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动质体线粒体中的RNA编辑

RNA editing in kinetoplastid mitochondria.

作者信息

Hajduk S L, Harris M E, Pollard V W

机构信息

Department of Biochemistry, School of Medicine, University of Alabama, Birmingham 35294.

出版信息

FASEB J. 1993 Jan;7(1):54-63. doi: 10.1096/fasebj.7.1.8422975.

DOI:10.1096/fasebj.7.1.8422975
PMID:8422975
Abstract

RNA editing in the mitochondrion of kinetoplastid protozoa results in the posttranscriptional addition and deletion of uridine residues in mRNAs. Editing of mRNAs can lead to the formation of initiation codons for mitochondrial translation, the correction of frame-shifted genes at the RNA level, and in extensively edited mRNAs, the formation of complete reading frames. Kinetoplastid RNA editing requires that genetic information from two or more separately transcribed genes be brought together to form the mature, edited mRNA. The information necessary for the proper insertion or deletion of uridines in the mRNA is present in small mitochondrial transcripts termed guide RNAs (gRNAs). Editing of mRNAs appears to be associated with a high molecular weight complex, called the editosome, containing specific gRNAs, unedited mRNAs, and proteins. Editing is likely a two-step process involving first the breakage of a phosphodiester bond at the editing site and formation of a chimeric molecule with a gRNA covalently joined to the 5' end of the 3' portion of an mRNA. The chimera is resolved by the rejoining of the 5' end of the mRNA to the 3' portion of the mRNA with the addition or deletion of a uridine at the junction point. Two models are proposed for the biochemical mechanism of RNA editing. The first is an enzymatic cascade of cleavage and ligation while the other supports successive rounds of transesterification. The obvious functional necessity for editing in kinetoplastid mitochondria is the formation of translatable mRNAs. Far less clear is the evolutionary origin of editing and the role editing plays in regulating mitochondrial gene expression.

摘要

动质体原生动物线粒体中的RNA编辑导致mRNA转录后尿苷残基的添加和缺失。mRNA的编辑可导致线粒体翻译起始密码子的形成、在RNA水平上对移码基因的校正,以及在经过广泛编辑的mRNA中形成完整的阅读框。动质体RNA编辑要求来自两个或更多个单独转录基因的遗传信息聚集在一起,以形成成熟的、经过编辑的mRNA。mRNA中尿苷正确插入或缺失所需的信息存在于称为引导RNA(gRNA)的线粒体小转录本中。mRNA的编辑似乎与一种高分子量复合物有关,这种复合物称为编辑体,包含特定的gRNA、未编辑的mRNA和蛋白质。编辑可能是一个两步过程,首先是在编辑位点处磷酸二酯键的断裂,并形成一个与gRNA共价连接到mRNA 3'部分5'端的嵌合分子。通过将mRNA的5'端与mRNA的3'部分重新连接,并在连接点处添加或缺失一个尿苷来解析该嵌合体。针对RNA编辑的生化机制提出了两种模型。第一种是切割和连接的酶促级联反应,而另一种支持连续的转酯反应轮次。动质体线粒体中编辑的明显功能必要性是形成可翻译的mRNA。编辑的进化起源以及编辑在调节线粒体基因表达中所起的作用则远没有那么清楚。

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RNA editing in kinetoplastid mitochondria.动质体线粒体中的RNA编辑
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