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Activation mode of the eukaryotic m2G10 tRNA methyltransferase Trm11 by its partner protein Trm112

机译:真核m2G10 tRNA甲基转移酶Trm11被其伴侣蛋白Trm112激活的模式。

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摘要

Post-transcriptional and post-translational modifications of factors involved in translation are very important for the control and accuracy of protein biosynthesis. Among these factors, tRNAs harbor the largest variety of grafted chemical structures, which participate in tRNA stability or mRNA decoding. Here, we focused on Trm112 protein, which associates with four different eukaryotic methyltransferases modifying tRNAs (Trm9 and Trm11) but also 18S-rRNA (Bud23) and translation termination factor eRF1 (Mtq2). In particular, we have investigated the role of Trm112 in the Trm11–Trm112 complex, which forms 2-methylguanosine at position 10 on several tRNAs and thereby is assumed to stabilize tRNA structure. We show that Trm112 is important for Trm11 enzymatic activity by influencing S-adenosyl-L-methionine binding and by contributing to tRNA binding. Using hydrogen-deuterium eXchange coupled to mass spectrometry, we obtained experimental evidences that the Trm11–Trm112 interaction relies on the same molecular bases as those described for other Trm112–methyltransferases complexes. Hence, all Trm112-dependent methyltransferases compete to interact with this partner.
机译:转录后和翻译后修饰因子的翻译对于蛋白质生物合成的控制和准确性非常重要。在这些因素中,tRNA包含最多种类的嫁接化学结构,这些结构参与tRNA稳定性或mRNA解码。在这里,我们专注于Trm112蛋白,该蛋白与修饰tRNA的四个不同的真核甲基转移酶(Trm9和Trm11)以及18S-rRNA(Bud23)和翻译终止因子eRF1(Mtq2)相关。特别是,我们研究了Trm112在Trm11–Trm112复合物中的作用,该复合物在几种tRNA的第10位形成2-甲基鸟苷,因此被认为可以稳定tRNA的结构。我们显示,Trm112通过影响S-腺苷-L-甲硫氨酸结合并促进tRNA结合,对Trm11酶活性很重要。使用氢-氘交换与质谱联用,我们获得了实验证据,表明Trm11–Trm112相互作用与其他Trm112–甲基转移酶复合物所描述的分子基础相同。因此,所有Trm112依赖性甲基转移酶竞争与该伴侣相互作用。

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