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Long PCR for VNTR analysis.

机译:用于VNTR分析的长PCR。

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摘要

The Polymerase Chain Reaction (PCR) has revolutionized the analysis of DNA from a variety of sources. With its sensitivity and ability to amplify degraded DNAs and small quantities of samples, coupled with fast turn-around-time, PCR is often the analytical method of choice for DNA profiling in forensic laboratories. RFLP methods, while requiring larger amounts of high molecular weight DNA and needing approximately 6-8 weeks of analytical time, still provide a higher power of discrimination per locus than that achieved using the loci currently available for PCR. The combination of both RFLP and PCR would be advantageous for some applications. A new technique, Long PCR, allows for the effective amplification of long DNA targets from approximately 0.5 kb to > 20 kb of genomic DNA. Currently, several Long PCR systems are commercially available. Using a Taq/Pyrococcus DNA polymerase enzyme system and DNA isolated from bloodstains, we have successfully amplified 1-20 ng of Chelex-extracted DNA, an amount commonly used in Amp-FLP technology. The robustness of Long PCR in comparison to RFLP was also examined through the use of partially degraded blood samples. Long PCR was then used to amplify both D2S44 and D5S110 RFLP loci. Although all D2 and D5 alleles were detected, the larger alleles were amplified at significantly lower levels than the smaller alleles.
机译:聚合酶链反应(PCR)彻底改变了来自各种来源的DNA分析。由于具有灵敏度高,能够扩增降解的DNA和少量样品的能力以及快速的转换时间,PCR通常是法医实验室进行DNA分析的首选分析方法。 RFLP方法虽然需要大量的高分子量DNA,并且需要大约6-8周的分析时间,但仍提供了比使用当前可用于PCR的基因座更高的每个基因座判别能力。 RFLP和PCR的结合对于某些应用将是有利的。 Long PCR是一种新技术,可将长DNA靶标有效地扩增出大约0.5 kb至> 20 kb的基因组DNA。当前,几种长PCR系统是可商购的。使用Taq /火球菌DNA聚合酶系统和从血迹中分离的DNA,我们已成功扩增了1-20 ng Chelex提取的DNA,这是Amp-FLP技术中常用的量。通过使用部分降解的血样,还检验了Long PCR与RFLP相比的稳健性。然后使用长PCR扩增D2S44和D5S110 RFLP基因座。尽管检测到所有D2和D5等位基因,但较大的等位基因的扩增水平明显低于较小的等位基因。

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