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Transcript cleavage factors GreA and GreB act as transient catalytic components of RNA polymerase

机译:转录裂解因子GreA和GreB充当RNA聚合酶的瞬时催化成分

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摘要

Prokaryotic transcription elongation factors GreA and GreB stimulate intrinsic nucleolytic activity of RNA polymerase (RNAP). The proposed biological role of Gre-induced RNA hydrolysis includes transcription proofreading, suppression of transcriptional pausing and arrest, and facilitation of RNAP transition from transcription initiation to transcription elongation. Using an array of biochemical and molecular genetic methods, we mapped the interaction interface between Gre and RNAP and identified the key residues in Gre responsible for induction of nucleolytic activity in RNAP. We propose a structural model in which the C-terminal globular domain of Gre binds near the opening of the RNAP secondary channel, the N-terminal coiled-coil domain (NTD) protrudes inside the RNAP channel, and the tip of the NTD is brought to the immediate vicinity of RNAP catalytic center. Two conserved acidic residues D41 and E44 located at the tip of the NTD assist RNAP by coordinating the Mg2+ ion and water molecule required for catalysis of RNA hydrolysis. If so, Gre would be the first transcription factor known to directly participate in the catalytic act of RNAP.
机译:原核转录延伸因子GreA和GreB刺激RNA聚合酶(RNAP)的内在核酸溶解活性。 Gre诱导的RNA水解的拟议生物学作用包括转录校对,抑制转录暂停和停滞以及促进RNAP从转录起始到转录延伸的过渡。使用一系列生化和分子遗传学方法,我们绘制了Gre和RNAP之间的相互作用界面,并鉴定了Gre中负责诱导RNAP溶核活性的关键残基。我们提出了一个结构模型,其中Gre的C端球状结构域在RNAP二级通道的开口附近结合,N端螺旋结构域(NTD)突出到RNAP通道内,并且NTD的尖端被带入到RNAP催化中心附近。位于NTD末端的两个保守的酸性残基D41和E44通过协调催化RNA水解所需的Mg 2 + 离子和水分子来辅助RNAP。如果是这样,Gre将是已知直接参与RNAP催化作用的第一个转录因子。

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