Affiliation:
1. Departments of Microbiology1 and
2. Biochemistry,2 University of Illinois, Urbana, Illinois 61801
Abstract
ABSTRACT
The genes encoding several key fatty acid biosynthetic enzymes (called the
fab
cluster) are clustered in the order
plsX-fabH-fabD-fabG-acpP-fabF
at min 24 of the
Escherichia coli
chromosome. A difficulty in analysis of the
fab
cluster by the polar allele duplication approach (Y. Zhang and J. E. Cronan, Jr., J. Bacteriol. 178:3614–3620, 1996) is that several of these genes are essential for the growth of
E. coli
. We overcame this complication by use of the
fab
gene cluster of
Salmonella typhimurium
, a close relative of
E. coli
, to provide functions necessary for growth. The
S. typhimurium fab
cluster was isolated by complementation of an
E. coli fabD
mutant and was found to encode proteins with >94% homology to those of
E. coli
. However, the
S. typhimurium
sequences cannot recombine with the
E. coli
sequences required to direct polar allele duplication via homologous recombination. Using this approach, we found that although approximately 60% of the
plsX
transcripts initiate at promoters located far upstream and include the upstream
rpmF
ribosomal protein gene, a promoter located upstream of the
plsX
coding sequence (probably within the upstream gene,
rpmF
) is sufficient for normal growth. We have also found that the
fabG
gene is obligatorily cotranscribed with upstream genes. Insertion of a transcription terminator cassette (Ω-Cm cassette) between the
fabD
and
fabG
genes of the
E. coli
chromosome abolished
fabG
transcription and blocked cell growth, thus providing the first indication that
fabG
is an essential gene. Insertion of the Ω-Cm cassette between
fabH
and
fabD
caused greatly decreased transcription of the
fabD
and
fabG
genes and slower cellular growth, indicating that
fabD
has only a weak promoter(s).
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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