Genome-wide profiles of STAT1 DNA association using chromatin immunoprecipitation and massively parallel sequencing

Robertson, Gordon; Hirst, Martin; Bainbridge, Matthew N.; Bilenky, Misha; Zhao, Yongjun; Zeng, Thomas; Euskirchen, Ghia; Bernier, Bridget; Varhol, Richard; Delaney, Allen; Thiessen, Nina; Griffith, Obi L.; He, Ann; Marra, Marco A.; Snyder, M; Jones, Steven J.M.

doi:10.1038/nmeth1068

Cited by 1,238 publications

(1,037 citation statements)

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“…1), we searched for HIF-1a binding sites by quantifying the local enrichment of tags (Robertson et al 2007) (see ''Materials and methods''). Next, we classified the putatively identified binding sites as ''hypoxia-responsive'' or ''non-hypoxia-responsive.''…”

Section: Resultsmentioning

confidence: 99%

“…In the HIF-1a ChIP-Seq analysis, if the identified regions demonstrated an overlap between 1% O 2 (hypoxia) and 21% O 2 (normoxia), regions with more than a twofold (hypoxia/ normoxia) change in peak strength were identified as ''bindings enriched in hypoxia.'' The statistical significance determined for this selection procedure compared to the background rate was evaluated using Poisson probabilities as previously described (Robertson et al 2007):Pðx; kÞ ¼ 1 À P x t¼0 e Àk k t t! ;where P(x,k) is the probability of enrichment, k is the expected tag number in the 121-bp window calculated for the WCE sample, and x is the observed tag number in the 121-bp window.…”

Section: Computational Proceduresmentioning

confidence: 99%

“…For example, the Illumina GA sequencer can sequence 200-250 million sequences per run. By utilizing Illumina GA and ChIP technologies (ChIP-Seq), the binding sites of several transcription factors have been reported (Valouev et al 2008;Robertson et al 2007;Kwon et al 2009;Welboren et al 2009;Park 2009). On the other hand, we also developed a method for sequencing the 5 0 -ends of mRNAs by combining our oligo-capping technique with the Illumina GA sequencer (Tsuchihara et al 2009).…”

Section: Introductionmentioning

confidence: 99%

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Genome-wide identification and annotation of HIF-1α binding sites in two cell lines using massively parallel sequencing

Tanimoto

Tsuchihara

Kanai

et al. 2010

HUGO J

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We identified 531 and 616 putative HIF-1a target sites by ChIP-Seq in the cancerous cell line DLD-1 and the non-cancerous cell line TIG-3, respectively. We also examined the positions and expression levels of transcriptional start sites (TSSs) in these cell lines using our TSS-Seq method. We observed that 121 and 48 genes in DLD-1 and TIG-3 cells, respectively, had HIF-1a binding sites in proximal regions of the previously reported TSSs that were up-regulated at the transcriptional level. In addition, 193 and 123 of the HIF-1a target sites, respectively, were located in proximal regions of previously uncharacterized TSSs, namely, TSSs of putative alternative promoters of protein-coding genes or promoters of putative non-protein-coding transcripts. The hypoxic response of DLD-1 cells was more significant than that of TIG-3 cells with respect to both the number of target sites and the degree of induced changes in transcript expression. The Nucleosome-Seq and ChIP-Seq analyses of histone modifications revealed that the chromatin formed an open structure in regions surrounding the HIF-1a binding sites, but this event occurred prior to the actual binding of HIF1a. Different cellular histories may be encoded by chromatin structures and determine the activation of specific genes in response to hypoxic shock.

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Section: Resultsmentioning

confidence: 99%

Section: Computational Proceduresmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Genome-wide identification and annotation of HIF-1α binding sites in two cell lines using massively parallel sequencing

Tanimoto

Tsuchihara

Kanai

et al. 2010

HUGO J

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“…However, ChIP-sequencing, which combines ChIP and massively parallel sequencing, can be used to directly identify the DNA sequences bound by transcription factors, including strength of binding, in vivo [17]. Here, we performed global DNA sequence analysis of triplicate TCF7L2 ChIP samples in the human colorectal cell line, HCT116, where TCF7L2 is abundantly produced.…”

Section: Introductionmentioning

confidence: 99%

Disease-associated loci are significantly over-represented among genes bound by transcription factor 7-like 2 (TCF7L2) in vivo

Zhao

Schug

et al. 2010

Diabetologia

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Aims/hypothesis Transcription factor 7-like 2 (TCF7L2) has been strongly implicated in type 2 diabetes and cancer. Our goal was to identify the DNA sequences bound by this transcription factor in vivo. Methods We applied chromatin immunoprecipitation and sequencing to globally identify and map human DNA sequences bound by TCF7L2 in the colorectal carcinoma cell line, HCT116, where it is abundantly expressed. ResultsWe identified 1,095 discrete binding sites across the genome, of which a subset were within 5 kb of 548 annotated NCBI Reference Sequence (RefSeq) genes. Despite using a cancer cell line, the most significant functions represented using pathway analysis software were related to diabetes, genetic disorders and coronary artery disease. As one of the enriched categories was related to genetic disorders, we queried our results against all published genome-wide association studies (GWAS) and found a highly significant over-representation of reported loci from among the genes bound by TCF7L2 within 5 kb (p=7.50×10 −15 ). This observation was primarily driven by excess loci revealed from GWAS of metabolic and cardiovascular traits; however, there was no or only minor enrichment of GWAS-derived loci for cancer, and inflammatory or neurological diseases. Of the specific traits, the most enriched loci were for type 2 diabetes and height. When defining the distance from genes at 50 kb or 500 kb, this enrichment pattern persisted, with some additional evidence for enrichment of cancer-related loci. Conclusions/interpretation A highly significant proportion of genes bound by TCF7L2 are known disease-associated loci. These findings suggest that TCF7L2 is a central node in the regulation of human diabetes and other diseaseassociated genes.

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“…The knowledge of alternative promoter usage in different mammalian tissues is very limited and cannot be addressed without high-resolution genome-wide mapping of the promoter regions. However, the high-throughput approaches, such as CAGE (14), deepCAGE (15), ChIP-chip (16,17) or ChIP-seq (7), to annotate promoters at genome level need to be applied with caution because of the inherent problems with each method. For example, cytoplasmic enzyme complexes can add caps to 5 0 -monophosphate RNA molecules generated by ribonuclease cleavage (18), and hence CAGE tags could represent 5 0 ends of RNAs generated by cleavage and subsequent re-capping (19).…”

Section: Introductionmentioning

confidence: 99%

Genome-Wide Mapping of RNA Pol-II Promoter Usage in Mouse Tissues by ChIP-Seq

Pal

Gupta

Davuluri

2014

Methods in Molecular Biology

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Genome-wide profiles of STAT1 DNA association using chromatin immunoprecipitation and massively parallel sequencing

Cited by 1,238 publications

References 32 publications

Genome-wide identification and annotation of HIF-1α binding sites in two cell lines using massively parallel sequencing

Genome-wide identification and annotation of HIF-1α binding sites in two cell lines using massively parallel sequencing

Disease-associated loci are significantly over-represented among genes bound by transcription factor 7-like 2 (TCF7L2) in vivo

Genome-Wide Mapping of RNA Pol-II Promoter Usage in Mouse Tissues by ChIP-Seq

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