Digital polymerase chain reaction for characterisation of DNA reference materials

Q1 Biochemistry, Genetics and Molecular Biology

Biomolecular Detection and Quantification Pub Date : 2016-12-01 DOI:10.1016/j.bdq.2016.04.001

Somanath Bhat, Kerry R. Emslie

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引用次数: 27

Abstract

Accurate, reliable and reproducible quantification of nucleic acids (DNA/RNA) is important for many diagnostic applications and in routine laboratory testing, for example, for pathogen detection and detection of genetically modified organisms in food. To ensure reliable nucleic acid measurement, reference materials (RM) that are accurately characterised for quantity of target nucleic acid sequences (in copy number or copy number concentration) with a known measurement uncertainty are needed. Recently developed digital polymerase chain reaction (dPCR) technology allows absolute and accurate quantification of nucleic acid target sequences without need for a reference standard. Due to these properties, this technique has the potential to not only improve routine quantitative nucleic acid analysis, but also to be used as a reference method for certification of nucleic acid RM. The article focuses on the use and application of both dPCR and RMs for accurate quantification.

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数字聚合酶链反应用于鉴定DNA参比物

准确、可靠和可重复的核酸(DNA/RNA)定量对于许多诊断应用和常规实验室检测非常重要，例如用于病原体检测和食品中转基因生物的检测。为了确保可靠的核酸测量，需要具有已知测量不确定度的标准物质(RM)，以准确表征目标核酸序列的数量(拷贝数或拷贝数浓度)。最近发展的数字聚合酶链反应(dPCR)技术可以在不需要参考标准的情况下绝对准确地定量核酸靶标序列。由于这些特性，该技术不仅具有改进常规核酸定量分析的潜力，而且可以作为核酸RM认证的参考方法。本文重点介绍了dPCR和均方根法用于准确定量的使用和应用。

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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