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一种基于系统水平质谱的技术,可实现 RNA 帽转录组中外加修饰的 RNA 的准确和敏感定量。

A systems-level mass spectrometry-based technique for accurate and sensitive quantification of the RNA cap epitranscriptome.

机构信息

State Key Laboratory of Reproductive Regulation and Breeding of Grassland Livestock, School of Life Sciences, Inner Mongolia University, Hohhot, People's Republic of China.

Antimicrobial Resistance Interdisciplinary Research Group, Singapore-MIT Alliance for Research and Technology, Singapore, Singapore.

出版信息

Nat Protoc. 2023 Sep;18(9):2671-2698. doi: 10.1038/s41596-023-00857-0. Epub 2023 Aug 11.

Abstract

Chemical modifications of transcripts with a 5' cap occur in all organisms and function in many aspects of RNA metabolism. To facilitate analysis of RNA caps, we developed a systems-level mass spectrometry-based technique, CapQuant, for accurate and sensitive quantification of the cap epitranscriptome. The protocol includes the addition of stable isotope-labeled cap nucleotides (CNs) to RNA, enzymatic hydrolysis of endogenous RNA to release CNs, and off-line enrichment of CNs by ion-pairing high-pressure liquid chromatography, followed by a 17 min chromatography-coupled tandem quadrupole mass spectrometry run for the identification and quantification of individual CNs. The total time required for the protocol can be up to 7 d. In this approach, 26 CNs can be quantified in eukaryotic poly(A)-tailed RNA, bacterial total RNA and viral RNA. This protocol can be modified to analyze other types of RNA and RNA from in vitro sources. CapQuant stands out from other methods in terms of superior specificity, sensitivity and accuracy, and it is not limited to individual caps nor does it require radiolabeling. Thanks to its unique capability of accurately and sensitively quantifying RNA caps on a systems level, CapQuant can reveal both the RNA cap landscape and the transcription start site distribution of capped RNA in a broad range of settings.

摘要

所有生物都会对转录物进行 5' 帽结构的化学修饰,这些修饰在 RNA 代谢的多个方面发挥功能。为了便于 RNA 帽结构的分析,我们开发了一种基于系统水平的质谱技术 CapQuant,用于对帽转录组进行精确和灵敏的定量分析。该方案包括向 RNA 中添加稳定同位素标记的帽核苷酸 (CNs),用酶水解内源性 RNA 以释放 CNs,然后通过离子对高压液相色谱法离线富集 CNs,随后进行 17 分钟的色谱-串联四极杆质谱联用分析,以鉴定和定量单个 CNs。该方案总共需要长达 7 天的时间。在这种方法中,可以在真核多聚(A)尾 RNA、细菌总 RNA 和病毒 RNA 中定量 26 种 CNs。该方案可以修改以分析其他类型的 RNA 和体外来源的 RNA。CapQuant 在特异性、灵敏度和准确性方面优于其他方法,它不仅不受限于单个帽结构,也不需要放射性标记。由于其能够在系统水平上准确和灵敏地定量 RNA 帽结构的独特能力,CapQuant 可以揭示广泛条件下 RNA 帽结构的全貌和加帽 RNA 的转录起始位点分布。

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