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Optimal primer design using the novel primer design program: MSPprimer provides accurate methylation analysis of the ATM promoter

机译:使用新型引物设计程序的最佳引物设计:MSPprimer提供ATM启动子的准确甲基化分析

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摘要

Methylation-specific polymerase chain reaction (PCR) (MSP) is frequently used to study gene silencing by promoter hypermethylation. However, non-specific primer design can lead to false-positive detection of methylation. We present a novel, web-based algorithm for the design of primers for bisulfite-PCRs (MSP, sequencing, COBRA and multiplex-MSP), allowing the determination of a specificity score, which is based on the thermodynamic characteristics of the primer 3'-end. PCR amplification with primers not reaching a high specificity score can result in false-positive findings. We used MSPprimer to design MSP primers for analysis of the ATM promoter. In 37 non-small cell lung cancer (NSCLC) samples and 43 breast cancer samples no promoter methylation was detected. Conversely, published MSP primers not reaching the required specificity score led to non-specific amplification of DNA not converted by bisulfite. The result was a false-positive incidence of ATM promoter methylation of 24% in NSCLC and 48% in breast cancers, similar to published studies. This highlights the critical need for specific primer design for MSP. MSPprimer is a convenient tool to achieve this goal, which is available free of charge to the scientific community.
机译:甲基化特异性聚合酶链反应(PCR)(MSP)通常用于研究启动子超甲基化引起的基因沉默。但是,非特异性引物设计可能导致甲基化的假阳性检测。我们提出了一种基于网络的新颖算法,用于设计亚硫酸氢盐-PCR的引物(MSP,测序,COBRA和Multiple-MSP),从而可以基于引物3'的热力学特性确定特异性得分。 -结束。用未达到高特异性评分的引物进行PCR扩增可能会导致假阳性结果。我们使用MSPprimer设计MSP引物来分析ATM启动子。在37个非小细胞肺癌(NSCLC)样本和43个乳腺癌样本中,未检测到启动子甲基化。相反,已发布的MSP引物未达到所需的特异性得分,则导致了非亚硫酸氢盐转化的DNA的非特异性扩增。结果是,NSCLC中ATM启动子甲基化的假阳性发生率为24%,在乳腺癌中为48%,类似于已发表的研究。这突显了MSP特定底漆设计的迫切需求。 MSPprimer是实现此目标的便捷工具,科学界可以免费使用。

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