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首页> 外文期刊>Combinatorial Chemistry & High Throughput Screening >PCR/SSCP Detects Reliably and Efficiently DNA Sequence Variations in Large Scale Screening Projects
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PCR/SSCP Detects Reliably and Efficiently DNA Sequence Variations in Large Scale Screening Projects

机译:PCR / SSCP可在大规模筛选项目中可靠且有效地检测DNA序列变异

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摘要

A simple and fast method with high reliability is necessary for the identification of mutations, polymorphisms and sequence variants (MPSV) within many genes and many samples, e.g. for clarifying the genetic background of individuals with multifactorial diseases. Here we review our experience with the polymerase chain reaction/single-strand conformation polymorphism (PCR/SSCP) analysis to identify MPSV in a number of genes thought to be involved in the pathogenesis of multifactorial neurological disorders, including autoimmune diseases like multiple sclerosis (MS) and neurodegenerative disorders like Parkinsons disease (PD). The method is based on the property of the DNA that the electrophoretic mobility of single stranded nucleic acids depends not only on their size but also on their sequence. The target sequences were amplified, digested into fragments ranging from 50-240 base pairs (bp), heat-denatured and analysed on native polyacrylamide (PAA) gels of different composition. The analysis of a gre at number of different PCR products demonstrates that the detection rate of MPSV depends on the fragment lengths, the temperature during electrophoresis and the composition of the gel. In general, the detection of MPSV is neither influenced by their location within the DNA fragment nor by the type of substitution, i.e., transitions or transversions. The standard PCR/SSCP system described here provides high reliability and detection rates. It allows the efficient analysis of a large number of DNA samples and many different genes.
机译:为了鉴定许多基因和许多样品(例如,大肠杆菌)中的突变,多态性和序列变异(MPSV),需要一种具有高可靠性的简单快速方法。阐明多因素疾病患者的遗传背景。在这里,我们回顾了我们在聚合酶链反应/单链构象多态性(PCR / SSCP)分析中的经验,以鉴定出与多因素神经系统疾病的发病机理有关的许多基因中的MPSV,包括多发性硬化症(MS)等自身免疫性疾病)和神经退行性疾病(如帕金森病(PD))。该方法基于DNA的特性,即单链核酸的电泳迁移率不仅取决于其大小,还取决于其序列。扩增靶序列,消化成50-240个碱基对(bp)的片段,热变性并在不同组成的天然聚丙烯酰胺(PAA)凝胶上进行分析。对许多不同PCR产物的gre的分析表明,MPSV的检测率取决于片段长度,电泳过程中的温度和凝胶的组成。通常,MPSV的检测既不受它们在DNA片段内的位置的影响,也不受取代类型即过渡或颠换的影响。此处描述的标准PCR / SSCP系统具有很高的可靠性和检测率。它可以有效分析大量DNA样品和许多不同的基因。

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