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Overcoming the restriction barrier to plasmid transformation and targeted mutagenesis in Bifidobacterium breve UCC2003
Authors:Mary O'Connell Motherway  Jonathan O'Driscoll  Gerald F Fitzgerald  Douwe Van Sinderen
Institution:1. Alimentary Pharmabiotic Centre,;2. Department of Microbiology and;3. Present address: New England Biolabs, Inc., 240 County Road, Ipswich, MA 01938‐2723, USA.;4. Department of Food and Nutritional Sciences , National University of Ireland, Cork, Western Road, Cork, Ireland.
Abstract:In silico analysis of the Bifidobacterium breve UCC2003 genome predicted two distinct loci, which encode three different restriction/modification systems, each comprising a modification methylase and a restriction endonuclease. Based on sequence homology and observed protection against restriction we conclude that the first restriction endonuclease, designated BbrI, is an isoschizomer of BbeI, the second, BbrII, is a neoschizomer of SalI, while the third, BbrIII, is an isoschizomer of PstI. Expression of each of the B. breve UCC2003 methylase‐encoding genes in B. breve JCM 7017 established that BbrII and BbrIII are active and restrict incoming DNA. By exploiting knowledge on restriction/modification in B. breve UCC2003 we successfully increased the transformation efficiency to a level that allows the reliable generation of mutants by homologous recombination using a non‐replicative plasmid.
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