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RNA编辑底物、产物及潜在中间体的定量分析:对发育调控的影响

Quantitation of RNA editing substrates, products and potential intermediates: implications for developmental regulation.

作者信息

Riley G R, Myler P J, Stuart K

机构信息

Seattle Biomedical Research Institute, WA 98109.

出版信息

Nucleic Acids Res. 1995 Feb 25;23(4):708-12. doi: 10.1093/nar/23.4.708.

DOI:10.1093/nar/23.4.708
PMID:7534910
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC306742/
Abstract

Kinetoplast mitochondrial RNA editing is the developmentally regulated post-transcriptional process of uridine insertion and deletion in mRNAs directed by short guide RNAs (gRNAs), which creates functional mRNAs. Two mechanisms are proposed: transesterification which predicts gRNA/mRNA chimeric intermediates, and enzymatic steps which allow but do not require chimeric intermediates. We quantitated the copy number of apocytochrome b (CYb) gRNAs, edited/unedited mRNAs and gRNA/mRNA chimeras in bloodstream and procyclic form cells of Trypanosoma brucei. Both forms have 35 copies/cell of two gRNAs. Bloodstream forms contain 15 unedited and edited CYb mRNA molecules/cell while procyclic forms have four times as much unedited and over 10 times as much edited mRNA. Chimera levels are very low, 350-5000-fold lower than unedited mRNA or gRNAs, but are over 10 times more abundant in procyclic than bloodstream forms. These results are consistent with chimeras being editing intermediates if their resolution is rapid in respect to their formation, although they could be non-productive byproducts of the editing reaction. Bloodstream chimera sequences differ from procyclic chimeras. These results indicate that developmental regulation is not by gRNA abundance and suggest that it occurs at the level of gRNA utilization possibly by changing abundance of unedited CYb mRNA.

摘要

动质体线粒体RNA编辑是一种在发育过程中受到调控的转录后过程,即在短引导RNA(gRNA)的指导下,对mRNA进行尿苷插入和缺失操作,从而产生功能性mRNA。目前提出了两种机制:一种是酯交换反应,该反应预测会形成gRNA/mRNA嵌合中间体;另一种是酶促步骤,该步骤允许但不要求形成嵌合中间体。我们对布氏锥虫血流形式和前循环形式细胞中的脱辅基细胞色素b(CYb)gRNA、编辑/未编辑的mRNA以及gRNA/mRNA嵌合体的拷贝数进行了定量分析。两种形式的细胞中每种gRNA均有35个拷贝/细胞。血流形式的细胞中含有15个未编辑和编辑过的CYb mRNA分子/细胞,而前循环形式细胞中的未编辑mRNA数量是其4倍,编辑过的mRNA数量则超过其10倍。嵌合体水平非常低,比未编辑的mRNA或gRNA低350 - 5000倍,但在前循环形式细胞中的丰度比血流形式细胞高10倍以上。如果嵌合体的分解相对于其形成而言很快,那么这些结果与嵌合体是编辑中间体的观点一致,尽管它们可能是编辑反应的非生产性副产物。血流形式的嵌合体序列与前循环形式的不同。这些结果表明,发育调控并非由gRNA丰度决定,而是可能通过改变未编辑CYb mRNA的丰度,在gRNA利用水平上发生。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bf92/306742/33f193d32eb9/nar00004-0178-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bf92/306742/33f193d32eb9/nar00004-0178-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bf92/306742/33f193d32eb9/nar00004-0178-a.jpg

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本文引用的文献

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J Biol Chem. 1994 Feb 25;269(8):6101-8.
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The IsTaR 1 serodeme of Trypanosoma brucei: development of a new serodeme.
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The Architecture of Trypanosoma brucei editosomes.布氏锥虫编辑体的结构
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Identification by Random Mutagenesis of Functional Domains in KREPB5 That Differentially Affect RNA Editing between Life Cycle Stages of Trypanosoma brucei.通过随机诱变鉴定布氏锥虫生命周期各阶段中对RNA编辑有不同影响的KREPB5功能结构域。
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