Site-specific insertion of gene cassettes into integrons.

Collis, CM; Grammaticopoulos, G; Briton, J; Stokes, HW; Hall, RM

Site-specific insertion of gene cassettes into integrons.

Collis, CM Grammaticopoulos, G Briton, J Stokes, HW Hall, RM

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Publication Type:: Journal Article
Citation:: Mol Microbiol, 1993, 9 (1), pp. 41 - 52
Issue Date:: 1993-07

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Field	Value	Language
dc.contributor.author	Collis, CM	en_US
dc.contributor.author	Grammaticopoulos, G	en_US
dc.contributor.author	Briton, J	en_US
dc.contributor.author	Stokes, HW	en_US
dc.contributor.author	Hall, RM	en_US
dc.date.issued	1993-07	en_US
dc.identifier.citation	Mol Microbiol, 1993, 9 (1), pp. 41 - 52	en_US
dc.identifier.issn	0950-382X	en_US
dc.identifier.uri	http://hdl.handle.net/10453/26088
dc.description.abstract	Site-specific insertion of gene cassettes into the insert region of integrons has been demonstrated. Insertion was only observed if the integron DNA integrase was expressed in the recipient cell and if the cassette DNA was ligated prior to transformation. The essential ligation products were resistant to treatment with exonuclease III, indicating that they were closed circular molecules. Insertion of cassettes into integron fragments containing either no insert (one recombination site), or one gene cassette (two recombination sites), was demonstrated. In the latter case, insertion occurred predominantly at the core site located 5' to the resident cassette, which corresponds to the only site available when no insert is present in the recipient. When DNA molecules including two gene cassettes were used, insertion of only one of the gene cassettes was generally observed, suggesting that resolution of the circular molecule to generate two independent circular cassettes occurred more rapidly than insertion into the recipient integron.	en_US
dc.language	eng	en_US
dc.relation.ispartof	Mol Microbiol	en_US
dc.relation.isbasedon	10.1111/j.1365-2958.1993.tb01667.x	en_US
dc.subject.classification	Microbiology	en_US
dc.subject.mesh	Escherichia coli	en_US
dc.subject.mesh	Integrases	en_US
dc.subject.mesh	DNA Nucleotidyltransferases	en_US
dc.subject.mesh	DNA, Bacterial	en_US
dc.subject.mesh	DNA, Circular	en_US
dc.subject.mesh	DNA, Recombinant	en_US
dc.subject.mesh	DNA Transposable Elements	en_US
dc.subject.mesh	Mutagenesis, Insertional	en_US
dc.subject.mesh	Mutagenesis, Site-Directed	en_US
dc.subject.mesh	Gene Expression Regulation, Bacterial	en_US
dc.subject.mesh	Recombination, Genetic	en_US
dc.subject.mesh	Base Sequence	en_US
dc.subject.mesh	Molecular Sequence Data	en_US
dc.title	Site-specific insertion of gene cassettes into integrons.	en_US
dc.type	Journal Article
utslib.citation.volume	1	en_US
utslib.citation.volume	9	en_US
utslib.location.activity	England	en_US
utslib.for	0605 Microbiology	en_US
utslib.for	06 Biological Sciences	en_US
utslib.for	07 Agricultural and Veterinary Sciences	en_US
utslib.for	11 Medical and Health Sciences	en_US
dc.location.activity	ISI:A1993LL41500005	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 Science
utslib.copyright.status	closed_access
pubs.issue	1	en_US
pubs.publication-status	Published	en_US
pubs.volume	9	en_US

Abstract:

Site-specific insertion of gene cassettes into the insert region of integrons has been demonstrated. Insertion was only observed if the integron DNA integrase was expressed in the recipient cell and if the cassette DNA was ligated prior to transformation. The essential ligation products were resistant to treatment with exonuclease III, indicating that they were closed circular molecules. Insertion of cassettes into integron fragments containing either no insert (one recombination site), or one gene cassette (two recombination sites), was demonstrated. In the latter case, insertion occurred predominantly at the core site located 5' to the resident cassette, which corresponds to the only site available when no insert is present in the recipient. When DNA molecules including two gene cassettes were used, insertion of only one of the gene cassettes was generally observed, suggesting that resolution of the circular molecule to generate two independent circular cassettes occurred more rapidly than insertion into the recipient integron.

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http://hdl.handle.net/10453/26088