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Mapping accessible chromatin regions using Sono-Seq.


ABSTRACT: Disruptions in local chromatin structure often indicate features of biological interest such as regulatory regions. We find that sonication of cross-linked chromatin, when combined with a size-selection step and massively parallel short-read sequencing, can be used as a method (Sono-Seq) to map locations of high chromatin accessibility in promoter regions. Sono-Seq sites frequently correspond to actively transcribed promoter regions, as evidenced by their co-association with RNA Polymerase II ChIP regions, transcription start sites, histone H3 lysine 4 trimethylation (H3K4me3) marks, and CpG islands; signals over other sites, such as those bound by the CTCF insulator, are also observed. The pattern of breakage by Sono-Seq overlaps with, but is distinct from, that observed for FAIRE and DNase I hypersensitive sites. Our results demonstrate that Sono-Seq can be a useful and simple method by which to map many local alterations in chromatin structure. Furthermore, our results provide insights into the mapping of binding sites by using ChIP-Seq experiments and the value of reference samples that should be used in such experiments.

SUBMITTER: Auerbach RK 

PROVIDER: S-EPMC2736440 | biostudies-literature | 2009 Sep

REPOSITORIES: biostudies-literature

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Mapping accessible chromatin regions using Sono-Seq.

Auerbach Raymond K RK   Euskirchen Ghia G   Rozowsky Joel J   Lamarre-Vincent Nathan N   Moqtaderi Zarmik Z   Lefrançois Philippe P   Struhl Kevin K   Gerstein Mark M   Snyder Michael M  

Proceedings of the National Academy of Sciences of the United States of America 20090818 35


Disruptions in local chromatin structure often indicate features of biological interest such as regulatory regions. We find that sonication of cross-linked chromatin, when combined with a size-selection step and massively parallel short-read sequencing, can be used as a method (Sono-Seq) to map locations of high chromatin accessibility in promoter regions. Sono-Seq sites frequently correspond to actively transcribed promoter regions, as evidenced by their co-association with RNA Polymerase II Ch  ...[more]

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