A Global Clustering Algorithm to Identify Long Intergenic Non-Coding RNA - with Applications in Mouse Macrophages
Identification of diffuse signals from the chromatin immunoprecipitation and high-throughput massively parallel sequencing (ChIP-Seq) technology poses significant computational challenges, and there are few methods currently available. We present a novel global clustering approach to enrich diffuse...
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| Published in | PloS one Vol. 6; no. 9; p. e24051 |
|---|---|
| Main Authors | , , , , , |
| Format | Journal Article |
| Language | English |
| Published |
United States
Public Library of Science
30.09.2011
Public Library of Science (PLoS) |
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| Online Access | Get full text |
| ISSN | 1932-6203 1932-6203 |
| DOI | 10.1371/journal.pone.0024051 |
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| Abstract | Identification of diffuse signals from the chromatin immunoprecipitation and high-throughput massively parallel sequencing (ChIP-Seq) technology poses significant computational challenges, and there are few methods currently available. We present a novel global clustering approach to enrich diffuse CHIP-Seq signals of RNA polymerase II and histone 3 lysine 4 trimethylation (H3K4Me3) and apply it to identify putative long intergenic non-coding RNAs (lincRNAs) in macrophage cells. Our global clustering method compares favorably to the local clustering method SICER that was also designed to identify diffuse CHIP-Seq signals. The validity of the algorithm is confirmed at several levels. First, 8 out of a total of 11 selected putative lincRNA regions in primary macrophages respond to lipopolysaccharides (LPS) treatment as predicted by our computational method. Second, the genes nearest to lincRNAs are enriched with biological functions related to metabolic processes under resting conditions but with developmental and immune-related functions under LPS treatment. Third, the putative lincRNAs have conserved promoters, modestly conserved exons, and expected secondary structures by prediction. Last, they are enriched with motifs of transcription factors such as PU.1 and AP.1, previously shown to be important lineage determining factors in macrophages, and 83% of them overlap with distal enhancers markers. In summary, GCLS based on RNA polymerase II and H3K4Me3 CHIP-Seq method can effectively detect putative lincRNAs that exhibit expected characteristics, as exemplified by macrophages in the study. |
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| AbstractList | Identification of diffuse signals from the chromatin immunoprecipitation and high-throughput massively parallel sequencing (ChIP-Seq) technology poses significant computational challenges, and there are few methods currently available. We present a novel global clustering approach to enrich diffuse CHIP-Seq signals of RNA polymerase II and histone 3 lysine 4 trimethylation (H3K4Me3) and apply it to identify putative long intergenic non-coding RNAs (lincRNAs) in macrophage cells. Our global clustering method compares favorably to the local clustering method SICER that was also designed to identify diffuse CHIP-Seq signals. The validity of the algorithm is confirmed at several levels. First, 8 out of a total of 11 selected putative lincRNA regions in primary macrophages respond to lipopolysaccharides (LPS) treatment as predicted by our computational method. Second, the genes nearest to lincRNAs are enriched with biological functions related to metabolic processes under resting conditions but with developmental and immune-related functions under LPS treatment. Third, the putative lincRNAs have conserved promoters, modestly conserved exons, and expected secondary structures by prediction. Last, they are enriched with motifs of transcription factors such as PU.1 and AP.1, previously shown to be important lineage determining factors in macrophages, and 83% of them overlap with distal enhancers markers. In summary, GCLS based on RNA polymerase II and H3K4Me3 CHIP-Seq method can effectively detect putative lincRNAs that exhibit expected characteristics, as exemplified by macrophages in the study. Identification of diffuse signals from the chromatin immunoprecipitation and high-throughput massively parallel sequencing (ChIP-Seq) technology poses significant computational challenges, and there are few methods currently available. We present a novel global clustering approach to enrich diffuse CHIP-Seq signals of RNA polymerase II and histone 3 lysine 4 trimethylation (H3K4Me3) and apply it to identify putative long intergenic non-coding RNAs (lincRNAs) in macrophage cells. Our global clustering method compares favorably to the local clustering method SICER that was also designed to identify diffuse CHIP-Seq signals. The validity of the algorithm is confirmed at several levels. First, 8 out of a total of 11 selected putative lincRNA regions in primary macrophages respond to lipopolysaccharides (LPS) treatment as predicted by our computational method. Second, the genes nearest to lincRNAs are enriched with biological functions related to metabolic processes under resting conditions but with developmental and immune-related functions under LPS treatment. Third, the putative lincRNAs have