe. The cloned gene, consisting of a 241-codon open reading frame containing the site of the transposon insertion, was recloned to an S. aureus vector, pSK265, and shown to be functional in S. aureus. Activity was evaluated by determinations of α-hemolysin, β-hemolysin, and toxic shock syndrome toxin-1 production in early-stationary-phase cultures. The cloned gene showed considerable variation with respect to different exoproteins and different host strains compared with the chromosomal agr determinant; this variation could not be attributed to the higher copy number of the cloned gene and probably reflects inapparent subtleties of the regulatory system.

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Cloning, characterization and sequencing of an accessory gene regulator (agr) in Staphylococcus aureus

Abstract

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