The polymerase chain reaction (PCR) is widely used for applications which require a high level of specificity and reliability, such as genetic testing, clinical diagnostics, blood screening, forensics and biodefense. Great improvements to PCR performance have been achieved by the use of Hot Start activation strategies that aim to prevent DNA polymerase extension until more stringent, higher temperatures are reached. Herein we present a novel Hot Start activation approach in PCR where primers contain one or two thermolabile, 4-oxo-1-pentyl (OXP) phosphotriester (PTE) modification groups at 3′-terminal and 3′-penultimate internucleotide linkages. Studies demonstrated that the presence of one or more OXP PTE modifications impaired DNA polymerase primer extension at the lower temperatures that exist prior to PCR amplification. Furthermore, incubation of the OXP-modified primers at elevated temperatures was found to produce the corresponding unmodified phosphodiester (PDE) primer, which was then a suitable DNA polymerase substrate. The OXP-modified primers were tested in conventional PCR with endpoint detection, in one-step reverse transcription (RT)–PCR and in real-time PCR with SYBR Green I dye and Taqman® probe detection. When OXP-modified primers were used as substitutes for unmodified PDE primers in PCR, significant improvement was observed in the specificity and efficiency of nucleic acid target amplification.
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机译:聚合酶链反应(PCR)广泛用于需要高水平特异性和可靠性的应用,例如基因检测,临床诊断,血液筛查,法医学和生物防御。通过使用热启动激活策略已实现了PCR性能的极大提高,该策略旨在防止DNA聚合酶延伸直到达到更严格的温度。本文中,我们提出了一种新颖的PCR热启动激活方法,其中引物在3'-末端和3'-倒数第二个核苷酸间键处包含一个或两个热不稳定的4-氧代-1-戊基(OXP)磷酸三酯(PTE)修饰基团。研究表明,一种或多种OXP PTE修饰的存在在PCR扩增之前的较低温度下会损害DNA聚合酶引物的延伸。此外,发现在高温下孵育OXP修饰的引物可产生相应的未修饰的磷酸二酯(PDE)引物,然后将其用作合适的DNA聚合酶底物。 OXP修饰的引物在带有终点检测的常规PCR,一步反转录(RT)–PCR和带有SYBR Green I染料和Taqman®探针检测的实时PCR中进行了测试。当OXP修饰的引物在PCR中用作未修饰的PDE引物的替代物时,观察到核酸靶标扩增的特异性和效率有了显着改善。
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