Molecular cloning and characterization of protective outer membrane protein P.69 from Bordetella pertussis.

Charles, IG; Dougan, G; Pickard, D; Chatfield, S; Smith, M; Novotny, P; Morrissey, P; Fairweather, NF

Molecular cloning and characterization of protective outer membrane protein P.69 from Bordetella pertussis.

Charles, IG Dougan, G Pickard, D Chatfield, S Smith, M Novotny, P Morrissey, P Fairweather, NF

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Publication Type:: Journal Article
Citation:: Proc Natl Acad Sci U S A, 1989, 86 (10), pp. 3554 - 3558
Issue Date:: 1989-05

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Field	Value	Language
dc.contributor.author	Charles, IG	en_US
dc.contributor.author	Dougan, G	en_US
dc.contributor.author	Pickard, D	en_US
dc.contributor.author	Chatfield, S	en_US
dc.contributor.author	Smith, M	en_US
dc.contributor.author	Novotny, P	en_US
dc.contributor.author	Morrissey, P	en_US
dc.contributor.author	Fairweather, NF	en_US
dc.date.issued	1989-05	en_US
dc.identifier.citation	Proc Natl Acad Sci U S A, 1989, 86 (10), pp. 3554 - 3558	en_US
dc.identifier.issn	0027-8424	en_US
dc.identifier.uri	http://hdl.handle.net/10453/13236
dc.description.abstract	Protein P.69 is localized on the outer membrane of Bordetella pertussis and is one of the virulence factors believed to contribute to the disease state of whooping cough. We demonstrate that protein synthesis of P.69 is under genetic control of the vir locus. Using oligonucleotide probes derived from the protein sequence of a cyanogen bromide fragment, we have cloned the gene for P.69 from B. pertussis CN2992. Analysis of the DNA sequence reveals a G + C-rich gene capable of encoding a protein of 910 amino acids with a Mr of 93,478, suggesting that P.69 is a processed form of a larger precursor. In common with some of the genes in the pertussis toxin operon, the sequence CCTGG was found 5' to the ATG initiation codon. At the 3' end, 29 bases after the TAA stop codon, the sequence GTTTTTCCT was found and may have some function in transcription termination. A full-length clone of the gene for P.69 carried by the cosmid pBPI69 was unable to direct the expression of P.69 protein in an Escherichia coli host. The generation of P.69-fusion products allowed the detection of P.69-specific protein products synthesized in E. coli.	en_US
dc.language	eng	en_US
dc.relation.ispartof	Proc Natl Acad Sci U S A	en_US
dc.relation.isbasedon	10.1073/pnas.86.10.3554	en_US
dc.subject.mesh	Bordetella pertussis	en_US
dc.subject.mesh	Escherichia coli	en_US
dc.subject.mesh	Bacterial Outer Membrane Proteins	en_US
dc.subject.mesh	Recombinant Proteins	en_US
dc.subject.mesh	DNA, Bacterial	en_US
dc.subject.mesh	Antigens, Bacterial	en_US
dc.subject.mesh	Blotting, Western	en_US
dc.subject.mesh	Restriction Mapping	en_US
dc.subject.mesh	Cloning, Molecular	en_US
dc.subject.mesh	Gene Expression Regulation	en_US
dc.subject.mesh	Protein Processing, Post-Translational	en_US
dc.subject.mesh	Amino Acid Sequence	en_US
dc.subject.mesh	Base Sequence	en_US
dc.subject.mesh	Regulatory Sequences, Nucleic Acid	en_US
dc.subject.mesh	Genes, Bacterial	en_US
dc.subject.mesh	Molecular Sequence Data	en_US
dc.subject.mesh	Terminator Regions, Genetic	en_US
dc.title	Molecular cloning and characterization of protective outer membrane protein P.69 from Bordetella pertussis.	en_US
dc.type	Journal Article
utslib.citation.volume	10	en_US
utslib.citation.volume	86	en_US
utslib.location.activity	United States	en_US
utslib.for	060409 Molecular Evolution	en_US
dc.location.activity	ISI:A1989U652300025	en_US
pubs.embargo.period	Not known	en_US
pubs.organisational-group	/University of Technology Sydney
pubs.organisational-group	/University of Technology Sydney/Faculty of Engineering and Information Technology
pubs.organisational-group	/University of Technology Sydney/Faculty of Engineering and Information Technology/School of Mechanical and Mechatronic Engineering
pubs.organisational-group	/University of Technology Sydney/Faculty of Science
pubs.organisational-group	/University of Technology Sydney/Strength - ithree - Institute of Infection, Immunity and Innovation
utslib.copyright.status	closed_access
pubs.issue	10	en_US
pubs.publication-status	Published	en_US
pubs.volume	86	en_US

Abstract:

Protein P.69 is localized on the outer membrane of Bordetella pertussis and is one of the virulence factors believed to contribute to the disease state of whooping cough. We demonstrate that protein synthesis of P.69 is under genetic control of the vir locus. Using oligonucleotide probes derived from the protein sequence of a cyanogen bromide fragment, we have cloned the gene for P.69 from B. pertussis CN2992. Analysis of the DNA sequence reveals a G + C-rich gene capable of encoding a protein of 910 amino acids with a Mr of 93,478, suggesting that P.69 is a processed form of a larger precursor. In common with some of the genes in the pertussis toxin operon, the sequence CCTGG was found 5' to the ATG initiation codon. At the 3' end, 29 bases after the TAA stop codon, the sequence GTTTTTCCT was found and may have some function in transcription termination. A full-length clone of the gene for P.69 carried by the cosmid pBPI69 was unable to direct the expression of P.69 protein in an Escherichia coli host. The generation of P.69-fusion products allowed the detection of P.69-specific protein products synthesized in E. coli.

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http://hdl.handle.net/10453/13236