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PCR inhibition by reverse transcriptase leads to an overestimation of amplification efficiency

机译:逆转录酶抑制PCR会导致高估扩增效率

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摘要

This study addresses the problem of PCR inhibition by reverse transcriptase. It has been shown that the inhibition occurs mostly when a small amount of RNA is taken for RT reaction, and it is more visible for rarely expressed transcripts. We show here that the inhibition takes place regardless of what amount of template is utilized for RT. The inhibition possesses a global nature, i.e. the amplification of any given transcript may be compromised with different levels of inhibition. The process of inhibition also explains wrongfully derived PCR amplification efficiencies, sometimes more than 100%, when the sequential dilutions of unpurified RT sample are utilized to build the calibration curve. The RT influences PCR not only by inhibiting it. When microgram(s) of RNA are taken for RT reaction, reverse transcriptase may cause overamplification of some transcripts under certain PCR conditions. The possible mechanism of RT influence on PCR is presented, and a purification method is implemented to remove the effects of RT on PCR.
机译:这项研究解决了逆转录酶抑制PCR的问题。已经显示,抑制主要发生在少量的RNA用于RT反应时,而对于很少表达的转录本则更明显。我们在这里表明,无论使用多少模板进行RT抑制都会发生。抑制具有全局性质,即,任何给定转录物的扩增可能受到不同程度的抑制的损害。当使用未纯化的RT样品的连续稀释液建立校正曲线时,抑制过程还解释了错误地得出的PCR扩增效率,有时超过100%。 RT不仅仅通过抑制PCR来影响PCR。当将微克RNA进行RT反应时,逆转录酶可能会在某些PCR条件下引起某些转录物的过度扩增。提出了RT影响PCR的可能机制,并提出了纯化方法以消除RT对PCR的影响。

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