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Simple and Versatile Molecular Method of Copy-Number Measurement Using Cloned Competitors

机译:使用克隆竞争者测量拷贝数的简单而多功能的分子方法

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摘要

Variations and alterations of copy numbers (CNVs and CNAs) carry disease susceptibility and drug responsiveness implications. Although there are many molecular methods to measure copy numbers, sensitivity, reproducibility, cost, and time issues remain. In the present study, we were able to solve those problems utilizing our modified real competitive PCR method with cloned competitors (mrcPCR). First, the mrcPCR for ERBB2 copy number was established, and the results were comparable to current standard methods but with a shorter assay time and a lower cost. Second, the mrcPCR assays for 24 drug-target genes were established, and the results in a panel of NCI-60 cells were comparable to those from real-time PCR and microarray. Third, the mrcPCR results for FCGR3A and the FCGR3B CNVs were comparable to those by the paralog ratio test (PRT), but without PRT's limitations. These results suggest that mrcPCR is comparable to the currently available standard or the most sensitive methods. In addition, mrcPCR would be invaluable for measurement of CNVs in genes with variants of similar structures, because combination of the other methods is not necessary, along with its other advantages such as short assay time, small sample amount requirement, and applicability to all sequences and genes.
机译:拷贝数(CNV和CNA)的变化和改变带有疾病易感性和药物反应性。尽管有许多分子方法可以测量拷贝数,但是灵敏度,可重复性,成本和时间问题仍然存在。在本研究中,我们能够利用我们的改进的真实竞争PCR方法和克隆竞争者(mrcPCR)解决这些问题。首先,建立了用于ERBB2拷贝数的mrcPCR,其结果与当前的标准方法相当,但测定时间较短且成本较低。其次,建立了针对24种药物靶基因的mrcPCR检测方法,一组NCI-60细胞的结果与实时PCR和微阵列的结果相当。第三,FCGR3A和FCGR3B CNV的mrcPCR结果可与旁系同源比测试(PRT)相比,但不受PRT的限制。这些结果表明,mrcPCR与目前可用的标准或最敏感的方法具有可比性。此外,mrcPCR对于测量具有相似结构变体的基因中的CNV来说将是无价的,因为不需要其他方法的结合,同时它还具有其他优点,例如检测时间短,样品量少,适用于所有序列和基因。

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