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基于不对称 PCR 和荧光探针介导的熔解曲线的 ALDH2 基因单核苷酸多态性基因分型。

Single nucleotide polymorphism genotyping of ALDH2 gene based on asymmetric PCR and fluorescent probe-mediated melting curves.

机构信息

Department of Laboratory Medicine, The Affiliated Hospital of Southwest Medical University, Luzhou, 646000, PR China.

Department of Clinical Laboratory, Zigong Fourth People' Hospital, Zigong, 643099, PR China.

出版信息

Anal Biochem. 2022 Apr 1;642:114509. doi: 10.1016/j.ab.2021.114509. Epub 2021 Dec 2.

DOI:10.1016/j.ab.2021.114509
PMID:34864041
Abstract

Detection of single nucleotide polymorphisms (SNPs) is of great value in precision medicine. The polymorphism of the aldehyde dehydrogenase 2 (ALDH2) gene is caused by a G1510A transition, resulting in the substitution of glutamic acid by lysine at position 487. People of different ALDH2 genotypes show different susceptibility to cancer, metabolic diseases, etc. SNP analysis based on fluorescent probe-mediated melting curves is a relatively efficient and cost-effective method. Genomic DNA extracted from 100 whole blood samples was subjected to polymorphisms mutational analysis using asymmetric PCR and probe-mediated melting curves. Then a certain number of samples from each genotype were randomly selected for direct sequencing verification. The new assay can be performed in 2 h without post-PCR processing such as gel electrophoresis and validated by direct sequencing in a blind study with 100% concordance. Moreover, comparing the detection of polymorphisms of ALDH2 with the clinics, and an overall agreement of 100% (100/100) was demonstrated. Our study has shown a high level of concordance between DNA sequencing, which is suitable for the detection of clinical specimens. Based on the concept of probe-mediated melting curves, we further developed this platform as a universal strategy for the detection of polymorphisms related to folate metabolism.

摘要

单核苷酸多态性(SNP)的检测在精准医学中具有重要价值。醛脱氢酶 2(ALDH2)基因的多态性是由于 G1510A 转换引起的,导致第 487 位的谷氨酸被赖氨酸取代。不同 ALDH2 基因型的人对癌症、代谢疾病等的易感性不同。基于荧光探针介导的熔解曲线的 SNP 分析是一种相对高效且具有成本效益的方法。从 100 个全血样本中提取基因组 DNA,使用不对称 PCR 和探针介导的熔解曲线进行多态性突变分析。然后,从每种基因型中随机选择一定数量的样本进行直接测序验证。新的检测方法可以在 2 小时内完成,无需进行凝胶电泳等 PCR 后处理,并通过 100%一致性的盲法测序验证。此外,通过与临床检测 ALDH2 多态性的比较,显示出 100%(100/100)的总体一致性。我们的研究表明,DNA 测序具有高度的一致性,适用于临床标本的检测。基于探针介导的熔解曲线的概念,我们进一步将该平台开发为一种通用的叶酸代谢相关多态性检测策略。

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