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一个5'RNA茎环参与转录衰减机制,该机制控制枯草芽孢杆菌trpEDCFBA操纵子的表达。

A 5' RNA stem-loop participates in the transcription attenuation mechanism that controls expression of the Bacillus subtilis trpEDCFBA operon.

作者信息

Sudershana S, Du H, Mahalanabis M, Babitzke P

机构信息

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

出版信息

J Bacteriol. 1999 Sep;181(18):5742-9. doi: 10.1128/JB.181.18.5742-5749.1999.

Abstract

The trp RNA-binding attenuation protein (TRAP) regulates expression of the Bacillus subtilis trpEDCFBA operon by transcription attenuation. Tryptophan-activated TRAP binds to the nascent trp leader transcript by interacting with 11 (G/U)AG repeats. TRAP binding prevents formation of an antiterminator structure, thereby promoting formation of an overlapping terminator, and hence transcription is terminated before RNA polymerase can reach the trp structural genes. In addition to the antiterminator and terminator, a stem-loop structure is predicted to form at the 5' end of the trp leader transcript. Deletion of this structure resulted in a dramatic increase in expression of a trpE'-'lacZ translational fusion and a reduced ability to regulate expression in response to tryptophan. By introducing a series of point mutations in the 5' stem-loop, we found that both the sequence and the structure of the hairpin are important for its regulatory function and that compensatory changes that restored base pairing partially restored wild-type-like expression levels. Our results indicate that the 5' stem-loop functions primarily through the TRAP-dependent regulatory pathway. Gel shift results demonstrate that the 5' stem-loop increases the affinity of TRAP for trp leader RNA four- to fivefold, suggesting that the 5' structure interacts with TRAP. In vitro transcription results indicate that this 5' structure functions in the attenuation mechanism, since deletion of the stem-loop caused an increase in transcription readthrough. An oligonucleotide complementary to a segment of the 5' stem-loop was used to demonstrate that formation of the 5' structure is required for proper attenuation control of this operon.

摘要

色氨酸RNA结合衰减蛋白(TRAP)通过转录衰减来调控枯草芽孢杆菌trpEDCFBA操纵子的表达。色氨酸激活的TRAP通过与11个(G/U)AG重复序列相互作用,与新生的trp前导转录本结合。TRAP的结合会阻止抗终止子结构的形成,从而促进重叠终止子的形成,因此转录在RNA聚合酶到达trp结构基因之前就会终止。除了抗终止子和终止子外,预计在trp前导转录本的5'端会形成一个茎环结构。删除该结构会导致trpE'-'lacZ翻译融合体的表达显著增加,并降低了响应色氨酸调节表达的能力。通过在5'茎环中引入一系列点突变,我们发现发夹的序列和结构对其调节功能都很重要,并且恢复碱基配对的补偿性变化部分恢复了野生型样的表达水平。我们的结果表明,5'茎环主要通过TRAP依赖的调节途径发挥作用。凝胶迁移结果表明,5'茎环使TRAP对trp前导RNA的亲和力提高了四到五倍,这表明5'结构与TRAP相互作用。体外转录结果表明,这种5'结构在衰减机制中起作用,因为删除茎环会导致转录通读增加。使用与5'茎环的一段互补的寡核苷酸来证明5'结构的形成对于该操纵子的适当衰减控制是必需的。

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