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含有脱氧核糖核苷酸的tRNA转录物的结构及氨酰化能力

Structure and aminoacylation capacities of tRNA transcripts containing deoxyribonucleotides.

作者信息

Aphasizhev R, Théobald-Dietrich A, Kostyuk D, Kochetkov S N, Kisselev L, Giegé R, Fasiolo F

机构信息

UPR 9002, IBMC du CNRS, Strasbourg, France.

出版信息

RNA. 1997 Aug;3(8):893-904.

PMID:9257648
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1369534/
Abstract

The contribution of the ribose 2'-hydroxyls to RNA structure and function has been analyzed, but still remains controversial. In this work, we report the use of a mutant T7 RNA polymerase as a tool in RNA studies, applied to the aspartate and methionine tRNA aminoacylation systems from yeast. Our approach consists of determining the effect of substituting natural ribonucleotides by deoxyribonucleotides in RNA and, thereby, defining the subset of important 2'-hydroxyl groups. We show that deoxyribose-containing RNA can be folded in a global conformation similar to that of natural RNA. Melting curves of tRNAs, obtained by temperature-gradient gel electrophoresis, indicate that in deoxyribo-containing molecules, the thermal stability of the tertiary network drops down, whereas the stability of the secondary structure remains unaltered. Nuclease footprinting reveals a significant increase in the accessibility of both single- and double-stranded regions. As to the functionality of the deoxyribose-containing tRNAs, their in vitro aminoacylation efficiency indicates striking differential effects depending upon the nature of the substituted ribonucleotides. Strongest decrease in charging occurs for yeast initiator tRNA(Met) transcripts containing dG or dC residues and for yeast tRNA(Asp) transcripts with dU or dG. In the aspartate system, the decreased aminoacylation capacities can be correlated with the substitution of the ribose moieties of U11 and G27, disrupting two hydrogen bond contacts with the synthetase. Altogether, this suggests that specific 2'-hydroxyl groups in tRNAs can act as determinants specifying aminoacylation identity.

摘要

核糖2'-羟基对RNA结构和功能的贡献已得到分析,但仍存在争议。在这项工作中,我们报告了使用突变型T7 RNA聚合酶作为RNA研究工具,应用于酵母的天冬氨酸和甲硫氨酸tRNA氨基酰化系统。我们的方法包括确定用脱氧核糖核苷酸取代RNA中的天然核糖核苷酸的效果,从而确定重要的2'-羟基基团子集。我们表明,含脱氧核糖的RNA可以折叠成与天然RNA相似的整体构象。通过温度梯度凝胶电泳获得的tRNA熔解曲线表明,在含脱氧核糖的分子中,三级网络的热稳定性下降,而二级结构的稳定性保持不变。核酸酶足迹分析显示单链和双链区域的可及性显著增加。至于含脱氧核糖的tRNA的功能,它们的体外氨基酰化效率表明,根据取代的核糖核苷酸的性质,存在显著的差异效应。对于含有dG或dC残基的酵母起始tRNA(Met)转录本以及含有dU或dG的酵母tRNA(Asp)转录本,电荷的下降最为明显。在天冬氨酸系统中,氨基酰化能力的下降与U11和G27核糖部分的取代相关,这破坏了与合成酶的两个氢键接触。总之,这表明tRNA中特定的2'-羟基基团可以作为决定氨基酰化特异性的因素。