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首页> 外文期刊>Analytical Sciences >Direct Detection of Mutant DNA in a Mixed Population of Higher Copy Number Wild-Type DNA Based on Ligase Detection Reaction in Conjunction with Fluorescence Resonance Energy Transfer
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Direct Detection of Mutant DNA in a Mixed Population of Higher Copy Number Wild-Type DNA Based on Ligase Detection Reaction in Conjunction with Fluorescence Resonance Energy Transfer

机译:基于连接酶检测反应的荧光共振能量转移,直接检测较高拷贝数野生型DNA的混合群中的突变DNA

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摘要

We have developed an analytical system capable of detecting point mutations in a higher copy number of wild-type DNA based on an allele-specific ligase detection reaction (LDR) in conjunction with fluorescence resonance energy transfer (FRET). Streptavidin-functionalized quantum dots (QDs) used as FRET donors effectively captured biotinylated LDR products (target DNA strands) labeled with fluorophores as a FRET acceptor, enabling the formation of a sensitive energy transfer pair and direct detection of the targets without any post-LDR separation process, which is generally required for the LDR-based mutation analysis. Our experiments indicated that the present system had an ability to detect one mutant sequence in 10 normal sequences at a signal-to-background ratio of ca. 3.9.
机译:我们开发了一种能够基于荧光共振能量转移(FRET)的等位基因特异性连接酶检测反应(LDR)来检测野生型DNA的较高拷贝数量的点突变的分析系统。用作Fret供体的链霉抗生物素蛋白官能化量子点(QDS)有效地捕获了用荧光团标记的生物素化的LDR产品(靶DNA链)作为荧光剂,能够形成敏感能量转移对并直接检测没有任何后LDR的目标分离过程,通常需要基于LDR的突变分析。我们的实验表明,本系统能够在CA的信号到背景比下检测10个正常序列中的一种突变序列。 3.9。

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