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Critical evaluation of methods used to determine amplification efficiency refutes the exponential character of real-time PCR

机译:对用于确定扩增效率的方法的严格评估反驳了实时PCR的指数特征

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摘要

BackgroundThe challenge of determining amplification efficiency has long been a predominant aspect of implementing real-time qPCR, playing a critical role in the accuracy and reliability that can be achieved. Based upon analysis of amplification profile position, standard curves are currently the gold standard for amplification efficiency determination. However, in addition to being highly resource intensive, the efficacy of this approach is limited by the necessary assumption that all samples are amplified with the same efficiency as predicted by a standard curve. These limitations have driven efforts to develop methods for determining amplification efficiency by analyzing the fluorescence readings from individual amplification reactions. The most prominent approach is based on analysis of the "log-linear region", founded upon the presumption that amplification efficiency is constant within this region. Nevertheless, a recently developed sigmoidal model has provided new insights that challenge such historically held views, dictating that amplification efficiency is not only dynamic, but is linearly coupled to amplicon DNA quantity. Called "linear regression of efficiency" or LRE, this kinetic-based approach redefines amplification efficiency as the maximal efficiency (Emax) generated at the onset of thermocycling.
机译:背景技术确定扩增效率的挑战长期以来一直是实施实时qPCR的主要方面,在可实现的准确性和可靠性中起着至关重要的作用。基于对扩增曲线位置的分析,标准曲线目前是确定扩增效率的金标准。但是,除了需要大量资源外,此方法的有效性还受到以下必要假设的限制:所有样本均以与标准曲线所预测的相同效率进行扩增。这些局限性促使人们努力开发通过分析单个扩增反应的荧光读数来确定扩增效率的方法。最突出的方法是基于“对数线性区域”的分析,该假设基于在该区域内放大效率恒定的假设。然而,最近开发的S形模型提供了新的见解,挑战了这种历史观点,认为扩增效率不仅是动态的,而且与扩增子DNA的数量线性相关。这种基于动力学的方法称为“效率线性回归”或LRE,将扩增效率重新定义为热循环开始时产生的最大效率(Emax)。

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