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

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

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....

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Main Authors: Xiangying Sun, Zhezhen Wang, Johnathon M Hall, Carlos Perez-Cervantes, Alexander J Ruthenburg, Ivan P Moskowitz, Michael Gribskov, Xinan H Yang
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2020-02-01
Series:PLoS Computational Biology
Online Access:https://doi.org/10.1371/journal.pcbi.1007119
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spelling doaj-051a23354b0e48ffb502da9b4f7d411d2021-04-21T15:38:02ZengPublic Library of Science (PLoS)PLoS Computational Biology1553-734X1553-73582020-02-01162e100711910.1371/journal.pcbi.1007119Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.Xiangying SunZhezhen WangJohnathon M HallCarlos Perez-CervantesAlexander J RuthenburgIvan P MoskowitzMichael GribskovXinan H YangLong 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.https://doi.org/10.1371/journal.pcbi.1007119
collection DOAJ
language English
format Article
sources DOAJ
author Xiangying Sun
Zhezhen Wang
Johnathon M Hall
Carlos Perez-Cervantes
Alexander J Ruthenburg
Ivan P Moskowitz
Michael Gribskov
Xinan H Yang
spellingShingle Xiangying Sun
Zhezhen Wang
Johnathon M Hall
Carlos Perez-Cervantes
Alexander J Ruthenburg
Ivan P Moskowitz
Michael Gribskov
Xinan H Yang
Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.
PLoS Computational Biology
author_facet Xiangying Sun
Zhezhen Wang
Johnathon M Hall
Carlos Perez-Cervantes
Alexander J Ruthenburg
Ivan P Moskowitz
Michael Gribskov
Xinan H Yang
author_sort Xiangying Sun
title Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.
title_short Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.
title_full Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.
title_fullStr Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.
title_full_unstemmed Chromatin-enriched RNAs mark active and repressive cis-regulation: An analysis of nuclear RNA-seq.
title_sort chromatin-enriched rnas mark active and repressive cis-regulation: an analysis of nuclear rna-seq.
publisher Public Library of Science (PLoS)
series PLoS Computational Biology
issn 1553-734X
1553-7358
publishDate 2020-02-01
description 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.
url https://doi.org/10.1371/journal.pcbi.1007119
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