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J. Bacteriol., Dec 1995, 6866-6873, Vol 177, No. 23
X Li, GM Weinstock and BE Murray
A 22-kb segment of chromosomal DNA from Enterococcus faecalis OG1RF
containing the pyrimidine biosynthesis genes pyrC and pyrD was previously
detected as complementing Escherichia coli pyrC and pyrD mutations. In the
present study, it was found that the E. faecalis pyrimidine biosynthetic
genes in this clone (designated pKV48) are part of a larger cluster
resembling that seen in Bacillus spp. Transposon insertions were isolated
at a number of sites throughout the cluster and resulted in loss of the
ability to complement E. coli auxotrophs. The DNA sequences of the entire
pyrD gene of E. faecalis and selected parts of the rest of the cluster were
determined, and computer analyses found these to be similar to genes from
Bacillus subtilis and Bacillus caldolyticus pyrimidine biosynthesis
operons. Five of the transposon insertions were introduced back into the E.
faecalis chromosome, and all except insertions in pyrD resulted in
pyrimidine auxotrophy. The prototrophy of pyrD knockouts was observed for
two different insertions and suggests that E. faecalis is similar to
Lactococcus lactis, which has been shown to possess two pyrD genes. A
similar analysis was performed with the purL gene from E. faecalis,
contained in another cosmid clone, and purine auxotrophs were isolated. In
addition, a pool of random transposon insertions in pKV48, isolated in E.
coli, was introduced into the E. faecalis chromosome en masse, and an
auxotroph was obtained. These results demonstrate a new methodology for
constructing defined knockout mutations in E. faecalis.
Copyright © 1995, American Society for Microbiology
Generation of auxotrophic mutants of Enterococcus faecalis
Department of Microbiology and Molecular Genetics, University of Texas Medical School, Houston 77030, USA.
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