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Assessment of Primer/Template Mismatch Effects on Real-Time PCR Amplification of Target Taxa for GMO Quantification

机译:评估引物/模板错配对目标生物分类的实时PCR扩增的定量影响

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GMO quantification, based on real-time PCR, relies on the amplification of an event-specific transgene assay and a species-specific reference assay. The uniformity of the nucleotide sequences targeted by both assays across various transgenic varieties is an important prerequisite for correct quantification. Single nucleotide polymorphisms (SNPs) frequently occur in the maize genome and might lead to nucleotide variation in regions used to design primers and probes for reference assays. Further, they may affect the annealing of the primer to the template and reduce the efficiency of DNA amplification. We assessed the effect of a minor DNA template modification, such as a single base pair mismatch in the primer attachment site, on real-time PCR quantification. A model system was used based on the introduction of artificial mismatches between the forward primer and the DNA template in the reference assay targeting the maize starch synthase (SSIIb) gene. The results show that the presence of a mismatch between the primer and the DNA template causes partial to complete failure of the amplification of the initial DNA template depending on the type and location of the nucleotide mismatch. With this study, we show that the presence of a primer/template mismatch affects the estimated total DNA quantity to a varying degree.
机译:基于实时PCR的GMO定量依赖事件特异性转基因测定和物种特异性参考测定的扩增。两种测定法在各种转基因品种中靶向的核苷酸序列的一致性是正确定量的重要前提。单核苷酸多态性(SNP)经常发生在玉米基因组中,并可能导致核苷酸区域发生变异,这些区域用于设计引物和探针以供参考检测。此外,它们可能影响引物与模板的退火并降低DNA扩增的效率。我们评估了实时PCR定量中较小的DNA模板修饰(例如引物附着位点中的单个碱基对错配)的影响。基于在针对玉米淀粉合酶(SSIIb)基因的参考测定中正向引物和DNA模板之间的人工错配的引入,使用了模型系统。结果表明,取决于核苷酸错配的类型和位置,引物和DNA模板之间存在错配会导致部分初始DNA模板的扩增完全失败。通过这项研究,我们表明引物/模板错配的存在会在不同程度上影响估计的总DNA量。

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