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在深度转录组数据集中对RNA编辑进行定量分析。

Quantifying RNA Editing in Deep Transcriptome Datasets.

作者信息

Lo Giudice Claudio, Silvestris Domenico Alessandro, Roth Shalom Hillel, Eisenberg Eli, Pesole Graziano, Gallo Angela, Picardi Ernesto

机构信息

Institute of Biomembranes, Bioenergetics and Molecular Biotechnologies, National Research Council, Bari, Italy.

RNA Editing Lab, Oncohaematology Department, IRCCS Ospedale Pediatrico "Bambino Gesù," Rome, Italy.

出版信息

Front Genet. 2020 Mar 6;11:194. doi: 10.3389/fgene.2020.00194. eCollection 2020.

Abstract

Massive transcriptome sequencing through the RNAseq technology has enabled quantitative transcriptome-wide investigation of co-/post-transcriptional mechanisms such as alternative splicing and RNA editing. The latter is abundant in human transcriptomes in which million adenosines are deaminated into inosines by the ADAR enzymes. RNA editing modulates the innate immune response and its deregulation has been associated with different human diseases including autoimmune and inflammatory pathologies, neurodegenerative and psychiatric disorders, and tumors. Accurate profiling of RNA editing using deep transcriptome data is still a challenge, and the results depend strongly on processing and alignment steps taken. Accurate calling of the inosinome repertoire, however, is required to reliably quantify RNA editing and, in turn, investigate its biological and functional role across multiple samples. Using real RNAseq data, we demonstrate the impact of different bioinformatics steps on RNA editing detection and describe the main metrics to quantify its level of activity.

摘要

通过RNAseq技术进行的大规模转录组测序,使得对共转录/转录后机制(如可变剪接和RNA编辑)进行全转录组范围的定量研究成为可能。RNA编辑在人类转录组中很常见,其中数百万个腺苷被ADAR酶脱氨基变成肌苷。RNA编辑调节先天免疫反应,其失调与包括自身免疫和炎症性疾病、神经退行性和精神疾病以及肿瘤在内的多种人类疾病有关。使用深度转录组数据对RNA编辑进行准确的分析仍然是一个挑战,其结果在很大程度上取决于所采取的处理和比对步骤。然而,为了可靠地量化RNA编辑,并进而研究其在多个样本中的生物学和功能作用,需要准确地识别肌苷组库。利用真实的RNAseq数据,我们展示了不同生物信息学步骤对RNA编辑检测的影响,并描述了量化其活性水平的主要指标。

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