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RET1 催化的尿苷酰化作用塑造了布氏锥虫的线粒体转录组。

RET1-catalyzed uridylylation shapes the mitochondrial transcriptome in Trypanosoma brucei.

机构信息

Department of Microbiology and Molecular Genetics, School of Medicine, University of California, Irvine, California 92697, USA.

出版信息

Mol Cell Biol. 2010 Mar;30(6):1555-67. doi: 10.1128/MCB.01281-09. Epub 2010 Jan 19.

Abstract

RNA uridylylation is critical for the expression of the mitochondrial genome in trypanosomes. Short U tails are added to guide RNAs and rRNAs, while long A/U heteropolymers mark 3' ends of most mRNAs. Three divergent mitochondrial terminal uridylyl transferases (TUTases) are known: RET1 catalyzes guide RNA (gRNA) uridylylation, RET2 executes U insertion mRNA editing, and MEAT1 associates with the editosome-like complex. However, the activities responsible for 3' uridylylation of rRNAs and mRNAs, and the roles of these modifications, are unclear. To dissect the functions of mitochondrial TUTases, we investigated the effects of their repression and overexpression on abundance, processing, 3'-end status, and in vivo stability of major mitochondrially encoded RNA classes. We show that RET1 adds U tails to gRNAs, rRNAs, and select mRNAs and contributes U's into A/U heteropolymers. Furthermore, RET1's TUTase activity is required for the nucleolytic processing of gRNA, rRNA, and mRNA precursors. The U tail's presence does not affect the stability of gRNAs and rRNAs, while transcript-specific uridylylation triggers 3' to 5' mRNA decay. We propose that the minicircle-encoded antisense transcripts, which are stabilized by RET1-catalyzed uridylylation, may direct a nucleolytic cleavage of multicistronic precursors.

摘要

RNA 尿苷酰化对于原生动物线粒体基因组的表达至关重要。短 U 尾巴被添加到指导 RNA (gRNA) 和 rRNA 上,而长的 A/U 杂聚物则标记大多数 mRNA 的 3' 端。已知有三种不同的线粒体末端尿苷酰转移酶 (TUTase):RET1 催化 gRNA 的尿苷酰化,RET2 执行 U 插入 mRNA 编辑,而 MEAT1 与编辑体样复合物相关联。然而,负责 rRNA 和 mRNA 3' 尿苷酰化的活性以及这些修饰的作用尚不清楚。为了剖析线粒体 TUTase 的功能,我们研究了它们的抑制和过表达对主要线粒体编码 RNA 类别的丰度、加工、3'-末端状态和体内稳定性的影响。我们表明,RET1 将 U 尾巴添加到 gRNA、rRNA 和选定的 mRNA 上,并将 U 插入到 A/U 杂聚物中。此外,RET1 的 TUTase 活性对于 gRNA、rRNA 和 mRNA 前体的核切割加工是必需的。U 尾巴的存在不会影响 gRNA 和 rRNA 的稳定性,而转录特异性尿苷酰化触发 3' 到 5' mRNA 降解。我们提出,由 RET1 催化的尿苷酰化稳定的迷你环编码的反义转录本可能指导多顺反子前体的核切割。

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