Binding of the purified integron DNA integrase Intl1 to integron- and cassette-associated recombination sites.

Collis, CM; Kim, MJ; Stokes, HW; Hall, RM

Binding of the purified integron DNA integrase Intl1 to integron- and cassette-associated recombination sites.

Collis, CM Kim, MJ Stokes, HW Hall, RM

Permalink

Publication Type:: Journal Article
Citation:: Mol Microbiol, 1998, 29 (2), pp. 477 - 490
Issue Date:: 1998-07

Closed Access

	Filename	Description	Size
	2008005628OK.pdf		797.51 kB	Adobe PDF	View/Open

Copyright Clearance Process

Recently Added
In Progress
Closed Access

This item is closed access and not available.

Full metadata record

Field	Value	Language
dc.contributor.author	Collis, CM	en_US
dc.contributor.author	Kim, MJ	en_US
dc.contributor.author	Stokes, HW	en_US
dc.contributor.author	Hall, RM	en_US
dc.date.issued	1998-07	en_US
dc.identifier.citation	Mol Microbiol, 1998, 29 (2), pp. 477 - 490	en_US
dc.identifier.issn	0950-382X	en_US
dc.identifier.uri	http://hdl.handle.net/10453/8741
dc.description.abstract	The site-specific recombinase Intl1, encoded by class 1 integrons, catalyses the integration and excision of gene cassettes by recognizing two classes of sites, the integron-associated attl1 site and the 59-base element (59-be) family of sites that are associated with gene cassettes. Intl1 includes the four conserved amino acids that are characteristic of members of the integrase family, and Intl1 proteins with single amino acid substitutions at each of these positions had substantially reduced catalytic activity, consistent with this classification. Intl1 was purified as a fusion protein and shown to bind to isolated attl1 or 59-be recombination sites. Binding to attl1 was considerably stronger than to a 59-be. Binding adjacent to the recombination cross-over point was not detected. A strong Intl1 binding site within attl1 was localized by both deletion and footprinting analysis to a 14 bp region 24-37 bp to the left of the recombination cross-over point, and this region is known to be critical for recombination in vivo (Recchia et al., 1994). An imperfect (13/15) direct repeat of this region, located 41-55 bp to the left of the recombination cross-over point, contains a weaker Intl1 binding site. Mutation of the stronger binding site showed that a single base pair change accounted for the difference in the strength of binding.	en_US
dc.language	eng	en_US
dc.relation.ispartof	Mol Microbiol	en_US
dc.relation.isbasedon	10.1046/j.1365-2958.1998.00936.x	en_US
dc.subject.classification	Microbiology	en_US
dc.subject.mesh	Recombinases	en_US
dc.subject.mesh	Integrases	en_US
dc.subject.mesh	DNA Nucleotidyltransferases	en_US
dc.subject.mesh	Bacterial Proteins	en_US
dc.subject.mesh	Recombinant Fusion Proteins	en_US
dc.subject.mesh	DNA Footprinting	en_US
dc.subject.mesh	Recombination, Genetic	en_US
dc.subject.mesh	Binding Sites	en_US
dc.subject.mesh	Amino Acid Sequence	en_US
dc.subject.mesh	Base Sequence	en_US
dc.subject.mesh	Conserved Sequence	en_US
dc.subject.mesh	Substrate Specificity	en_US
dc.subject.mesh	Mutation	en_US
dc.subject.mesh	Molecular Sequence Data	en_US
dc.title	Binding of the purified integron DNA integrase Intl1 to integron- and cassette-associated recombination sites.	en_US
dc.type	Journal Article
utslib.citation.volume	2	en_US
utslib.citation.volume	29	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:000075560500008	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	2	en_US
pubs.publication-status	Published	en_US
pubs.volume	29	en_US

Abstract:

The site-specific recombinase Intl1, encoded by class 1 integrons, catalyses the integration and excision of gene cassettes by recognizing two classes of sites, the integron-associated attl1 site and the 59-base element (59-be) family of sites that are associated with gene cassettes. Intl1 includes the four conserved amino acids that are characteristic of members of the integrase family, and Intl1 proteins with single amino acid substitutions at each of these positions had substantially reduced catalytic activity, consistent with this classification. Intl1 was purified as a fusion protein and shown to bind to isolated attl1 or 59-be recombination sites. Binding to attl1 was considerably stronger than to a 59-be. Binding adjacent to the recombination cross-over point was not detected. A strong Intl1 binding site within attl1 was localized by both deletion and footprinting analysis to a 14 bp region 24-37 bp to the left of the recombination cross-over point, and this region is known to be critical for recombination in vivo (Recchia et al., 1994). An imperfect (13/15) direct repeat of this region, located 41-55 bp to the left of the recombination cross-over point, contains a weaker Intl1 binding site. Mutation of the stronger binding site showed that a single base pair change accounted for the difference in the strength of binding.

Please use this identifier to cite or link to this item:

http://hdl.handle.net/10453/8741