Methylome analysis using MeDIP-seq with low DNA concentrations

被引:213
作者
Taiwo, Oluwatosin [1 ,2 ]
Wilson, Gareth A. [1 ]
Morris, Tiffany [1 ]
Seisenberger, Stefanie [3 ]
Reik, Wolf [3 ,4 ]
Pearce, Daniel [2 ]
Beck, Stephan [1 ]
Butcher, Lee M. [1 ]
机构
[1] UCL, Univ Coll London UCL Canc Inst, London, England
[2] UCL, UCL Inst Hlth Ageing, London, England
[3] Babraham Inst, Lab Dev Genet & Imprinting, Cambridge, England
[4] Univ Cambridge, Ctr Trophoblast Res, Cambridge, England
基金
英国医学研究理事会; 英国工程与自然科学研究理事会; 英国惠康基金; 英国生物技术与生命科学研究理事会;
关键词
EMBRYONIC STEM-CELLS; MAMMALIAN DNA; HUMAN GENOME; METHYLATION; 5-HYDROXYMETHYLCYTOSINE; DIFFERENTIATION; 5-CARBOXYLCYTOSINE; 5-METHYLCYTOSINE; IDENTIFICATION; ALIGNMENT;
D O I
10.1038/nprot.2012.012
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
DNA methylation is an epigenetic mark that has a crucial role in many biological processes. To understand the functional consequences of DNA methylation on phenotypic plasticity, a genome-wide analysis should be embraced. This in turn requires a technique that balances accuracy, genome coverage, resolution and cost, yet is low in DNA input in order to minimize the drain on precious samples. Methylated DNA immunoprecipitation-sequencing (MeDIP-seq) fulfils these criteria, combining MeDIP with massively parallel DNA sequencing. Here we report an improved protocol using 100-fold less genomic DNA than that commonly used. We show comparable results for specificity (>97%) and enrichment (>100-fold) over a wide range of DNA concentrations (5,000-50 ng) and demonstrate the utility of the protocol for the generation of methylomes from rare bone marrow cells using 160-300 ng of starting DNA. The protocol described here, i.e., DNA extraction to generation of MeDIP-seq library, can be completed within 3-5 d.
引用
收藏
页码:617 / 636
页数:20
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