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Analysis of single nucleotide polymorphisms with solid phase invasive cleavage reactions

机译:固相侵入性裂解反应分析单核苷酸多态性

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Using microparticles as the capture surface and fluorescence resonance energy transfer as the detection technology, we have demonstrated the feasibility of performing the invasive cleavage reaction on a solid phase. An effective tool for many genomic applications, the solution phase invasive cleavage assay is a signal amplification method capable of distinguishing nucleic acids that differ by only a single base mutation. The method positions two overlapping oligonucleotides, the probe and upstream oligonucleotides, on the target nucleic acid to create a complex recognized and cleaved by a structure-specific 5′-nuclease. For microarray and other multiplex applications, however, the method must be adapted to a solid phase platform. Effective cleavage of the probe oligonucleotide occurred when either of the two required overlapping oligonucleotides was configured as the particle-bound reagent and also when both oligonucleotides were attached to the solid phase. Positioning probe oligonucleotides away from the particle surface via long tethers improved both the signal and the reaction rates. The particle-based invasive cleavage reaction was capable of distinguishing the ApoE Cys158 and Arg158 alleles at target concentrations as low as 100?amol/assay (0.5 pM).
机译:使用微粒作为捕获表面和荧光共振能量转移作为检测技术,我们已经证明了在固相上进行侵入性裂解反应的可行性。溶液相侵入切割测定法是许多基因组学应用的有效工具,是一种信号放大方法,能够区分仅存在一个碱基突变的核酸。该方法在靶核酸上定位两个重叠的寡核苷酸,即探针和上游寡核苷酸,以产生被结构特异性5'-核酸酶识别和切割的复合物。但是,对于微阵列和其他多重应用,该方法必须适用于固相平台。当将两个所需的重叠寡核苷酸中的任何一个配置为结合颗粒的试剂时,以及当两个寡核苷酸都连接到固相上时,探针寡核苷酸都会发生有效切割。通过长系链将探针寡核苷酸定位在远离粒子表面的位置,可以改善信号和反应速率。基于颗粒的侵入性裂解反应能够以低至100?amol /测定(0.5 pM)的目标浓度区分ApoE Cys158和Arg158等位基因。

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