首页> 美国卫生研究院文献>The EMBO Journal >A mutation in region 1.1 of sigma70 affects promoter DNA binding by Escherichia coli RNA polymerase holoenzyme.
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A mutation in region 1.1 of sigma70 affects promoter DNA binding by Escherichia coli RNA polymerase holoenzyme.

机译:sigma70区域1.1中的突变影响大肠杆菌RNA聚合酶全酶对启动子DNA的结合。

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摘要

The sigma subunit of eubacterial RNA polymerase is essential for initiation of transcription at promoter sites. It directs recognition of DNA sequences by holoenzyme (alpha2betabeta'sigma) and facilitates subsequent steps in the initiation pathway. The primary sigma factor from Escherichia coli, sigma70, has four regions that are conserved among members of the sigma70 family. Previous work has shown that region 1.1 modulates DNA binding by regions 2 and 4 when sigma is separated from the core subunits, and is required for efficient progression through the later steps of initiation in the context of holoenzyme. In this report, we show that an amino acid substitution at position 53 in region 1.1, which converts isoleucine to alanine (I53A), creates a sigma factor that associates with the core subunits to form holoenzyme, but the holoenzyme is severely deficient for promoter binding. The I53A phenotype can be suppressed by truncation of five amino acids from the C-terminus of sigma70. We propose that the behavior of sigma70-I53A is a consequence of impaired ability to undergo a critical conformational change upon binding to the core subunits, which is needed to expose the DNA-binding domains and confer promoter recognition capability upon holoenzyme.
机译:真细菌RNA聚合酶的σ亚基对于启动子启动子的转录至关重要。它指导全酶(α2betabeta'sigma)对DNA序列的识别,并促进起始途径中的后续步骤。大肠杆菌的主要sigma因子sigma70具有四个在sigma70家族成员中保守的区域。先前的工作表明,当σ与核心亚基分开时,区域1.1会调节区域2和区域4的DNA结合,这对于在完整酶作用下通过后续起始步骤有效进行是必需的。在此报告中,我们显示区域1.1中第53位的氨基酸取代将异亮氨酸转化为丙氨酸(I53A),创建了一个与核心亚基缔合形成全酶的sigma因子,但该全酶严重缺乏启动子结合能力。 I53A表型可以通过从sigma70的C端截短五个氨基酸来抑制。我们提出,sigma70-I53A的行为是与核心亚基结合后经历关键构象变化的能力受损的结果,这需要暴露DNA结合域并赋予全酶启动子识别能力。

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