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SNP Genotyping by Gel-immobilized ssDNA and Biolumometric Assay Coupled with Allele-specific Primer Extension Reaction

机译:通过凝胶固定化的SSDNA和生物测量测定与等位基因特异性引物延伸反应的SNP基因分型

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The new gel-immobilization method for preparing a single stranded DNA (ssDNA) template has been described for single nucleotide polymorphisms (SNPs) genotyping by bioluminometric assay based on allele-specfic extension reaction. In this method, PCR products amplified by a primer modified with acrylamide group at the 5'-terminal is copolymerized with acrylamide monomer to form gel. After the ssDNA immobilized on gel being denatured, the impurities are removed by electrophoresis. SNPs genotyping is performed by allele-specific primer extension reaction. The SNP type was identified by comparing the signal intensities from the extension by two allele specific primers hybridized on gel-mobilized ssDNA. If the 3' end of a primer is complementary to the template, polymerase extension occurs and pyrophosphate (PPi) released. The signal is produced by using PPi conversion and luciferase reactions. As many bases are extended in one extension reaction, the sensitivity of the method is very high. This new strategy of the ssDNA immobilization is robust, simple, and inexpensive. It can be used for various application of DNA analysis, such as SNP genotyping and pyrosequencing.
机译:已经基于等位基因测定法基于等位基因测定的对等核苷酸多态性(SNPS)基因分型来描述用于制备单链DNA(SSDNA)模板的新凝胶固定方法。在该方法中,通过在5'-末端用丙烯酰胺基改性的引物扩增的PCR产物与丙烯酰胺单体共聚以形成凝胶。在固定在凝胶上被变性的SSDNA后,通过电泳除去杂质。 SNPS基因分型由等位基因特异性引物延伸反应进行。通过将来自延伸的信号强度与在凝胶化的SSDNA上杂交的两个等位基因特异性引物进行比较来鉴定SNP型。如果引物的3'末端与模板互补,则发生聚合酶延伸和溶解的焦磷酸盐(PPI)。通过使用PPI转化和荧光素酶反应产生信号。随着许多碱基在一个延伸反应中延伸,该方法的灵敏度非常高。 SSDNA固定化的新策略是强大,简单,廉价的。它可用于DNA分析的各种应用,例如SNP基因分型和焦磷酸盐。

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