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酵母快速 tRNA 降解途径与延伸因子 1A 竞争底物 tRNA,并作用于缺少一种或多种修饰的 tRNA。

The yeast rapid tRNA decay pathway competes with elongation factor 1A for substrate tRNAs and acts on tRNAs lacking one or more of several modifications.

机构信息

Department of Biochemistry and Biophysics, Center for RNA Biology, University of Rochester School of Medicine, Rochester, New York 14642, USA.

出版信息

RNA. 2012 Oct;18(10):1886-96. doi: 10.1261/rna.033654.112. Epub 2012 Aug 15.

DOI:10.1261/rna.033654.112
PMID:22895820
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3446711/
Abstract

The structural and functional integrity of tRNA is crucial for translation. In the yeast Saccharomyces cerevisiae, certain aberrant pre-tRNA species are subject to nuclear surveillance, leading to 3' exonucleolytic degradation, and certain mature tRNA species are subject to rapid tRNA decay (RTD) if they are appropriately hypomodified or bear specific destabilizing mutations, leading to 5'-3' exonucleolytic degradation by Rat1 and Xrn1. Thus, trm8-Δ trm4-Δ strains are temperature sensitive due to lack of m(7)G(46) and m(5)C and the consequent RTD of tRNA(Val(AAC)), and tan1-Δ trm44-Δ strains are temperature sensitive due to lack of ac(4)C(12) and Um(44) and the consequent RTD of tRNA(Ser(CGA)) and tRNA(Ser(UGA)). It is unknown how the RTD pathway interacts with translation and other cellular processes, and how generally this pathway acts on hypomodified tRNAs. We provide evidence here that elongation factor 1A (EF-1A) competes with the RTD pathway for substrate tRNAs, since its overexpression suppresses the tRNA degradation and the growth defect of strains subject to RTD, whereas reduced levels of EF-1A have the opposite effect. We also provide evidence that RTD acts on a variety of tRNAs lacking one or more different modifications, since trm1-Δ trm4-Δ mutants are subject to RTD of tRNA(Ser(CGA)) and tRNA(Ser(UGA)) due to lack of m(2,2)G(26) and m(5)C, and since trm8-Δ, tan1-Δ, and trm1-Δ single mutants are each subject to RTD. These results demonstrate that RTD interacts with the translation machinery and acts widely on hypomodified tRNAs.

摘要

tRNA 的结构和功能完整性对于翻译至关重要。在酵母酿酒酵母中,某些异常的前 tRNA 物种会受到核监测,导致 3'外切核酸酶降解,如果成熟的 tRNA 物种适当低修饰或携带特定的不稳定突变,则会受到快速 tRNA 降解(RTD),导致 Rat1 和 Xrn1 的 5'-3'外切核酸酶降解。因此,trm8-Δ trm4-Δ 菌株由于缺乏 m(7)G(46)和 m(5)C,以及随后的 tRNA(Val(AAC))的 RTD,以及 tan1-Δ trm44-Δ 菌株由于缺乏 ac(4)C(12)和 Um(44),以及随后的 tRNA(Ser(CGA))和 tRNA(Ser(UGA))的 RTD,因此对温度敏感。目前尚不清楚 RTD 途径如何与翻译和其他细胞过程相互作用,以及该途径通常如何作用于低修饰的 tRNA。我们在这里提供的证据表明,延伸因子 1A(EF-1A)与 RTD 途径竞争底物 tRNA,因为其过表达可抑制 RTD 菌株的 tRNA 降解和生长缺陷,而 EF-1A 水平降低则具有相反的效果。我们还提供了证据表明 RTD 作用于多种缺乏一种或多种不同修饰的 tRNA,因为 trm1-Δ trm4-Δ 突变体由于缺乏 m(2,2)G(26)和 m(5)C,因此受到 RTD 的影响 tRNA(Ser(CGA))和 tRNA(Ser(UGA)),并且 trm8-Δ、tan1-Δ 和 trm1-Δ 单突变体各自受到 RTD 的影响。这些结果表明,RTD 与翻译机制相互作用,并广泛作用于低修饰的 tRNA。

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tRNAs marked with CCACCA are targeted for degradation.带有 CCACCA 标记的 tRNA 被靶向降解。
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The yeast rapid tRNA decay pathway primarily monitors the structural integrity of the acceptor and T-stems of mature tRNA.酵母快速 tRNA 降解途径主要监测成熟 tRNA 的接受体和 T 茎的结构完整性。
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