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首页> 外文期刊>Molecular human reproduction. >Quantification of the common deletion in human testicular mitochondrial DNA by competitive PCR assay using a chimaeric competitor.
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Quantification of the common deletion in human testicular mitochondrial DNA by competitive PCR assay using a chimaeric competitor.

机译:通过使用chimaeric竞争者的竞争PCR分析定量人类睾丸线粒体DNA中的常见缺失。

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摘要

The "common" 4977 bp deletion in mitochondrial DNA (Delta4977) is commonly used as an indicator of tissue deterioration in ageing and bioenergetic diseases. Deletion levels are normally measured by a serial dilution polymerase chain reaction (PCR) approach, where test reactions are compared with dilutions of control amplifications of DNA from a similar sized stable region of the mitochondrial genome. The end-point of this assay is the dilution that can just detect any PCR product; however, this is an inherently unstable measure. We constructed a chimaeric DNA construct that binds to both control and deletion primers with similar annealing properties. This was used in a competitive PCR assay to quantify Delta4977 in human testicular tissues that had been well-characterized using the serial dilution approach. We found the competitive assay to be highly replicable as it compares the PCR product of the construct with that of test DNA samples during the linear growth phase of the PCR reaction. Moreover, the serial dilution assay was shown to significantly overestimate the amounts of deleted mitochondrial DNA present. The assay promises to throw new light on the role of mitochondrial DNA deletions in tissue dysfunction and ageing, as such deletions can now be determined with high accuracy and repeatability and is much cheaper to apply than real-time fluorescent quantitative PCR.
机译:线粒体DNA(Delta4977)中的“常见” 4977 bp缺失通常用作衰老和生物能疾病中组织退化的指标。缺失水平通常通过连续稀释聚合酶链反应(PCR)方法测量,其中将测试反应与来自线粒体基因组相似大小稳定区域的DNA的控制扩增的稀释度进行比较。该测定的终点是可以检测任何PCR产物的稀释液。但是,这是一种固有的不稳定措施。我们构建了一个嵌合DNA结构,可与具有相似退火特性的控制和缺失引物结合。将其用于竞争性PCR分析中,以定量检测使用系列稀释法已很好表征的人睾丸组织中的Delta4977。我们发现竞争性测定法具有高度可复制性,因为它在PCR反应的线性生长阶段将构建体的PCR产物与测试DNA样品的产物进行了比较。而且,显示出连续稀释测定法显着高估了存在的缺失的线粒体DNA的量。该测定有望为线粒体DNA缺失在组织功能障碍和衰老中的作用提供新的思路,因为这种缺失现在可以高精度和可重复性确定,并且比实时荧光定量PCR便宜得多。

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