FruR-mediated transcriptional activation at the ppsA promoter of Escherichia coli

被引:22
|
作者
Nègre, D
Oudot, C
Prost, JF
Murakami, K
Ishihama, A
Cozzone, AJ
Cortay, JC
机构
[1] CNRS, Inst Biol & Chim Prot, F-69367 Lyon, France
[2] Natl Inst Genet, Shizuoka 411, Japan
关键词
base removal interference; FruR protein of Escherichia coli; mutant alpha subunit of RNA polymerase; ppsA gene; transcription activation;
D O I
10.1006/jmbi.1997.1548
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The start site of transcription of the ppsA gene, whose expression is controlled by the regulatory protein FruR in Escherichia coli, was determined by primer extension of in vivo transcripts. The interactions of the ppsA promoter with either RNA polymerase or FruR factor were analysed by the base removal method. Our results indicate that: (i) the RNA polymerase binding site has a -10 extended module but lacks its -35 hexamer; (ii) FruR binds to a target DT IA region centered around position -45.5 upstream of the ppsA gene. In addition, circular permutation analysis showed that, upon binding to its site, FruR induces a sharp bend of 120 degrees in the DNA helix, which suggests a crucial involvement of FruR-induced bending in ppsA promoter activation. Direct contacts between the upstream activating DNA and RNA polymerase were studied in an in vitro transcription assay by using reconstituted RNA polymerase mutants containing Ala substitutions in the C-terminal domain of their a subunit. The alpha[L262A], alpha[R265A] and alpha[N268A] substitutions, which caused the most drastic reduction in the FruR-mediated activation of the ppsA promoter, had previously been shown to inhibit the upstream element-mediated activation at the rrnBP1 promoter. (C) 1998 Academic Press Limited.
引用
收藏
页码:355 / 365
页数:11
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