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枯草芽孢杆菌的σ28因子和大肠杆菌的σ32因子(htpR)是具有重叠启动子特异性的次要σ因子。

Bacillus subtilis sigma 28 and Escherichia coli sigma 32 (htpR) are minor sigma factors that display an overlapping promoter specificity.

作者信息

Briat J F, Gilman M Z, Chamberlin M J

出版信息

J Biol Chem. 1985 Feb 25;260(4):2038-41.

PMID:3918995
Abstract

Bacillus subtilis sigma 28-specific promoters (P28) are utilized by a minor form of B. subtilis RNA polymerase (sigma 28RNA polymerase) and not by the predominant RNA polymerases of B. subtilis (sigma 43 RNA polymerase) or Escherichia coli (sigma 70 RNA polymerase). However B. subtilis P28 are effective promoters in E. coli. This transcription depends on the E. coli htpR+ gene. Similarly, the E. coli rpoD heat shock promoter which is under control of htpR is used in vitro by B. subtilis sigma 28 RNA polymerase. These observations are explained by the fact that E. coli htpR is a minor sigma factor (sigma 32) which shares an overlapping promoter specificity with B. subtilis sigma 28 RNA polymerase. Hence control of bacterial regulons by minor sigma factors is not restricted to Bacilli, or bacteria that carry out a complex differentiation process, but is probably a general, regulatory mechanism in prokaryotes. Transcription from B. subtilis P28 in E. coli does not depend on a heat shock. This suggests that the sequences that control E. coli sigma 32 action are separate from those that control the heat shock regulon. Hence the action of polymerases controlled by minor sigma factors in both B. subtilis and E. coli appears to be controlled by a separate set of regulatory factors.

摘要

枯草芽孢杆菌σ28特异性启动子(P28)被枯草芽孢杆菌RNA聚合酶的一种次要形式(σ28RNA聚合酶)所利用,而不被枯草芽孢杆菌的主要RNA聚合酶(σ43RNA聚合酶)或大肠杆菌(σ70RNA聚合酶)所利用。然而,枯草芽孢杆菌P28在大肠杆菌中是有效的启动子。这种转录依赖于大肠杆菌htpR+基因。同样,受htpR控制的大肠杆菌rpoD热休克启动子在体外被枯草芽孢杆菌σ28RNA聚合酶所利用。这些观察结果可以解释为,大肠杆菌htpR是一种次要的σ因子(σ32),它与枯草芽孢杆菌σ28RNA聚合酶具有重叠的启动子特异性。因此,由次要σ因子控制细菌调节子并不局限于芽孢杆菌或进行复杂分化过程的细菌,而可能是原核生物中的一种普遍的调节机制。在大肠杆菌中,从枯草芽孢杆菌P28进行的转录不依赖于热休克。这表明控制大肠杆菌σ32作用的序列与控制热休克调节子的序列是分开的。因此,在枯草芽孢杆菌和大肠杆菌中,由次要σ因子控制的聚合酶的作用似乎受一套独立的调节因子控制。

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