conserved promoters, modestly conserved exons, and expected secondary structures by prediction. Last, they are enriched with motifs of transcription factors such as PU.1 and AP.1, previously shown to be important lineage determining factors in macrophages, and 83% of them overlap with distal enhancers markers. In summary, GCLS based on RNA polymerase II and H3K4Me3 CHIP-Seq method can effectively detect putative lincRNAs that exhibit expected characteristics, as exemplified by macrophages in the study.Identification of diffuse signals from the chromatin immunoprecipitation and high-throughput massively parallel sequencing (ChIP-Seq) technology poses significant computational challenges, and there are few methods currently available. We present a novel global clustering approach to enrich diffuse CHIP-Seq signals of RNA polymerase II and histone 3 lysine 4 trimethylation (H3K4Me3) and apply it to identify putative long intergenic non-coding RNAs (lincRNAs) in macrophage cells. Our global clustering method compares favorably to the local clustering method SICER that was also designed to identify diffuse CHIP-Seq signals. The validity of the algorithm is confirmed at several levels. First, 8 out of a total of 11 selected putative lincRNA regions in primary macrophages respond to lipopolysaccharides (LPS) treatment as predicted by our computational method. Second, the genes nearest to lincRNAs are enriched with biological functions related to metabolic processes under resting conditions but with developmental and immune-related functions under LPS treatment. Third, the putative lincRNAs have conserved promoters, modestly conserved exons, and expected secondary structures by prediction. Last, they are enriched with motifs of transcription factors such as PU.1 and AP.1, previously shown to be important lineage determining factors in macrophages, and 83% of them overlap with distal enhancers markers. In summary, GCLS based on RNA polymerase II and H3K4Me3 CHIP-Seq method can effectively detect putative lincRNAs that exhibit expected characteristics, as exemplified by macrophages in the study. |
| Audience | Academic |
| Author | Garmire, David G. Subramaniam, Shankar Huang, Wendy Glass, Christopher K. Yao, Joyee Garmire, Lana X. |
| AuthorAffiliation | 1 Department of Bioengineering, Jacobs School of Engineering, University of California San Diego, La Jolla, California, United States of America 3 Department of Cellular and Molecular Medicine, School of Medicine, University of California San Diego, La Jolla, California, United States of America 2 Department of Electrical Engineering, University of Hawaii at Manoa, Honolulu, Hawaii, United States of America Georgia Institute of Technology, United States of America |
| AuthorAffiliation_xml | – name: Georgia Institute of Technology, United States of America – name: 3 Department of Cellular and Molecular Medicine, School of Medicine, University of California San Diego, La Jolla, California, United States of America – name: 1 Department of Bioengineering, Jacobs School of Engineering, University of California San Diego, La Jolla, California, United States of America – name: 2 Department of Electrical Engineering, University of Hawaii at Manoa, Honolulu, Hawaii, United States of America |
| Author_xml | – sequence: 1 givenname: Lana X. surname: Garmire fullname: Garmire, Lana X. – sequence: 2 givenname: David G. surname: Garmire fullname: Garmire, David G. – sequence: 3 givenname: Wendy surname: Huang fullname: Huang, Wendy – sequence: 4 givenname: Joyee surname: Yao fullname: Yao, Joyee – sequence: 5 givenname: Christopher K. surname: Glass fullname: Glass, Christopher K. – sequence: 6 givenname: Shankar surname: Subramaniam fullname: Subramaniam, Shankar |
| BackLink | https://www.ncbi.nlm.nih.gov/pubmed/21980340$$D View this record in MEDLINE/PubMed |
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| Notes | ObjectType-Article-1 SourceType-Scholarly Journals-1 ObjectType-Feature-2 content type line 14 content type line 23 Conceived and designed the experiments: LXG CKG SS. Performed the experiments: WH JY. Analyzed the data: LXG DG. Wrote the paper: LXG SS. |
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| SubjectTerms | Algorithms Animals Atherosclerosis B cells Bioengineering Bioinformatics Biology Chromatin Chromatin Immunoprecipitation - methods Cluster Analysis Clustering Computation Computational Biology - methods Computer applications Deoxyribonucleic acid DNA DNA binding proteins DNA-directed RNA polymerase Engineering Engineering schools Enhancers Enrichment Exons Gene expression Genes Genome Genomes Histones - chemistry Humans Identification Immunoprecipitation International conferences Lipopolysaccharides Lipopolysaccharides - metabolism Lysine Macrophages Macrophages - metabolism Medicine Methylation Mice Multiprocessing Non-coding RNA Oligonucleotide Array Sequence Analysis Predictions Proteins PU.1 protein Ribonucleic acid RNA RNA polymerase RNA polymerase II RNA Polymerase II - metabolism RNA, Untranslated - genetics Sequence Analysis, DNA Transcription factors |
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| Title | A Global Clustering Algorithm to Identify Long Intergenic Non-Coding RNA - with Applications in Mouse Macrophages |
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