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甲基化 DNA 免疫沉淀(MeDIP)和甲基化 CpG 结合域(MBD)蛋白捕获用于全基因组 DNA 甲基化分析的比较揭示了 CpG 序列覆盖偏差。

Comparison of methyl-DNA immunoprecipitation (MeDIP) and methyl-CpG binding domain (MBD) protein capture for genome-wide DNA methylation analysis reveal CpG sequence coverage bias.

机构信息

Epigenetics Laboratory, Garvan Institute of Medical Research, Darlinghurst, NSW, Australia.

出版信息

Epigenetics. 2011 Jan;6(1):34-44. doi: 10.4161/epi.6.1.13313. Epub 2011 Jan 1.

DOI:10.4161/epi.6.1.13313
PMID:20818161
Abstract

DNA methylation primarily occurs at CpG dinucleotides in mammals and is a common epigenetic mark that plays a critical role in the regulation of gene expression. Profiling DNA methylation patterns across the genome is vital to understand DNA methylation changes that occur during development and in disease phenotype. In this study, we compared two commonly used approaches to enrich for methylated DNA regions of the genome, namely methyl-DNA immunoprecipitation (MeDIP) that is based on enrichment with antibodies specific for 5'-methylcytosine (5MeC), and capture of methylated DNA using a methyl-CpG binding domain-based (MBD) protein to discover differentially methylated regions (DMRs) in cancer. The enriched methylated DNA fractions were interrogated on Affymetrix promoter tiling arrays and differentially methylated regions were identified. A detailed validation study of 42 regions was performed using Sequenom MassCLEAVE technique. This detailed analysis revealed that both enrichment techniques are sensitive for detecting DMRs and preferentially identified different CpG rich regions of the prostate cancer genome, with MeDIP commonly enriching for methylated regions with a low CpG density, while MBD capture favors regions of higher CpG density and identifies the greatest proportion of CpG islands. This is the first detailed validation report comparing different methylated DNA enrichment techniques for identifying regions of differential DNA methylation. Our study highlights the importance of understanding the nuances of the methods used for DNA genome-wide methylation analyses so that accurate interpretation of the biology is not overlooked.

摘要

DNA 甲基化主要发生在哺乳动物的 CpG 二核苷酸中,是一种常见的表观遗传标记,在基因表达调控中起着关键作用。对整个基因组的 DNA 甲基化模式进行分析对于理解发育过程中和疾病表型中发生的 DNA 甲基化变化至关重要。在这项研究中,我们比较了两种常用于富集基因组中甲基化 DNA 区域的方法,即基于针对 5'-甲基胞嘧啶(5MeC)的抗体富集的甲基化 DNA 免疫沉淀(MeDIP),以及使用基于甲基化 CpG 结合域(MBD)的蛋白质捕获甲基化 DNA 以发现癌症中的差异甲基化区域(DMR)。对 Affymetrix 启动子平铺阵列进行了富集的甲基化 DNA 分数的检测,并鉴定了差异甲基化区域。使用 Sequenom MassCLEAVE 技术对 42 个区域进行了详细的验证研究。这项详细的分析表明,两种富集技术都能灵敏地检测到 DMRs,并且优先鉴定前列腺癌基因组中不同的富含 CpG 的区域,MeDIP 通常富集低 CpG 密度的甲基化区域,而 MBD 捕获则倾向于高 CpG 密度的区域,并鉴定出最大比例的 CpG 岛。这是第一篇比较不同的甲基化 DNA 富集技术用于鉴定差异 DNA 甲基化区域的详细验证报告。我们的研究强调了理解用于全基因组 DNA 甲基化分析的方法细节的重要性,以便不会忽视对生物学的准确解释。

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