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LARP1 functions as a molecular switch for mTORC1-mediated translation of an essential class of mRNAs

机译:LARP1充当分子开关,用于mTORC1介导的必不可少的mRNA类翻译

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The RNA binding protein, LARP1, has been proposed to function downstream of mTORC1 to regulate the translation of 5’TOP mRNAs such as those encoding ribosome proteins (RP). However, the roles of LARP1 in the translation of 5’TOP mRNAs are controversial and its regulatory roles in mTORC1-mediated translation remain unclear. Here we show that LARP1 is a direct substrate of mTORC1 and Akt/S6K1. Deep sequencing of LARP1-bound mRNAs reveal that non-phosphorylated LARP1 interacts with both 5’ and 3’UTRs of RP mRNAs and inhibits their translation. Importantly, phosphorylation of LARP1 by mTORC1 and Akt/S6K1 dissociates it from 5’UTRs and relieves its inhibitory activity on RP mRNA translation. Concomitantly, phosphorylated LARP1 scaffolds mTORC1 on the 3’UTRs of translationally-competent RP mRNAs to facilitate mTORC1-dependent induction of translation initiation. Thus, in response to cellular mTOR activity, LARP1 serves as a phosphorylation-sensitive molecular switch for turning off or on RP mRNA translation and subsequent ribosome biogenesis.
机译:已经提出了RNA结合蛋白LARP1在mTORC1的下游起作用,以调节5'TOP mRNA的翻译,例如编码核糖体蛋白(RP)的那些。但是,LARP1在5'TOP mRNA的翻译中的作用尚有争议,其在mTORC1介导的翻译中的调控作用尚不清楚。在这里,我们显示LARP1是mTORC1和Akt / S6K1的直接底物。与LARP1结合的mRNA的深度测序表明,未磷酸化的LARP1与RP ​​mRNA的5'和3'UTR相互作用并抑制其翻译。重要的是,mTORC1和Akt / S6K1使LARP1磷酸化,使其与5'UTR分离,并减轻了其对RP mRNA翻译的抑制活性。同时,磷酸化的LARP1支架将mTORC1修饰在具有翻译能力的RP mRNA的3’UTR上,以促进mTORC1依赖性的翻译起始诱导。因此,响应细胞mTOR活性,LARP1充当磷酸化敏感性分子开关,用于关闭或开启RP mRNA翻译以及随后的核糖体生物发生。

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