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Fluorescence resonance energy transfer (FRET) using ssDNA binding fluorescent dye

机译:使用ssDNA结合荧光染料的荧光共振能量转移(FRET)

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摘要

There is a need for simple and inexpensive methods for genotyping single nucleotide polymorphisms (SNPs) and short insertion/deletion variations (InDels). In this work, I demonstrate that a single-stranded DNA (ssDNA) binding dye can be used as a donor fluorophore for fluorescence resonance energy transfer (FRET). The method presented is a homogenous assay in which detection is based on the FRET from the fluorescence of the ssDNA dye bound to the unmodified detection primer to the fluorescent nucleotide analog incorporated into this detection primer during cyclic template directed primer extension reaction. Collection of the FRET emission spectrum with a scanning fluorescence spectrophotometer allows powerful data analysis. The fluorescence emission signal is modified by the optical properties of the assay vessel. This seems to be a completely neglected parameter. By proper selection of the optical properties of the assay plate one can improve the detection of the fluorescence emission signal.
机译:需要用于对单核苷酸多态性(SNP)和短插入/缺失变异(InDels)进行基因分型的简单且廉价的方法。在这项工作中,我证明了单链DNA(ssDNA)结合染料可以用作荧光共振能量转移(FRET)的供体荧光团。提出的方法是一种均相测定,其中检测基于FRET,即从与未修饰的检测引物结合的ssDNA染料的荧光到在循环模板指导的引物延伸反应期间掺入该检测引物中的荧光核苷酸类似物。使用扫描荧光分光光度计收集FRET发射光谱可进行强大的数据分析。荧光发射信号被测定容器的光学性质所修饰。这似乎是一个完全被忽略的参数。通过适当选择测定板的光学性质,可以改善荧光发射信号的检测。

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