首页> 外文期刊>Nucleic Acids Research >Recognition and coupling of A-to-I edited sites are determined by the tertiary structure of the RNA.
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Recognition and coupling of A-to-I edited sites are determined by the tertiary structure of the RNA.

机译:A至I编辑位点的识别和偶联取决于RNA的三级结构。

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Adenosine-to-inosine (A-to-I) editing has been shown to be an important mechanism that increases protein diversity in the brain of organisms from human to fly. The family of ADAR enzymes converts some adenosines of RNA duplexes to inosines through hydrolytic deamination. The adenosine recognition mechanism is still largely unknown. Here, to investigate it, we analyzed a set of selectively edited substrates with a cluster of edited sites. We used a large set of individual transcripts sequenced by the 454 sequencing technique. On average, we analyzed 570 single transcripts per edited region at four different developmental stages from embryogenesis to adulthood. To our knowledge, this is the first time, large-scale sequencing has been used to determine synchronous editing events. We demonstrate that edited sites are only coupled within specific distances from each other. Furthermore, our results show that the coupled sites of editing are positioned on the same side of a helix, indicating that the three-dimensional structure is key in ADAR enzyme substrate recognition. Finally, we propose that editing by the ADAR enzymes is initiated by their attraction to one principal site in the substrate.
机译:腺苷到肌苷(A到I)的编辑已被证明是一种重要的机制,可以增加生物体从人到人的大脑中蛋白质的多样性。 ADAR酶家族通过水解脱氨作用将RNA双链体的某些腺苷转化为肌苷。腺苷识别机制仍然很大程度上未知。在这里,为了对其进行调查,我们分析了一组选择性编辑的底物和一组编辑位点。我们使用了大量通过454测序技术测序的单个转录本。平均而言,我们分析了从胚胎发生到成年的四个不同发育阶段每个编辑区域的570个单转录本。据我们所知,这是第一次大规模测序用于确定同步编辑事件。我们证明,编辑后的站点仅在彼此之间的特定距离内耦合。此外,我们的结果表明,编辑的耦合位点位于螺旋的同一侧,表明三维结构是ADAR酶底物识别的关键。最后,我们建议通过ADAR酶对底物一个主要位点的吸引来启动编辑。

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