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涉及16个基因位点的快速多重聚合酶链反应扩增的演示。

Demonstration of rapid multiplex PCR amplification involving 16 genetic loci.

作者信息

Vallone Peter M, Hill Carolyn R, Butler John M

机构信息

National Institute of Standards and Technology, Biochemical Science Division, 100 Bureau Drive, Mail Stop 8311, Gaithersburg, MD 20899-8311, USA.

出版信息

Forensic Sci Int Genet. 2008 Dec;3(1):42-5. doi: 10.1016/j.fsigen.2008.09.005. Epub 2008 Oct 26.

Abstract

Current forensic DNA typing is conducted in approximately 8-10h. Steps include DNA extraction, quantification, polymerase chain reaction (PCR) amplification of multiple short tandem repeat (STR) loci, capillary electrophoresis separation with fluorescence detection, data analysis and DNA profile interpretation. The PCR amplification portion of the workflow typically takes approximately 3h with standard thermal cycling protocols. Here we demonstrate a rapid cycling protocol that amplifies 15 STR loci and the sex-typing marker amelogenin from the Identifiler STR typing kit in less than 36 min. This rapid protocol employs commercially available polymerases and the widely used GeneAmp 9700 thermal cycler. Complete concordance of STR allele calls (for 60 samples) between the rapid and standard thermal cycling protocols were observed although there was incomplete adenylation at several of the loci examined and some PCR artifacts were detected. Using less than 750 pg of template DNA and 28 cycles, STR peaks for all loci were above a 150 relative fluorescent unit (RFU) detection threshold with fully adequate inter-locus balance and heterozygote peak height ratios of greater than 0.84.

摘要

目前法医DNA分型检测大约需要8至10小时。步骤包括DNA提取、定量、对多个短串联重复序列(STR)位点进行聚合酶链反应(PCR)扩增、通过荧光检测进行毛细管电泳分离、数据分析以及DNA图谱解读。采用标准热循环方案时,工作流程中的PCR扩增部分通常耗时约3小时。在此,我们展示了一种快速循环方案,该方案能在不到36分钟的时间内,从Identifiler STR分型试剂盒中扩增出15个STR位点和性别分型标记物牙釉蛋白。这种快速方案使用市售聚合酶和广泛应用的GeneAmp 9700热循环仪。尽管在检测的几个位点存在不完全腺苷酸化现象且检测到一些PCR假象,但快速热循环方案与标准热循环方案之间的STR等位基因分型(针对60个样本)完全一致。使用不到750 pg的模板DNA和28个循环,所有位点的STR峰均高于150相对荧光单位(RFU)的检测阈值,基因座间平衡充分,杂合子峰高比大于0.84。

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