Literature DB >> 23436351

DNase I digestion of isolated nulcei for genome-wide mapping of DNase hypersensitivity sites in chromatin.

Guoyu Ling1, David J Waxman.   

Abstract

DNase I hypersensitivity (DHS) analysis is a powerful method to analyze chromatin structure and identify genomic regulatory elements. Integration of a high-throughput detection method into DHS analysis makes genome-wide mapping of DHS sites possible at a reasonable cost. Here we describe methods for DHS analysis carried out with mouse liver nuclei, involving DNase I digestion followed by isolation of DNase I-released DNA fragments suitable for high-throughput, next generation DNA sequencing (DNase-seq). A real-time PCR-based assay used to optimize DNase I digestion conditions is also described.

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Year:  2013        PMID: 23436351      PMCID: PMC3889470          DOI: 10.1007/978-1-62703-284-1_3

Source DB:  PubMed          Journal:  Methods Mol Biol        ISSN: 1064-3745


  11 in total

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4.  DNase-chip: a high-resolution method to identify DNase I hypersensitive sites using tiled microarrays.

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Journal:  Nat Methods       Date:  2006-07       Impact factor: 28.547

5.  Unbiased, genome-wide in vivo mapping of transcriptional regulatory elements reveals sex differences in chromatin structure associated with sex-specific liver gene expression.

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Review 7.  Structure and function of active chromatin and DNase I hypersensitive sites.

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Journal:  FEBS J       Date:  2011-05-26       Impact factor: 5.542

8.  DNase-seq: a high-resolution technique for mapping active gene regulatory elements across the genome from mammalian cells.

Authors:  Lingyun Song; Gregory E Crawford
Journal:  Cold Spring Harb Protoc       Date:  2010-02

9.  Quantification of DNaseI-sensitivity by real-time PCR: quantitative analysis of DNaseI-hypersensitivity of the mouse beta-globin LCR.

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