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J. Bacteriol., 07 1995, 3647-3655, Vol 177, No. 13
M Kaiser and G Sawers
The pfl operon is expressed at high levels anaerobically. Growth of
Escherichia coli in the presence of nitrate or nitrite led to a 45%
decrease in expression when cells were cultivated in rich medium. Nitrate
repression, however, was significantly enhanced (sevenfold) when the cells
were cultured in minimal medium. Regulation of pfl expression by nitrate
was dependent on the NarL, NarP, NarQ, and NarX proteins but independent of
FNR, ArcA, and integration host factor, which are additional regulators of
pfl expression. Strains unable to synthesize any one of the NarL, NarP,
NarQ, or NarX proteins, but retaining the capacity to synthesize the
remaining three, exhibited essentially normal nitrate regulation. In
contrast, narL narP and narX narQ double null mutants were devoid of
nitrate regulation when cultured in rich medium but they retained some
nitrate repression (1.3- fold) when grown in minimal medium. By using lacZ
fusions, it was possible to localize the DNA sequences required to mediate
nitrate repression to the pfl promoter-regulatory region. DNase I
footprinting studies identified five potential binding sites for the
wild-type NarL protein in the pfl promoter-regulatory region. Specific
footprints were obtained only when NarL was phosphorylated with acetyl
phosphate before the binding reaction was performed. Each of the protected
regions contained at least one heptamer sequence which has been deduced
from mutagenesis studies to be essential for NarL binding (K. Tyson, A.
Bell, J. Cole, and S. Busby, Mol. Microbiol. 7:151-157, 1993).
Copyright © 1995, American Society for Microbiology
Nitrate repression of the Escherichia coli pfl operon is mediated by the dual sensors NarQ and NarX and the dual regulators NarL and NarP
Lehrstuhl fur Mikrobiologie, Universitat Munchen, Germany.
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