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用于氨酰化的受体茎与tRNA之间存在保守关系的证据。

Evidence for a conserved relationship between an acceptor stem and a tRNA for aminoacylation.

作者信息

Hou Y M, Sterner T, Bhalla R

机构信息

Department of Biochemistry and Molecular Biology, Thomas Jefferson University, Philadelphia, Pennsylvania 19107, USA.

出版信息

RNA. 1995 Sep;1(7):707-13.

PMID:7585255
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1369312/
Abstract

The anticodon-independent aminoacylation of RNA hairpin helices that reconstruct tRNA acceptor stems has been demonstrated for at least 10 aminoacyl-tRNA synthetases. For Escherichia coli cysteine tRNA synthetase, the specificity of aminoacylation of the acceptor stem is determined by the U73 nucleotide adjacent to the amino acid attachment site. Because U73 is present in all known cysteine tRNAs, we investigated the ability of the E. coli cystein enzyme to aminoacylate a heterologous acceptor stem. We show here that a minihelixCys based on the acceptor-T psi C stem of yeast tRNACys is a substrate for the E. coli enzyme, and that aminoacylation of this minihelix is dependent on U73. Additionally, we identify two base pairs in the acceptor stem that quantitatively convert the E. coli acceptor stem to the yeast acceptor stem. The influence of U73 and these two base pairs is completely retained in the full-length tRNA. This suggests a conserved relationship between the acceptor stem alone and the acceptor stem in the context of a tRNA for aminoacylation with cysteine. However, the primary determinant in the species-specific aminoacylation of the E. coli and yeast cysteine tRNAs is a tertiary base pair at position 15:48 outside of the acceptor stem. Although E. coli tRNACys has an unusual G15:G48 tertiary base pair, yeast tRNACys has a more common G15:C48 that prevents efficient aminoacylation of yeast tRNACys by the E. coli enzyme.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

对于至少10种氨酰-tRNA合成酶,已证实可对重构tRNA受体茎的RNA发夹螺旋进行不依赖反密码子的氨酰化。对于大肠杆菌半胱氨酸tRNA合成酶,受体茎氨酰化的特异性由与氨基酸连接位点相邻的U73核苷酸决定。由于U73存在于所有已知的半胱氨酸tRNA中,我们研究了大肠杆菌半胱氨酸酶对异源受体茎进行氨酰化的能力。我们在此表明,基于酵母tRNACys的受体-TψC茎构建的小螺旋Cys是大肠杆菌酶的底物,并且该小螺旋的氨酰化依赖于U73。此外,我们在受体茎中鉴定出两个碱基对,它们可将大肠杆菌受体茎定量转化为酵母受体茎。U73和这两个碱基对的影响在全长tRNA中完全保留。这表明单独的受体茎与tRNA背景下用于半胱氨酸氨酰化的受体茎之间存在保守关系。然而,大肠杆菌和酵母半胱氨酸tRNA物种特异性氨酰化的主要决定因素是受体茎外15:48位的三级碱基对。尽管大肠杆菌tRNACys具有不寻常的G15:G48三级碱基对,但酵母tRNACys具有更常见的G15:C48,这会阻止大肠杆菌酶对酵母tRNACys进行有效氨酰化。(摘要截短至250字)

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