Human Saliva and Dried Saliva Spots as Source of DNA for PCR based HLA Typing using a Combination of Taq DNA Polymerase and AccuPrimeTaq Polymerase

Walailak Journal of Science and Technology (WJST) Pub Date : 2019-02-28 DOI:10.48048/wjst.2020.4430

Prerana Madhusudhana Murthy, Anupama Cheleri Neduvat, Cheemalamarri Veenadhar, Sudarson Sundarrajan, S. Padmanabhan

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引用次数: 1

Abstract

Genomic DNA extracted from human saliva samples showed high inter-subject variations in DNA yield, compelling the need to explore a methodology for the accurate quantitation of the extracted genomic DNA. Quantitative assessment of DNA extracted from saliva was achieved using human coagulation factor XIII as an internal control for subsequent downstream applications of amplification of human leucocyte antigen (HLA) genes by PCR. The PCR signals for the HLA target genes, namely, HLA-A, -B, -C , DPB1, DQB1, and DRB1 of exons 2 and 3, improved greatly with the use of a combination of Taq DNA polymerase and AccuPrimeTaq DNA polymerase. We also describe a new method of using dried saliva spots (DSS) as an alternate source of genomic DNA for HLA typing. PCR-based typing of DNA from human saliva offers a potential method for HLA typing and amplification, and typing of DNA, thus presented, could be applied in forensic science to saliva samples recovered from crime scenes.

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用Taq DNA聚合酶和AccuPrimeTaq聚合酶联合检测人唾液和干唾液斑点作为HLA分型的DNA来源

从人类唾液样本中提取的基因组DNA在DNA产量方面显示出很高的学科间差异，迫切需要探索一种准确定量提取基因组DNA的方法。使用人凝血因子XIII作为内控物，对唾液中提取的DNA进行定量评估，随后通过PCR扩增人白细胞抗原(HLA)基因进行下游应用。Taq DNA聚合酶与AccuPrimeTaq DNA聚合酶联合使用后，HLA靶基因2、3外显子HLA- a、-B、-C、DPB1、DQB1、DRB1的PCR信号明显改善。我们还描述了一种使用干唾液斑点(DSS)作为HLA分型基因组DNA的替代来源的新方法。基于聚合酶链反应的人唾液DNA分型为HLA分型和扩增提供了一种潜在的方法，因此，DNA分型可以应用于法医学，用于从犯罪现场回收的唾液样本。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Walailak Journal of Science and Technology (WJST)

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