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TbRGG2 促进动质体 RNA 编辑起始,并使其越过内在暂停位点进行。

TbRGG2 facilitates kinetoplastid RNA editing initiation and progression past intrinsic pause sites.

机构信息

Department of Microbiology and Immunology, University at Buffalo School of Medicine, Buffalo, New York 14214, USA.

出版信息

RNA. 2010 Nov;16(11):2239-51. doi: 10.1261/rna.2285510. Epub 2010 Sep 20.

Abstract

TbRGG2 is an essential kinetoplastid RNA editing accessory factor that acts specifically on pan-edited RNAs. To understand the mechanism of TbRGG2 action, we undertook an in-depth analysis of edited RNA populations in TbRGG2 knockdown cells and an in vitro examination of the biochemical activities of the protein. We demonstrate that TbRGG2 down-regulation more severely impacts editing at the 5' ends of pan-edited RNAs than at their 3' ends. The initiation of editing is reduced to some extent in TbRGG2 knockdown cells. In addition, TbRGG2 plays a post-initiation role as editing becomes stalled in TbRGG2-depleted cells, resulting in an overall decrease in the 3' to 5' progression of editing. Detailed analyses of edited RNAs from wild-type and TbRGG2-depleted cells reveal that TbRGG2 facilitates progression of editing past intrinsic pause sites that often correspond to the 3' ends of cognate guide RNAs (gRNAs). In addition, noncanonically edited junction regions are either absent or significantly shortened in TbRGG2-depleted cells, consistent with impaired gRNA transitions. Sequence analysis further suggests that TbRGG2 facilitates complete utilization of certain gRNAs. In vitro RNA annealing and in vivo RNA unwinding assays demonstrate that TbRGG2 can modulate RNA-RNA interactions. Collectively, these data are consistent with a model in which TbRGG2 facilitates initiation and 3' to 5' progression of editing through its ability to affect gRNA utilization, both during the transition between specific gRNAs and during usage of certain gRNAs.

摘要

TbRGG2 是一种必需的动基体 RNA 编辑辅助因子,专门作用于全编辑 RNA。为了了解 TbRGG2 作用的机制,我们对 TbRGG2 敲低细胞中的编辑 RNA 群体进行了深入分析,并对该蛋白的生化活性进行了体外检测。我们证明 TbRGG2 的下调对全编辑 RNA 的 5' 端编辑的影响比对 3' 端编辑的影响更为严重。在 TbRGG2 敲低细胞中,编辑的起始在一定程度上减少。此外,编辑在 TbRGG2 耗尽的细胞中停滞,导致编辑从 3' 到 5' 的进展总体减少,因此 TbRGG2 发挥了起始后的作用。对野生型和 TbRGG2 耗尽细胞中的编辑 RNA 进行详细分析表明,TbRGG2 促进编辑越过内在暂停位点的进展,这些暂停位点通常对应于同源向导 RNA(gRNA)的 3' 末端。此外,非规范编辑的连接区在 TbRGG2 耗尽的细胞中要么不存在,要么明显缩短,这与 gRNA 转变受损一致。序列分析进一步表明,TbRGG2 有助于某些 gRNA 的完全利用。体外 RNA 退火和体内 RNA 解链实验表明,TbRGG2 可以调节 RNA-RNA 相互作用。总的来说,这些数据与以下模型一致,即 TbRGG2 通过影响 gRNA 的利用,促进编辑的起始和 3' 到 5' 的进展,无论是在特定 gRNA 之间的转变期间还是在某些 gRNA 的使用期间。

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