DHPLC-Based Method for DNA Methylation Analysis of Differential Methylated Regions from Imprinted Genes

DNA甲基化 甲基化 生物 分子生物学 CpG站点 表观遗传学 亚硫酸氢盐测序 差异甲基化区 照明菌甲基化试验 基因 基因组印记 DNA 5-甲基胞嘧啶 胞嘧啶 甲基化DNA免疫沉淀 亚硫酸氢盐 印记(心理学)
作者
Philippe Couvert,Karine Poirier,Alain Carrié,Céline Chalas,Pierre Jouannet,Chérif Beldjord,T. Bienvenu,Jamel Chelly,Antoine Kerjean
出处
期刊:BioTechniques [Future Science Ltd]
卷期号:34 (2): 356-362 被引量:23
标识
DOI:10.2144/03342rr06
摘要

The bisulfite genomic sequencing method is one of the most widely used techniques for methylation analysis in heterogeneous unbiased PCR, amplifying for both methylated and unmethylated alleles simultaneously. However, it requires labor-intensive and time-consuming cloning and sequencing steps. In the current study, we used a denaturing high-performance liquid chromatography (DHPLC) procedure in a complementary way with the bisulfite genomic sequencing to analyze the methylation of differentially methylated regions (DMRs) of imprinted genes. We showed reliable and reproducible results in distinguishing overall methylation profiles of DMRs regions of human SNRPN, H19, MEST/PEG1, LIT1, IGF2, TSSC5, WT1 antisense, and mouse H19, Mest/Peg1, Igf2R imprinted genes. These DHPLC profiles were in accordance with bisulfite genomic sequencing data and may serve as a type of "fingerprint," revealing the overall methylation status of DMRs associated with sample heterogeneity. We conclude that DHPLC analysis could be used to increase the throughput efficiency of methylation pattern analysis of imprinted genes after the bisulfite conversion of genomic DNA and unbiased PCR amplification.
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