Department of Genetics, Center for Genome Sciences, Washington University School of Medicine, 4444 Forest Park Parkway, St. Louis, Missouri 63110, USA.
Nucleic Acids Res. 2013 Jun;41(11):e116. doi: 10.1093/nar/gkt230. Epub 2013 Apr 15.
DNA methylation is a mechanism for long-term transcriptional regulation and is required for normal cellular differentiation. Failure to properly establish or maintain DNA methylation patterns leads to cell dysfunction and diseases such as cancer. Identifying DNA methylation signatures in complex tissues can be challenging owing to inaccurate cell enrichment methods and low DNA yields. We have developed a technique called laser capture microdissection-reduced representation bisulfite sequencing (LCM-RRBS) for the multiplexed interrogation of the DNA methylation status of cytosine-guanine dinucleotide islands and promoters. LCM-RRBS accurately and reproducibly profiles genome-wide methylation of DNA extracted from microdissected fresh frozen or formalin-fixed paraffin-embedded tissue samples. To demonstrate the utility of LCM-RRBS, we characterized changes in DNA methylation associated with gonadectomy-induced adrenocortical neoplasia in the mouse. Compared with adjacent normal tissue, the adrenocortical tumors showed reproducible gains and losses of DNA methylation at genes involved in cell differentiation and organ development. LCM-RRBS is a rapid, cost-effective, and sensitive technique for analyzing DNA methylation in heterogeneous tissues and will facilitate the investigation of DNA methylation in cancer and organ development.
DNA 甲基化是一种长期转录调控的机制,对于正常的细胞分化是必需的。未能正确建立或维持 DNA 甲基化模式会导致细胞功能障碍和癌症等疾病。由于不准确的细胞富集方法和低 DNA 产量,在复杂组织中识别 DNA 甲基化特征具有挑战性。我们开发了一种称为激光捕获显微切割-简化重亚硫酸盐测序(LCM-RRBS)的技术,用于对胞嘧啶-鸟嘌呤二核苷酸岛和启动子的 DNA 甲基化状态进行多路询问。LCM-RRBS 可以准确且可重复地对从小鼠新鲜冷冻或福尔马林固定石蜡包埋组织样本中提取的 DNA 进行全基因组甲基化分析。为了证明 LCM-RRBS 的实用性,我们研究了与性腺切除诱导的小鼠肾上腺皮质肿瘤发生相关的 DNA 甲基化变化。与相邻的正常组织相比,肾上腺皮质肿瘤在涉及细胞分化和器官发育的基因中表现出可重复的 DNA 甲基化获得和丧失。LCM-RRBS 是一种快速、具有成本效益和敏感的分析异质组织中 DNA 甲基化的技术,将有助于癌症和器官发育中 DNA 甲基化的研究。
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