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一种用于测定人类核DNA和线粒体DNA数量与质量的模块化实时荧光定量PCR概念。

A modular real-time PCR concept for determining the quantity and quality of human nuclear and mitochondrial DNA.

作者信息

Niederstätter Harald, Köchl Silvano, Grubwieser Petra, Pavlic Marion, Steinlechner Martin, Parson Walther

机构信息

Institute of Legal Medicine, Innsbruck Medical University, Innsbruck, Austria.

出版信息

Forensic Sci Int Genet. 2007 Mar;1(1):29-34. doi: 10.1016/j.fsigen.2006.10.007. Epub 2006 Nov 30.

Abstract

We developed a modular real-time (rt) PCR system for absolute quantification of human nuclear (n) and mitochondrial (mt) DNA. For determination of the number of amplifiable template molecules with a minimum length required for downstream genotyping and assessment of the PCR-relevant degradation grade of the template DNA, primers yielding differently sized PCR products (nDNA: 79, 156, and 246 bp; mtDNA: 102, 143, 283, and 404 bp) and TaqMan hybridization probes were used for amplification and on-line product detection. DNase-degraded DNA served as model to demonstrate the effects of DNA fragmentation on rtPCR quantification and subsequent genotyping. Introduction of cloned internal amplification positive controls (IPCs)--generated by in vitro mutagenesis of primer-binding sites of the wild-type nDNA and mtDNA targets--enabled functionality-testing of the reaction mixture and detection of PCR inhibitors in DNA extracts, without a need for additional TaqMan probes. A hematin model was used to test the ability of the quantitative real-time (rtq) PCR system to predict the effects of inhibitors in downstream PCR-based genotyping.

摘要

我们开发了一种用于绝对定量人类核(n)DNA和线粒体(mt)DNA的模块化实时(rt)PCR系统。为了确定具有下游基因分型所需最小长度的可扩增模板分子数量,并评估模板DNA的PCR相关降解程度,使用产生不同大小PCR产物的引物(nDNA:79、156和246 bp;mtDNA:102、143、283和404 bp)和TaqMan杂交探针进行扩增和在线产物检测。DNase降解的DNA用作模型,以证明DNA片段化对rtPCR定量和后续基因分型的影响。引入通过对野生型nDNA和mtDNA靶标的引物结合位点进行体外诱变产生的克隆内部扩增阳性对照(IPC),能够对反应混合物进行功能测试并检测DNA提取物中的PCR抑制剂,而无需额外的TaqMan探针。使用血红素模型测试定量实时(rtq)PCR系统预测下游基于PCR的基因分型中抑制剂影响的能力。

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