Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements

Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements

<p>Abstract</p> <p>Background</p> <p>Transcription factor binding to DNA requires both an appropriate binding element and suitably open chromatin, which together help to define regulatory elements within the genome. Current methods of identifying regulatory elements, su...

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Main Authors: Rye Morten, Sætrom Pål, Håndstad Tony, Drabløs Finn
Format: Article
Language:English
Published: BMC 2011-11-01
Series:BMC Biology
Subjects:
transcription factor
ChIP-Seq
histone modification
chromatin
Online Access:http://www.biomedcentral.com/1741-7007/9/80
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spelling doaj-b781abe5bb9f45938f5340631e93764a2020-11-24T21:49:48ZengBMCBMC Biology1741-70072011-11-01918010.1186/1741-7007-9-80Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elementsRye MortenSætrom PålHåndstad TonyDrabløs Finn<p>Abstract</p> <p>Background</p> <p>Transcription factor binding to DNA requires both an appropriate binding element and suitably open chromatin, which together help to define regulatory elements within the genome. Current methods of identifying regulatory elements, such as promoters or enhancers, typically rely on sequence conservation, existing gene annotations or specific marks, such as histone modifications and p300 binding methods, each of which has its own biases.</p> <p>Results</p> <p>Herein we show that an approach based on clustering of transcription factor peaks from high-throughput sequencing coupled with chromatin immunoprecipitation (Chip-Seq) can be used to evaluate markers for regulatory elements. We used 67 data sets for 54 unique transcription factors distributed over two cell lines to create regulatory element clusters. By integrating the clusters from our approach with histone modifications and data for open chromatin, we identified general methylation of lysine 4 on histone H3 (H3K4me) as the most specific marker for transcription factor clusters. Clusters mapping to annotated genes showed distinct patterns in cluster composition related to gene expression and histone modifications. Clusters mapping to intergenic regions fall into two groups either directly involved in transcription, including miRNAs and long noncoding RNAs, or facilitating transcription by long-range interactions. The latter clusters were specifically enriched with H3K4me1, but less with acetylation of lysine 27 on histone 3 or p300 binding.</p> <p>Conclusion</p> <p>By integrating genomewide data of transcription factor binding and chromatin structure and using our data-driven approach, we pinpointed the chromatin marks that best explain transcription factor association with different regulatory elements. Our results also indicate that a modest selection of transcription factors may be sufficient to map most regulatory elements in the human genome.</p> http://www.biomedcentral.com/1741-7007/9/80transcription factorChIP-Seqhistone modificationchromatin
collection DOAJ
language English
format Article
sources DOAJ
author Rye Morten
Sætrom Pål
Håndstad Tony
Drabløs Finn
spellingShingle Rye Morten
Sætrom Pål
Håndstad Tony
Drabløs Finn
Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements
BMC Biology
transcription factor
ChIP-Seq
histone modification
chromatin
author_facet Rye Morten
Sætrom Pål
Håndstad Tony
Drabløs Finn
author_sort Rye Morten
title Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements
title_short Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements
title_full Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements
title_fullStr Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements
title_full_unstemmed Clustered ChIP-Seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements
title_sort clustered chip-seq-defined transcription factor binding sites and histone modifications map distinct classes of regulatory elements
publisher BMC
series BMC Biology
issn 1741-7007
publishDate 2011-11-01
description <p>Abstract</p> <p>Background</p> <p>Transcription factor binding to DNA requires both an appropriate binding element and suitably open chromatin, which together help to define regulatory elements within the genome. Current methods of identifying regulatory elements, such as promoters or enhancers, typically rely on sequence conservation, existing gene annotations or specific marks, such as histone modifications and p300 binding methods, each of which has its own biases.</p> <p>Results</p> <p>Herein we show that an approach based on clustering of transcription factor peaks from high-throughput sequencing coupled with chromatin immunoprecipitation (Chip-Seq) can be used to evaluate markers for regulatory elements. We used 67 data sets for 54 unique transcription factors distributed over two cell lines to create regulatory element clusters. By integrating the clusters from our approach with histone modifications and data for open chromatin, we identified general methylation of lysine 4 on histone H3 (H3K4me) as the most specific marker for transcription factor clusters. Clusters mapping to annotated genes showed distinct patterns in cluster composition related to gene expression and histone modifications. Clusters mapping to intergenic regions fall into two groups either directly involved in transcription, including miRNAs and long noncoding RNAs, or facilitating transcription by long-range interactions. The latter clusters were specifically enriched with H3K4me1, but less with acetylation of lysine 27 on histone 3 or p300 binding.</p> <p>Conclusion</p> <p>By integrating genomewide data of transcription factor binding and chromatin structure and using our data-driven approach, we pinpointed the chromatin marks that best explain transcription factor association with different regulatory elements. Our results also indicate that a modest selection of transcription factors may be sufficient to map most regulatory elements in the human genome.</p>
topic transcription factor
ChIP-Seq
histone modification
chromatin
url http://www.biomedcentral.com/1741-7007/9/80
work_keys_str_mv AT ryemorten clusteredchipseqdefinedtranscriptionfactorbindingsitesandhistonemodificationsmapdistinctclassesofregulatoryelements
AT sætrompal clusteredchipseqdefinedtranscriptionfactorbindingsitesandhistonemodificationsmapdistinctclassesofregulatoryelements
AT handstadtony clusteredchipseqdefinedtranscriptionfactorbindingsitesandhistonemodificationsmapdistinctclassesofregulatoryelements
AT drabløsfinn clusteredchipseqdefinedtranscriptionfactorbindingsitesandhistonemodificationsmapdistinctclassesofregulatoryelements
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