Affiliation:
1. Department of Biotechnology, Faculty of Life Science and Biotechnology, Fukuyama University, Fukuyama-shi, Hiroshima, Japan
Abstract
ABSTRACT
The
Bacillus subtilis ilv-leu
operon functions in the biosynthesis of branched-chain amino acids. It undergoes catabolite activation involving a promoter-proximal
cre
which is mediated by the complex of CcpA and P-Ser-HPr. This activation of
ilv-leu
expression is negatively regulated through CodY binding to a high-affinity site in the promoter region under amino acid-rich growth conditions, and it is negatively regulated through TnrA binding to the TnrA box under nitrogen-limited growth conditions. The CcpA-mediated catabolite activation of
ilv-leu
required a helix face-dependent interaction of the complex of CcpA and P-Ser-HPr with RNA polymerase and needed a 19-nucleotide region upstream of
cre
for full activation. DNase I footprinting indicated that CodY binding to the high-affinity site competitively prevented the binding of the complex of CcpA and P-Ser-HPr to
cre
. This CodY binding not only negated catabolite activation but also likely inhibited transcription initiation from the
ilv-leu
promoter. The footprinting also indicated that TnrA and the complex of CcpA and P-Ser-HPr simultaneously bound to the TnrA box and the
cre
site, respectively, which are 112 nucleotides apart; TnrA binding to its box was likely to induce DNA bending. This implied that interaction of TnrA bound to its box with the complex of CcpA and P-Ser-HPr bound to
cre
might negate catabolite activation, but TnrA bound to its box did not inhibit transcription initiation from the
ilv-leu
promoter. Moreover, this negation of catabolite activation by TnrA required a 26-nucleotide region downstream of the TnrA box.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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