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枯草芽孢杆菌tyrS基因转录抗终止的tRNA决定因素。

tRNA determinants for transcription antitermination of the Bacillus subtilis tyrS gene.

作者信息

Grundy F J, Collins J A, Rollins S M, Henkin T M

机构信息

Department of Microbiology, The Ohio State University, Columbus 43210, USA.

出版信息

RNA. 2000 Aug;6(8):1131-41. doi: 10.1017/s1355838200992100.

Abstract

Transcriptional regulation of the T box family of aminoacyl-tRNA synthetase and amino acid biosynthesis genes in Gram-positive bacteria is mediated by a conserved transcription antitermination system, in which readthrough of a termination site in the leader region of the mRNA is directed by a specific interaction with the cognate uncharged tRNA. The specificity of this interaction is determined in part by pairing of the anticodon of the tRNA with a "specifier sequence" in the leader, a codon representing the appropriate amino acid, as well as by pairing of the acceptor end of the tRNA with an unpaired region of the antiterminator. Previous studies have indicated that although these interactions are necessary for antitermination, they are unlikely to be sufficient. In the current study, the effect of multiple mutations in tRNA(Tyr) on readthrough of the tyrS leader region terminator, independent of other tRNA functions, was assessed using a system for in vivo expression of pools of tRNA variants; this system may be generally useful for in vivo expression of RNAs with defined end points. Although alterations in helical regions of tRNA(Tyr) that did not perturb base pairing were generally permitted, substitutions affecting conserved features of tRNAs were not. The long variable arm of tRNA(Tyr) could be replaced by either a short variable arm or a long insertion of a stable stem-loop structure. These results indicate that the tRNA-leader RNA interaction is highly constrained, and is likely to involve recognition of the overall tertiary structure of the tRNA.

摘要

革兰氏阳性菌中氨酰 - tRNA合成酶T盒家族和氨基酸生物合成基因的转录调控由一个保守的转录抗终止系统介导,在该系统中,mRNA前导区终止位点的通读是由与同源无电荷tRNA的特异性相互作用引导的。这种相互作用的特异性部分由tRNA的反密码子与前导区的“指定序列”(代表相应氨基酸的密码子)配对决定,也由tRNA的受体端与抗终止子的未配对区域配对决定。先前的研究表明,虽然这些相互作用对于抗终止是必要的,但它们不太可能是充分的。在当前研究中,使用一个用于体内表达tRNA变体库的系统,评估了tRNA(Tyr)中的多个突变对tyrS前导区终止子通读的影响,该系统独立于其他tRNA功能;这个系统可能普遍适用于体内表达具有确定端点的RNA。虽然一般允许tRNA(Tyr)螺旋区域中不干扰碱基配对的改变,但影响tRNA保守特征的替代则不被允许。tRNA(Tyr)的长可变臂可以被短可变臂或稳定茎环结构的长插入所取代。这些结果表明,tRNA - 前导RNA相互作用受到高度限制,并且可能涉及对tRNA整体三级结构的识别。

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