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AlkAniline-Seq:一种通过高通量测序同时检测 RNA 中 7-甲基鸟嘌呤(mG)和 3-甲基胞嘧啶(mC)的高灵敏度和特异性方法。

AlkAniline-Seq: A Highly Sensitive and Specific Method for Simultaneous Mapping of 7-Methyl-guanosine (mG) and 3-Methyl-cytosine (mC) in RNAs by High-Throughput Sequencing.

机构信息

Université de Lorraine, CNRS, INSERM, EpiRNASeq Core Facility, UMS2008/US40 IBSLor, Nancy, France.

Université de Lorraine, CNRS, UMR7365 IMoPA, Nancy, France.

出版信息

Methods Mol Biol. 2021;2298:77-95. doi: 10.1007/978-1-0716-1374-0_5.

Abstract

Epitranscriptomics is an emerging field where the development of high-throughput analytical technologies is essential to profile the dynamics of RNA modifications under different conditions. Despite important advances during the last 10 years, the number of RNA modifications detectable by next-generation sequencing is restricted to a very limited subset. Here, we describe a highly efficient and fast method called AlkAniline-Seq to map simultaneously two different RNA modifications: 7-methyl-guanosine (mG) and 3-methyl-cytosine (mC) in RNA. Our protocol is based on three subsequent chemical/enzymatic steps allowing the enrichment of RNA fragments ending at position n + 1 to the modified nucleotide, without any prior RNA selection. Therefore, AlkAniline-Seq demonstrates an outstanding sensitivity and specificity for these two RNA modifications. We have validated AlkAniline-Seq using bacterial, yeast, and human total RNA, and here we present, as an example, a synthetic view of the complete profiling of these RNA modifications in S. cerevisiae tRNAs.

摘要

表观转录组学是一个新兴领域,其中高通量分析技术的发展对于在不同条件下描绘 RNA 修饰的动态至关重要。尽管在过去的 10 年中取得了重要进展,但下一代测序可检测的 RNA 修饰数量仅限于非常有限的子集。在这里,我们描述了一种称为 AlkAniline-Seq 的高效快速方法,可同时对两种不同的 RNA 修饰进行定位:RNA 中的 7-甲基鸟嘌呤(mG)和 3-甲基胞嘧啶(mC)。我们的方案基于三个随后的化学/酶步骤,允许富集修饰核苷酸位置 n+1 处结束的 RNA 片段,而无需任何预先的 RNA 选择。因此,AlkAniline-Seq 对这两种 RNA 修饰具有出色的灵敏度和特异性。我们已经使用细菌、酵母和人类总 RNA 验证了 AlkAniline-Seq,并且在此我们以酿酒酵母 tRNA 中这些 RNA 修饰的完整分析为例,提供了一个综合视图。

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