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多重模板聚合酶链反应

Multi-template polymerase chain reaction.

作者信息

Kalle Elena, Kubista Mikael, Rensing Christopher

机构信息

Department of Forest Mycology and Plant Pathology, Swedish University of Agricultural Sciences, Allmas alle 5, 75007 Uppsala, Sweden.

TATAA Biocenter, Odinsgatan 28, 41103 Göteborg, Sweden; Institute of Biotechnology, Czech Academy of Sciences.

出版信息

Biomol Detect Quantif. 2014 Dec 4;2:11-29. doi: 10.1016/j.bdq.2014.11.002. eCollection 2014 Dec.

Abstract

PCR is a formidable and potent technology that serves as an indispensable tool in a wide range of biological disciplines. However, due to the ease of use and often lack of rigorous standards many PCR applications can lead to highly variable, inaccurate, and ultimately meaningless results. Thus, rigorous method validation must precede its broad adoption to any new application. Multi-template samples possess particular features, which make their PCR analysis prone to artifacts and biases: multiple homologous templates present in copy numbers that vary within several orders of magnitude. Such conditions are a breeding ground for chimeras and heteroduplexes. Differences in template amplification efficiencies and template competition for reaction compounds undermine correct preservation of the original template ratio. In addition, the presence of inhibitors aggravates all of the above-mentioned problems. Inhibitors might also have ambivalent effects on the different templates within the same sample. Yet, no standard approaches exist for monitoring inhibitory effects in multitemplate PCR, which is crucial for establishing compatibility between samples.

摘要

聚合酶链反应(PCR)是一项强大且有效的技术,在广泛的生物学学科中都是不可或缺的工具。然而,由于其使用简便且往往缺乏严格的标准,许多PCR应用可能会导致结果高度可变、不准确,最终毫无意义。因此,在将其广泛应用于任何新的领域之前,必须进行严格的方法验证。多模板样本具有特殊的特征,这使得它们的PCR分析容易产生假象和偏差:多个同源模板以数量级变化的拷贝数存在。这种情况是嵌合体和异源双链体的滋生地。模板扩增效率的差异以及模板对反应化合物的竞争破坏了原始模板比例的正确保存。此外,抑制剂的存在会加剧上述所有问题。抑制剂对同一样本中的不同模板也可能产生矛盾的影响。然而,在多模板PCR中,不存在用于监测抑制作用的标准方法,而这对于确定样本之间的兼容性至关重要。

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