O Gray scite author profile

O Gray

5Publications

66Citation Statements Received

91Citation Statements Given

How they've been cited

169

How they cite others

117

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Structural and genetic analyses of a par locus that regulates plasmid partition in Bacillus subtilis

Chang¹,

Chang²,

Gray³

1987

J Bacteriol

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The BaciUus plasmid pLS11 partitions faithfully during ceil division. Using a partition-deficient plasmid vector, we randomly cloned DNA fragments of plasmid pLST1 and identified the locus that regulates plasmid partition (par) by cis complementation in Bacillus subtlis. The cloned par gene conferred upon the vector plasmid a high degree of segregational stability. The par locus was mapped to a 167-base-pair segment on pLS11, and its nucleotide sequence was determined. The cloned par fragment regulated the partition of several different Bacillus replicons, and it only functioned in cis; it did not contain the replication function nor elevate the plasmid copy number in B. subtilis. The expression of par was orientation specific with respect to the replication origin on the same plasmid. We propose that the pLS11-derived par functions as a single-stranded site that interacts with other components involved in plasmid partition during cell division.

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Expression of Eukaryotic Genes in B. subtilis Using Signals of penP

Chang¹,

Gray²,

Ho³

et al. 1982

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Molecular cloning and expression of Bacillus licheniformis beta-lactamase gene in Escherichia coli and Bacillus subtilis.

Gray¹,

Chang²

1981

106

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The chromosomal beta-lactamase (penicillinase, penP) gene from Bacillus licheniformis 749/C has been cloned in Escherichia coli. The locations of the target sites for various restriction enzymes on the 4.2-kilobase EcoRI fragment were determined. By matching the restriction mapping data with the potential nucleotide sequences of the penP gene deduced from known protein sequence, we established the exact position of the penP gene on the fragment. A bifunctional plasmid vector carrying the penP gene, plasmid pOG2165, was constructed which directs the synthesis of the heterologous beta-lactamase in both E. coli and Bacillus subtilis hosts. The protein synthesized in E. coli and B. subtilis is similar in size to the processed beta-lactamase made in B. licheniformis. Furthermore, the beta-lactamase made in B. subtilis is efficiently secreted by the host into the culture medium, indicating that B. subtilis is capable of carrying out the post-translational proteolytic cleavage(s) to convert the membrane-bound precursor enzyme into the soluble extracellular form.

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Species-specific monoclonal antibody to a 43,000-molecular-weight membrane protein of Mycoplasma pneumoniae

Madsen¹,

Saeed²,

Gray³

et al. 1986

J Clin Microbiol

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A murine immunoglobulin GI monoclonal antibody was produced that binds to a protease-sensitive, periodate-insensitive epitope on a 43,000-molecular-weight Mycoplasma pneumoniae membrane polypeptide. The 43,000-molecular-weight polypeptide appeared to be a major antigenic component of M. pneumoniae, as determined by immunoblot analysis. This monoclonal antibody reacted with 33 different clinical isolates of M. pneumoniae, but not with normal-flora Mycoplasma species or 18 other microorganisms potentially inhabiting the normal or diseased human respiratory tract. This apparent species-specific monoclonal antibody may have application for the detection of M. pneumoniae antigen in clinical specimens.

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Hæmolytic Streptococcal Infections

Rendle-Short

Gray²

1967

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O Gray

Structural and genetic analyses of a par locus that regulates plasmid partition in Bacillus subtilis

Expression of Eukaryotic Genes in B. subtilis Using Signals of penP

Molecular cloning and expression of Bacillus licheniformis beta-lactamase gene in Escherichia coli and Bacillus subtilis.

Species-specific monoclonal antibody to a 43,000-molecular-weight membrane protein of Mycoplasma pneumoniae

Hæmolytic Streptococcal Infections

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