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首页> 外文期刊>Journal of Molecular Biology >An RNA polymerase mutant deficient in DNA melting facilitates study of activation mechanism: application to an artificial activator of transcription.
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An RNA polymerase mutant deficient in DNA melting facilitates study of activation mechanism: application to an artificial activator of transcription.

机译:缺乏DNA融解的RNA聚合酶突变体有助于研究激活机制:应用于转录的人工激活剂。

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摘要

Transcription initiation is a major target for the regulation of gene expression in all organisms. Transcription activators can stimulate different steps in the initiation process including the initial binding of RNA polymerase (RNAP) to the promoter and a subsequent promoter-melting step. Typically, kinetic assays are required to determine whether an activator exerts its effect on the initial binding of RNAP or on the promoter-melting step. Here we take advantage of a mutant Escherichia coli RNAP that is deficient in promoter melting to assess the ability of an activator to stabilize the initial binding of RNAP to the promoter. For the well-characterized activator CRP, we show that this RNAP mutant can be used to distinguish between effects on initial binding and promoter melting; these results provide an independent confirmation of the results of kinetic analysis. We then employ the melting-deficient RNAP mutant to demonstrate an effect of an artificial activator of transcription on the initial binding of RNAP. Our findings demonstrate that a melting-deficient RNAP mutant can be used to trap a normally unstable intermediate in transcription initiation, thus providing a novel tool for probing activation mechanism.
机译:转录起始是调节所有生物中基因表达的主要目标。转录激活剂可以刺激启动过程中的不同步骤,包括RNA聚合酶(RNAP)与启动子的初始结合以及随后的启动子融化步骤。通常,需要进行动力学测定以确定活化剂是否对RNAP的初始结合或启动子融化步骤发挥作用。在这里,我们利用了缺乏启动子融解的突变型大肠杆菌RNAP来评估激活剂稳定RNAP与启动子的初始结合的能力。对于特征充分的激活剂CRP,我们证明了该RNAP突变体可用于区分对初始结合和启动子融化的影响。这些结果提供了动力学分析结果的独立确认。然后,我们采用熔解缺陷的RNAP突变体来证明转录的人工激活剂对RNAP初始结合的影响。我们的发现表明,熔解缺陷型RNAP突变体可用于捕获转录起始中通常不稳定的中间体,从而为探测激活机制提供了一种新颖的工具。

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