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Use of bacteriophage lambda recombination functions to promote gene replacement in Escherichia coli

Murphy, Kenan C.
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Authors
Murphy, Kenan C.
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Faculty Advisor
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UMass Chan Affiliations
Department of Molecular Genetics and Microbiology
Document Type
Journal Article
Publication Date
1998-04-29
Keywords
Bacteriophage lambda
 Calcium
 Chromosomes, Bacterial
 Cloning, Molecular
 DNA Primers
 DNA, Superhelical
 Escherichia coli
 Gene Targeting
 Genotype
 Operon
 Plasmids
 Polymerase Chain Reaction
 Recombinant Fusion Proteins
 *Recombination, Genetic
 Restriction Mapping
 Life Sciences
 Medicine and Health Sciences
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UMass Chan Faculty and Researcher Publications
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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC107131/pdf/jb002063.pdf
Abstract

Replacement of Escherichia coli's RecBCD function with phage lambda's Red function generates a strain whose chromosome recombines with short linear DNA fragments at a greatly elevated rate. The rate is at least 70-fold higher than that exhibited by a recBC sbcBC or recD strain. The value of the system is highlighted by gene replacement with a PCR-generated DNA fragment. The deltarecBCD::Plac-red kan replacement allele can be P1 transduced to other E. coli strains, making the hyper-Rec phenotype easily transferable.

Source

J Bacteriol. 1998 Apr;180(8):2063-71.

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https://hdl.handle.net/20.500.14038/42298
PubMed ID
9555887
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