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Detection and Analysis of RNA Ribose 2′-O-Methylations: Challenges and Solutions

机译:RNA核糖2-O-甲基化的检测和分析:挑战和解决方案

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摘要

Ribose 2′-O-methylation is certainly one of the most common RNA modifications found in almost any type of cellular RNA. It decorates transfer RNAs (tRNAs), ribosomal RNAs (rRNAs), small nuclear RNAs (snRNAs) (and most probably small nucleolar RNAs, snoRNAs), as well as regulatory RNAs like microRNAs (miRNAs) and Piwi-interacting RNAs (piRNAs), and finally, eukaryotic messenger RNAs (mRNAs). Due to this exceptional widespread of RNA 2′-O-methylation, considerable efforts were made in order to precisely map these numerous modifications. Extensive studies of RNA 2′-O-methylation were also stimulated by the discovery of C/D-box snoRNA-guided machinery, which insures site-specific modification of hundreds 2′-O-methylated residues in archaeal and eukaryotic rRNAs and some other RNAs. In this brief review we discussed both traditional approaches of RNA biochemistry and also modern deep sequencing-based methods, used for detection/mapping and quantification of RNA 2′-O-methylations.
机译:核糖2'-O-甲基化无疑是几乎在任何类型的细胞RNA中发现的最常见的RNA修饰之一。它修饰了转移RNA(tRNA),核糖体RNA(rRNA),小核RNA(snRNA)(以及最有可能的小核仁RNA,snoRNA)以及调节性RNA,例如microRNA(miRNA)和与Piwi相互作用的RNA(piRNA),最后是真核信使RNA(mRNA)。由于RNA 2'-O-甲基化的这种异常广泛的传播,人们做出了巨大的努力,以精确地绘制这些众多的修饰。 C / D-box snoRNA引导的机制的发现也刺激了对RNA 2'-O-甲基化的广泛研究,该机制确保了古细菌和真核rRNA等数百个2'-O-甲基化残基的位点特异性修饰。 RNA。在这篇简短的综述中,我们讨论了RNA生物化学的传统方法以及基于深度测序的现代方法,这些方法用于检测/映射和定量RNA 2'-O-甲基化。

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