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MS-qFRET: A quantum dot-based method for analysis of DNA methylation

机译:MS-qFRET:一种基于量子点的DNA甲基化分析方法

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摘要

DNA methylation contributes to carcinogenesis by silencing key tumor suppressor genes. Here we report an ultrasensitive and reliable nanotechnology assay, MS-qFRET, for detection and quantification of DNA methylation. Bisulfite-modified DNA is subjected to PCR amplification with primers that would differentiate between methylated and unmethylated DNA. Quantum dots are then used to capture PCR amplicons and determine the methylation status via fluorescence resonance energy transfer (FRET). Key features of MS-qFRET include its low intrinsic background noise, high resolution, and high sensitivity. This approach detects as little as 15 pg of methylated DNA in the presence of a 10,000-fold excess of unmethylated alleles, enables reduced use of PCR (as low as eight cycles), and allows for multiplexed analyses. The high sensitivity of MS-qFRET enables one-step detection of methylation at PYCARD, CDKN2B, and CDKN2A genes in patient sputum samples that contain low concentrations of methylated DNA, which normally would require a nested PCR approach. The direct application of MS-qFRET on clinical samples offers great promise for its translational use in early cancer diagnosis, prognostic assessment of tumor behavior, as well as monitoring response to therapeutic agents.
机译:DNA甲基化通过沉默关键的肿瘤抑制基因来促进癌变。在这里,我们报告了一种用于检测和定量DNA甲基化的超灵敏可靠的纳米技术测定MS-qFRET。亚硫酸氢盐修饰的DNA用引物进行PCR扩增,该引物会区分甲基化的DNA和未甲基化的DNA。然后使用量子点捕获PCR扩增子,并通过荧光共振能量转移(FRET)确定甲基化状态。 MS-qFRET的主要特征包括低固有背景噪声,高分辨率和高灵敏度。这种方法在存在10,000倍过量的未甲基化等位基因的情况下,可检测低至15 pg的甲基化DNA,可减少PCR的使用(低至8个循环),并允许进行多重分析。 MS-qFRET的高灵敏度可一步检测含有低浓度甲基化DNA的患者痰液样本中PYCARD,CDKN2B和CDKN2A基因的甲基化,这通常需要嵌套式PCR方法。 MS-qFRET在临床样品上的直接应用为其在早期癌症诊断,肿瘤行为的预后评估以及监测对治疗药物的反应中的翻译应用提供了广阔的前景。

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