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首页> 外文期刊>Journal of chromatography, B. Analytical technologies in the biomedical and life sciences >Identification and separation of PCR products based on their GC content by denaturing high-performance liquid chromatography
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Identification and separation of PCR products based on their GC content by denaturing high-performance liquid chromatography

机译:通过变性高效液相色谱法基于GC含量鉴定和分离PCR产物

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We show that denaturing high-performance liquid chromatography is a suitable method for the separation of DNA molecules of similar sizes but with different GC contents. A mixture of homologous molecules coining from different bacterial species may be obtained when PCR with degenerate primers is used for the amplification of a specific gene from an environmental sample. We have observed that, by selecting an appropriate temperature for the partial denaturation of the molecules, we are able to separate them according to the GC content of each DNA product. This allows us to determine if one or several types of molecules are amplified in the course of a PCR reaction. In the latter case it is possible, even with minority products, to isolate them by collecting the eluted volumes, followed by cloning, sequencing or reamplifying them by PCR, depending on the DNA concentration. We have applied this analysis to the amplification of a fragment of the ribA gene in the bacterial endosymbionts of insects, obtaining a high correlation coefficient (0.978) between retention time and the GC content of the molecules. (C) 2004 Elsevier B.V. All rights reserved.
机译:我们表明,变性高效液相色谱法是一种合适的方法,用于分离大小相似但GC含量不同的DNA分子。当使用简并引物进行PCR扩增环境样品中的特定基因时,可以得到不同细菌物种产生的同源分子的混合物。我们已经观察到,通过为分子的部分变性选择合适的温度,我们能够根据每种DNA产物的GC含量将其分离。这使我们能够确定在PCR反应过程中是否扩增了一种或几种类型的分子。在后一种情况下,甚至对于少数产品,也可以通过收集洗脱体积来分离它们,然后根据DNA浓度通过PCR对其进行克隆,测序或再扩增。我们已将此分析应用于昆虫细菌内共生体中ribA基因片段的扩增,从而在分子的保留时间和GC含量之间获得了很高的相关系数(0.978)。 (C)2004 Elsevier B.V.保留所有权利。

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