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首页> 外文期刊>Molecular and Cellular Probes: The Location, Diagnosis and Monitoring of Disease by Specific Molecules and Cell Lines >Accuracy and sensitivity of DNA pooling with microsatellite repeats using capillary electrophoresis.
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Accuracy and sensitivity of DNA pooling with microsatellite repeats using capillary electrophoresis.

机译:使用毛细管电泳的微卫星重复DNA合并的准确性和敏感性。

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摘要

DNA pooling is a genetic screening method that combines DNA from many individuals in a single polymerase chain reaction (PCR) reaction to generate a representation of allele frequencies. The substantial saving in effort with DNA pooling over individual genotyping facilitates linkage disequilibrium scanning of the human genome using many thousands of genetic markers, and is applicable to mapping of complex diseases such as schizophrenia. However, the literature to date has not addressed several crucial technical aspects of DNA pooling. These include: DNA quantification; the choice of electrophoresis methods; sensitivity (the minimum reliably detectable difference between pools); and methods of dealing with 'plus-A' stutter. We have examined these points and make recommendations as to the best procedures to adopt as well as quantifying reproducibility and sensitivity. We conclude that, although allele frequencies derived from microsatellite pooling are distorted, differences of 5% or greater between pools can be reliably detected. Copyright 1999 Academic Press.
机译:DNA汇集是一种遗传筛选方法,它将来自多个个体的DNA结合在一个聚合酶链反应(PCR)反应中,以生成等位基因频率的表示。与单个基因型分型相比,DNA合并所节省的大量精力有助于使用数千种遗传标记物对人类基因组进行连锁不平衡扫描,并且适用于复杂疾病(如精神分裂症)的作图。但是,迄今为止,文献尚未涉及DNA合并的几个关键技术方面。其中包括:DNA定量;电泳方法的选择;灵敏度(池之间的最小可靠可检测差异);以及处理“加号A”口吃的方法。我们已经检查了这些要点,并就采用的最佳程序以及量化可重复性和敏感性提出了建议。我们得出的结论是,尽管源自微卫星池的等位基因频率发生了畸变,但是池之间的5%或更大的差异可以被可靠地检测到。版权所有1999 Academic Press。

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