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基于结构的RNA聚合酶功能分析:最大亚基的“舵”对延伸复合物稳定性起关键作用,且不参与维持RNA-DNA杂交链长度。

Structure-based analysis of RNA polymerase function: the largest subunit's rudder contributes critically to elongation complex stability and is not involved in the maintenance of RNA-DNA hybrid length.

作者信息

Kuznedelov Konstantin, Korzheva Nataliya, Mustaev Arkady, Severinov Konstantin

机构信息

Waksman Institute, Rutgers, The State University, Piscataway, NJ 08854, USA.

出版信息

EMBO J. 2002 Mar 15;21(6):1369-78. doi: 10.1093/emboj/21.6.1369.

Abstract

Analysis of multisubunit RNA polymerase (RNAP) structures revealed several elements that may constitute the enzyme's functional sites. One such element, the 'rudder', is formed by an evolutionarily conserved segment of the largest subunit of RNAP and contacts the nascent RNA at the upstream edge of the RNA-DNA hybrid, where the DNA template strand separates from the RNA transcript and re-anneals with the non-template strand. Thus, the rudder could (i) maintain the correct length of the RNA-DNA hybrid; (ii) stabilize the nascent RNA in the complex; and (iii) promote or maintain localized DNA melting at the upstream edge of the bubble. We generated a recombinant RNAP mutant that lacked the rudder and studied its properties in vitro. Our results demonstrate that the rudder is not required for establishment of the upstream boundary of the transcription bubble during promoter complex formation, nor is it required for separation of the nascent RNA from the DNA template strand or transcription termination. Our results suggest that the rudder makes critical contributions to elongation complex stability through direct interactions with the nascent RNA.

摘要

对多亚基RNA聚合酶(RNAP)结构的分析揭示了几个可能构成该酶功能位点的元件。其中一个这样的元件,即“舵”,由RNAP最大亚基的一个进化保守片段形成,并在RNA-DNA杂交体的上游边缘与新生RNA接触,在此处DNA模板链与RNA转录本分离并与非模板链重新退火。因此,“舵”可以(i)维持RNA-DNA杂交体的正确长度;(ii)稳定复合物中的新生RNA;以及(iii)促进或维持气泡上游边缘的局部DNA解链。我们构建了一个缺少“舵”的重组RNAP突变体,并在体外研究了其特性。我们的结果表明,在启动子复合物形成过程中,转录气泡的上游边界的建立不需要“舵”,新生RNA与DNA模板链的分离或转录终止也不需要“舵”。我们的结果表明,“舵”通过与新生RNA的直接相互作用对延伸复合物的稳定性做出了关键贡献。

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