Untacking small RNA profiling and RNA fragment footprinting: Approaches and challenges in library construction.

IF 6.4 2区 生物学 Q1 CELL BIOLOGY Wiley Interdisciplinary Reviews: RNA Pub Date : 2024-05-01 DOI:10.1002/wrna.1852
Zhaokang Shen, Muhammad Naveed, Jianqiang Bao
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Abstract

Small RNAs (sRNAs) with sizes ranging from 15 to 50 nucleotides (nt) are critical regulators of gene expression control. Prior studies have shown that sRNAs are involved in a broad range of biological processes, such as organ development, tumorigenesis, and epigenomic regulation; however, emerging evidence unveils a hidden layer of diversity and complexity of endogenously encoded sRNAs profile in eukaryotic organisms, including novel types of sRNAs and the previously unknown post-transcriptional RNA modifications. This underscores the importance for accurate, unbiased detection of sRNAs in various cellular contexts. A multitude of high-throughput methods based on next-generation sequencing (NGS) are developed to decipher the sRNA expression and their modifications. Nonetheless, distinct from mRNA sequencing, the data from sRNA sequencing suffer frequent inconsistencies and high variations emanating from the adapter contaminations and RNA modifications, which overall skew the sRNA libraries. Here, we summarize the sRNA-sequencing approaches, and discuss the considerations and challenges for the strategies and methods of sRNA library construction. The pros and cons of sRNA sequencing have significant implications for implementing RNA fragment footprinting approaches, including CLIP-seq and Ribo-seq. We envision that this review can inspire novel improvements in small RNA sequencing and RNA fragment footprinting in future. This article is categorized under: RNA Evolution and Genomics > Computational Analyses of RNA RNA Processing > Processing of Small RNAs Regulatory RNAs/RNAi/Riboswitches > Biogenesis of Effector Small RNAs.

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解开小 RNA 分析和 RNA 片段足迹:文库构建的方法和挑战。
大小为 15 至 50 个核苷酸(nt)的小核糖核酸(sRNA)是基因表达控制的关键调节因子。先前的研究表明,sRNAs 参与了器官发育、肿瘤发生和表观基因组调控等广泛的生物过程;然而,新出现的证据揭示了真核生物内源性编码的 sRNAs 的多样性和复杂性,包括新型 sRNAs 和先前未知的转录后 RNA 修饰。这凸显了在各种细胞环境中准确、无偏见地检测 sRNA 的重要性。目前已开发出多种基于下一代测序(NGS)的高通量方法来解读 sRNA 的表达及其修饰。然而,与 mRNA 测序不同的是,sRNA 测序的数据经常出现不一致和高变异,这源于适配器污染和 RNA 修饰,它们在整体上歪曲了 sRNA 文库。在此,我们总结了 sRNA 测序方法,并讨论了 sRNA 文库构建策略和方法的注意事项和挑战。sRNA 测序的利弊对实施 RNA 片段足迹分析方法(包括 CLIP-seq 和 Ribo-seq)具有重要影响。我们希望这篇综述能为今后小 RNA 测序和 RNA 片段足迹分析带来新的启发。本文归类于RNA 进化与基因组学 > RNA 的计算分析 RNA 处理 > 小 RNAs 的处理 调控 RNAs/RNAi/Riboswitches > 效应小 RNAs 的生物发生。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
CiteScore
14.80
自引率
4.10%
发文量
67
审稿时长
6-12 weeks
期刊介绍: WIREs RNA aims to provide comprehensive, up-to-date, and coherent coverage of this interesting and growing field, providing a framework for both RNA experts and interdisciplinary researchers to not only gain perspective in areas of RNA biology, but to generate new insights and applications as well. Major topics to be covered are: RNA Structure and Dynamics; RNA Evolution and Genomics; RNA-Based Catalysis; RNA Interactions with Proteins and Other Molecules; Translation; RNA Processing; RNA Export/Localization; RNA Turnover and Surveillance; Regulatory RNAs/RNAi/Riboswitches; RNA in Disease and Development; and RNA Methods.
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