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Inosine modifications in human tRNAs are incorporated at the precursor tRNA level

机译:人tRNA中的肌苷修饰在前体tRNA水平上被整合

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摘要

Transfer RNAs (tRNAs) are key adaptor molecules of the genetic code that are heavily modified post-transcriptionally. Inosine at the first residue of the anticodon (position 34; I34) is an essential widespread tRNA modification that has been poorly studied thus far. The modification in eukaryotes results from a deamination reaction of adenine that is catalyzed by the heterodimeric enzyme adenosine deaminase acting on tRNA (hetADAT), composed of two subunits: ADAT2 and ADAT3. Using high-throughput small RNA sequencing (RNAseq), we show that this modification is incorporated to human tRNAs at the precursor tRNA level and during maturation. We also functionally validated the human genes encoding for hetADAT and show that the subunits of this enzyme co-localize in nucleus in an ADAT2-dependent manner. Finally, by knocking down HsADAT2, we demonstrate that variations in the cellular levels of hetADAT will result in changes in the levels of I34 modification in all its potential substrates. Altogether, we present RNAseq as a powerful tool to study post-transcriptional tRNA modifications at the precursor tRNA level and give the first insights on the biology of I34 tRNA modification in metazoans.
机译:转移RNA(tRNA)是遗传密码的关键衔接子分子,在转录后经过大量修饰。反密码子第一个残基(位置34; I34)上的肌苷是一种必需的广泛分布的tRNA修饰,到目前为止,该修饰还很少进行研究。真核生物中的修饰来自腺嘌呤的脱氨基反应,该反应由作用于tRNA的异二聚酶腺苷脱氨酶(hetADAT)催化,它由两个亚基:ADAT2和ADAT3组成。使用高通量小RNA测序(RNAseq),我们显示此修饰已在前体tRNA水平和成熟过程中整合到人tRNA中。我们还功能上验证了编码hetADAT的人类基因,并表明该酶的亚基以ADAT2依赖性方式共定位于细胞核中。最后,通过敲低HsADAT2,我们证明了hetADAT细胞水平的变化将导致其所有潜在底物中I34修饰水平的变化。总之,我们提出RNAseq是一种功能强大的工具,可以在前体tRNA水平上研究转录后tRNA的修饰,并对后生动物中I34 tRNA修饰的生物学特性提供了第一见解。

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