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用于DNA准确定量的竞争性PCR的理论与实验剖析

Theoretical and experimental dissection of competitive PCR for accurate quantification of DNA.

作者信息

Hirano Tetsuo, Haque Masudul, Utiyama Hiroyasu

机构信息

The Life Science Group, Faculty of Integrated Arts and Sciences, Hiroshima University, Hiroshima 739-8521, Japan.

出版信息

Anal Biochem. 2002 Apr 1;303(1):57-65. doi: 10.1006/abio.2001.5573.

Abstract

We frequently use competitive PCR in the plateau phase in quantifying DNA species with a small number of cells. However, the basic issues of this method are poorly understood. Here, first we analyze this method theoretically under a generalized condition that competitor and target DNA products accumulate with different amplification efficiencies. We show a theoretical reason that competitive PCR might quantify DNA more accurately during the plateau phase than during the exponential phase. Second, we demonstrate that the theoretical predictions are supported by the experimental results of beta-globin gene amplification using the lysates of human diploid fibroblast WS1 cells. We also demonstrate that we can correctly quantify target DNA by keeping the starting concentration of target DNA close to a constant preset value while using a constant number of PCR cycles and by using WS1 cells as control. Finally, we show the experimental errors in routine measurements of c-myc copy number/cell in human leukemia HL-60 cells with various levels of c-myc multiplication. The number of c-myc copies/cell was determined with an error rate of less than 10%, where agarose gel bands were stained with ethidium bromide for the product quantitation.

摘要

我们经常在平台期使用竞争性PCR来定量少量细胞中的DNA种类。然而,对该方法的基本问题了解甚少。在此,首先我们在一个广义条件下对该方法进行理论分析,即竞争物和靶DNA产物以不同的扩增效率积累。我们给出了一个理论依据,说明竞争性PCR在平台期可能比指数期更准确地定量DNA。其次,我们证明这些理论预测得到了使用人二倍体成纤维细胞WS1细胞裂解物进行β-珠蛋白基因扩增的实验结果的支持。我们还证明,在使用固定数量的PCR循环并以WS1细胞作为对照时,通过使靶DNA的起始浓度接近一个恒定的预设值,我们可以正确地定量靶DNA。最后,我们展示了在具有不同c-myc增殖水平的人白血病HL-60细胞中常规测量c-myc拷贝数/细胞时的实验误差。当用溴化乙锭对琼脂糖凝胶条带进行染色以进行产物定量时,确定c-myc拷贝数/细胞的误差率小于10%。

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