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J. Bacteriol., 07 1996, 3840-3845, Vol 178, No. 13
MM Zaman and TC Boles
Previously, we demonstrated that exonuclease I-deficient strains of
Escherichia coli accumulate high-molecular-weight linear plasmid
concatemers when transformed with plasmids carrying the chi sequence (5'-
GCTGGTGG-3') (M. M. Zaman and T. C. Boles, J. Bacteriol. 176:5093- 5100,
1994). Since high-molecular weight linear DNA is believed to be the natural
substrate for RecBCD-mediated recombination during conjugation (A. J. Clark
and K. B. Low, p. 155-215, in K. B. Low, ed., The Recombination of Genetic
Material, 1988), we analyzed the recombination frequencies of chi+ and chi0
plasmids in sbcB strains. Here, we report that chi sites stimulate plasmid
recombination frequency by 16-fold in sbcB strains. Chi-stimulated plasmid
recombination is dependent on RecBCD but is independent of RecF pathway
genes. The distribution of recombination products suggests that high-
molecular-weight linear plasmid DNA is a substrate for RecBCD-mediated
recombination. Surprisingly, our data also suggest that chi+ plasmids also
recombine by the RecBCD pathway in rec+ sbcB+ cells.
Copyright © 1996, American Society for Microbiology
Plasmid recombination by the RecBCD pathway of Escherichia coli
Graduate Department of Biochemistry, Brandeis University, Waltham, Massachusetts 02254, USA.
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