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Single nucleotide polymorphism genotyping using short, fluorescently labeled locked nucleic acid (LNA) probes and fluorescence polarization detection

机译:使用短的荧光标记锁定核酸(LNA)探针和荧光偏振检测进行单核苷酸多态性基因分型

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摘要

Locked nucleic acids (LNAs) are synthetic nucleic acid analogs that bind to complementary target molecules (DNA, RNA or LNA) with very high affinity. At the same time, this binding affinity is decreased substantially when the hybrids thus formed contain even a single mismatched base pair. We have exploited these properties of LNA probes to develop a new method for single nucleotide polymorphism genotyping. In this method, very short (hexamer or heptamer) LNA probes are labeled with either rhodamine or hexachlorofluorescein (HEX), and their hybridization to target DNAs is followed by measuring the fluorescence polarization (FP) of the dyes. The formation of perfectly complementary double-stranded hybrids gives rise to significant FP increases, whereas the presence of single mismatches results in very small or no changes of this parameter. Multiplexing of the assay can be achieved by using differentially labeled wild-type and mutant specific probes in the same solution. The method is homogeneous, and because of the use of extremely short LNA probes, the generation of a universal set of genotyping reagents is possible.
机译:锁定核酸(LNA)是合成核酸类似物,它们以非常高的亲和力与互补靶分子(DNA,RNA或LNA)结合。同时,当由此形成的杂合体甚至包含单个错配的碱基对时,该结合亲和力大大降低。我们已经利用LNA探针的这些特性来开发一种用于单核苷酸多态性基因分型的新方法。在这种方法中,用若丹明或六氯荧光素(HEX)标记非常短的(六聚体或七聚体)LNA探针,然后将它们与目标DNA杂交,然后测量染料的荧光偏振(FP)。完美互补的双链杂种的形成引起显着的FP增加,而单个错配的存在导致该参数的改变很小或没有改变。可以通过在同一溶液中使用差异标记的野生型和突变型特异性探针来实现测定的复用。该方法是均一的,并且由于使用了非常短的LNA探针,因此可以生成通用的基因分型试剂集。

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