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NusA刺激的RNA聚合酶暂停和终止参与枯草芽孢杆菌色氨酸操纵子的体外衰减机制。

NusA-stimulated RNA polymerase pausing and termination participates in the Bacillus subtilis trp operon attenuation mechanism invitro.

作者信息

Yakhnin Alexander V, Babitzke Paul

机构信息

Department of Biochemistry and Molecular Biology, Pennsylvania State University, University Park, PA 16802, USA.

出版信息

Proc Natl Acad Sci U S A. 2002 Aug 20;99(17):11067-72. doi: 10.1073/pnas.162373299. Epub 2002 Aug 2.

Abstract

The trp RNA-binding attenuation protein (TRAP) regulates expression of the Bacillus subtilis trpEDCFBA operon by transcription attenuation and translation control mechanisms. Both mechanisms require the binding of tryptophan-activated TRAP to the 11 (G/U)AG-repeat segment in the trp leader transcript. To promote termination, TRAP must bind to the nascent RNA before the antiterminator structure forms. Because only 20 nucleotides separate the TRAP-binding site from the 3' end of the antiterminator, TRAP has a short time frame to control this regulatory decision. Synchronization of factor binding and/or RNA folding with the RNA polymerase position is a major challenge in all attenuation mechanisms. Because RNA polymerase pausing allows this synchronization in many attenuation mechanisms, we performed experiments in vitro to determine whether pausing participates in the B. subtilis trp attenuation mechanism. We identified two NusA-stimulated pause sites in the trp leader region. Formation of pause hairpins participates in pausing at both positions. The first pause occurred at the nucleotide just preceding the critical overlap between the alternative antiterminator and terminator structures. TRAP binding to transcripts containing preexisting pause complexes releases RNA polymerase, suggesting that pausing provides additional time for TRAP to bind and promote termination. The second pause is downstream from the trp leader termination point, raising the possibility that this pause event participates in the trpE translation control mechanism. NusA also increases the efficiency of termination in the trp leader region and shifts termination one nucleotide upstream. Finally, NusA-stimulated termination is cooperative, suggesting that binding of multiple NusA molecules influences termination.

摘要

色氨酸RNA结合衰减蛋白(TRAP)通过转录衰减和翻译控制机制调节枯草芽孢杆菌trpEDCFBA操纵子的表达。这两种机制都需要色氨酸激活的TRAP与trp前导转录本中的11个(G/U)AG重复序列结合。为了促进终止,TRAP必须在抗终止子结构形成之前与新生RNA结合。由于TRAP结合位点与抗终止子的3'端仅相隔20个核苷酸,TRAP控制这一调节决定的时间框架很短。在所有衰减机制中,因子结合和/或RNA折叠与RNA聚合酶位置的同步是一个主要挑战。由于在许多衰减机制中RNA聚合酶暂停允许这种同步,我们进行了体外实验以确定暂停是否参与枯草芽孢杆菌trp衰减机制。我们在trp前导区域鉴定出两个NusA刺激的暂停位点。暂停发夹的形成参与了两个位置的暂停。第一个暂停发生在替代抗终止子和终止子结构之间关键重叠之前的核苷酸处。TRAP与含有预先存在的暂停复合物的转录本结合会释放RNA聚合酶,这表明暂停为TRAP结合并促进终止提供了额外的时间。第二个暂停位于trp前导终止点的下游,增加了这种暂停事件参与trpE翻译控制机制的可能性。NusA还提高了trp前导区域的终止效率,并使终止向上游移动了一个核苷酸。最后,NusA刺激的终止是协同的,这表明多个NusA分子的结合会影响终止。

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