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染色质富集 RNA 标记活跃和抑制的顺式调控:核 RNA-seq 分析。

Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.

机构信息

Department of Pediatrics, The University of Chicago, Chicago, Illinois, United States of America.

Department of Biological Sciences, Purdue University, West Lafayette, Indiana, United States of America.

出版信息

PLoS Comput Biol. 2020 Feb 10;16(2):e1007119. doi: 10.1371/journal.pcbi.1007119. eCollection 2020 Feb.

Abstract

Long noncoding RNAs (lncRNAs) localize in the cell nucleus and influence gene expression through a variety of molecular mechanisms. Chromatin-enriched RNAs (cheRNAs) are a unique class of lncRNAs that are tightly bound to chromatin and putatively function to locally cis-activate gene transcription. CheRNAs can be identified by biochemical fractionation of nuclear RNA followed by RNA sequencing, but until now, a rigorous analytic pipeline for nuclear RNA-seq has been lacking. In this study, we survey four computational strategies for nuclear RNA-seq data analysis and develop a new pipeline, Tuxedo-ch, which outperforms other approaches. Tuxedo-ch assembles a more complete transcriptome and identifies cheRNA with higher accuracy than other approaches. We used Tuxedo-ch to analyze benchmark datasets of K562 cells and further characterize the genomic features of intergenic cheRNA (icheRNA) and their similarity to enhancer RNAs (eRNAs). We quantify the transcriptional correlation of icheRNA and adjacent genes and show that icheRNA is more positively associated with neighboring gene expression than eRNA or cap analysis of gene expression (CAGE) signals. We also explore two novel genomic associations of cheRNA, which indicate that cheRNAs may function to promote or repress gene expression in a context-dependent manner. IcheRNA loci with significant levels of H3K9me3 modifications are associated with active enhancers, consistent with the hypothesis that enhancers are derived from ancient mobile elements. In contrast, antisense cheRNA (as-cheRNA) may play a role in local gene repression, possibly through local RNA:DNA:DNA triple-helix formation.

摘要

长链非编码 RNA(lncRNA)定位于细胞核内,并通过多种分子机制影响基因表达。富含染色质的 RNA(cheRNA)是一类独特的 lncRNA,它们与染色质紧密结合,并推测具有局部顺式激活基因转录的功能。cheRNA 可以通过核 RNA 的生化分级分离,然后进行 RNA 测序来鉴定,但到目前为止,核 RNA-seq 还缺乏严格的分析流程。在这项研究中,我们调查了四种用于核 RNA-seq 数据分析的计算策略,并开发了一种新的流程 Tuxedo-ch,它优于其他方法。Tuxedo-ch 组装了一个更完整的转录组,并比其他方法更准确地识别 cheRNA。我们使用 Tuxedo-ch 分析了 K562 细胞的基准数据集,并进一步描述了基因间 cheRNA(icheRNA)的基因组特征及其与增强子 RNA(eRNA)的相似性。我们量化了 icheRNA 和相邻基因的转录相关性,并表明 icheRNA 与相邻基因表达的正相关性高于 eRNA 或帽分析基因表达(CAGE)信号。我们还探索了 cheRNA 的两个新的基因组关联,这表明 cheRNA 可能以依赖于上下文的方式促进或抑制基因表达。具有显著 H3K9me3 修饰水平的 icheRNA 基因座与活性增强子相关,这与增强子源自古老的移动元件的假设一致。相比之下,反义 cheRNA(as-cheRNA)可能在局部基因抑制中发挥作用,可能通过局部 RNA:DNA:DNA 三螺旋形成。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0e7e/7034927/850439e389f2/pcbi.1007119.g001.jpg

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