meHOLMES: A CRISPR-cas12a-based method for rapid detection of DNA methylation in a sequence-independent manner

胞嘧啶 DNA 计算生物学 DNA甲基化 生物 CpG站点 亚硫酸氢盐 脱氨基 亚硫酸氢盐测序 清脆的 甲基化 分子生物学 胸腺嘧啶 遗传学 生物化学 基因 基因表达
作者
Songkuan Zhuang,Tianshuai Hu,Xike Zhou,Hongzhong Zhou,Shiping He,Jie Li,Long Qiu,Yuehui Zhang,Yong Xu,Pei Hao,Dayong Gu,Jin Wang
出处
期刊:Heliyon [Elsevier BV]
卷期号:10 (2): e24574-e24574
标识
DOI:10.1016/j.heliyon.2024.e24574
摘要

Aberrant DNA methylation is closely associated with various diseases, particularly cancer, and its precise detection plays an essential role in disease diagnosis and monitoring. In this study, we present a novel DNA methylation detection method (namely meHOLMES), which integrates both the TET2/APOBEC-mediated cytosine deamination step and the CRISPR-Cas12a-based signal readout step. TET2/APOBEC efficiently converts unmethylated cytosine to uracil, which is subsequently changed to thymine after PCR amplification. Utilizing a rationally designed crRNA, Cas12a specifically identifies unconverted methylated cytosines and generates detectable signals using either fluorescent reporters or lateral flow test strips. meHOLMES quantitatively detects methylated CpG sites with or without Protospacer Adjacent Motif (PAM) sequences in both artificial and real biological samples. In addition, meHOLMES can complete the whole detection process within 6 h, which is much faster than traditional bisulfite-based sample pre-treatment method. Above all, meHOLMES provides a simpler, faster, more accurate, and cost-effective approach for quantitation of DNA methylation levels in a sequence-independent manner.

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