首页> 美国卫生研究院文献>Nucleic Acids Research >Efficient cleavage of pre-tRNAs by E. coli RNAse P RNA requires the 2-hydroxyl of the ribose at the cleavage site.
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Efficient cleavage of pre-tRNAs by E. coli RNAse P RNA requires the 2-hydroxyl of the ribose at the cleavage site.

机译:大肠杆菌RNA酶P RNA对pre-tRNA的有效切割需要在切割位点具有核糖的2-羟基。

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摘要

RNAse P cleaves pre-tRNAs to liberate 5'-flanks and 5'-matured, 5'-phosphorylated tRNAs. It is not evident if the 2'-hydroxyls of the ribose moieties in the substrate are involved in the reaction. To study their influence in two different pre-tRNAs, we have modified specifically the 2'-hydroxyl groups at the cleavage site and in neighbouring positions. We have shown that these hydroxyls are important but not essential for the processing of these substrates by E. coli RNase P RNA (M1 RNA). The reduction in the catalytic efficiency was moderate for 2'-deoxy and severe for 2'-methoxy substitutions at the cleavage site. Additional effects of modifications in neighbouring positions were smaller. Based on our data we suggest that the modifications do not interfere with binding of the substrate, whereas they prevent an optimal steric arrangement for the hydrolysis reaction.
机译:RNAse P裂解pre-tRNA释放5'-侧翼和5'-成熟的5'-磷酸化tRNA。尚不清楚底物中核糖部分的2'-羟基是否参与反应。为了研究它们在两个不同的pre-tRNA中的影响,我们专门修饰了切割位点和邻近位置的2'-羟基。我们已经表明,这些羟基对于大肠杆菌RNase P RNA(M1 RNA)加工这些底物很重要,但不是必需的。对于2'-脱氧,催化效率的降低是中等的,对于裂解位点的2'-甲氧基取代的催化效率的降低是严重的。相邻位置修饰的附加影响较小。根据我们的数据,我们建议修饰不会干扰底物的结合,而会阻止水解反应的最佳空间排列。

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