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Electrochemical DNA sensor for detection of single nucleotide polymorphisms

机译:用于检测单核苷酸多态性的电化学DNA传感器

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摘要

In recent years there has been an increased interest in using biosensors for the recognition and monitoring of molecule interactions. DNA sensors and gene chips areparticularly relevant for directly applying the information gathered from the genome projects. In this work electrochemical techniques are used to develop methodologies to detect DNA polymorphisms in human genes using cytochrome P450 3A4 (CYP3A4) as a model gene. CYP3A4*1B oligonucleotides were immobilized on the surface of a gold electrode and hybridized with fully complementary oligonucleotide sequencesas well as with mismatched sequences corresponding to the CYP3A4*1A reference sequence. The methodology developed is based on double-stranded DNA’s ability to transport charge along nucleotide stacking. The perturbation of the double helix pi-stack introduced by a mismatched nucleotide reduces electron flow and can be detected by measuring the attenuation of the chargetransfer. The methodology developed could identify CYP3A4*1A homozygotes by the 5 μC charge attenuation observed when compared with DNA samples containing at least one CYP3A4*1B allele.
机译:近年来,人们越来越关注使用生物传感器来识别和监视分子相互作用。 DNA传感器和基因芯片与直接应用从基因组计划中收集的信息特别相关。在这项工作中,电化学技术被用于开发使用细胞色素P450 3A4(CYP3A4)作为模型基因来检测人类基因中DNA多态性的方法。将CYP3A4 * 1B寡核苷酸固定在金电极的表面上,并与完全互补的寡核苷酸序列以及与CYP3A4 * 1A参考序列相对应的错配序列杂交。所开发的方法是基于双链DNA沿着核苷酸堆积转运电荷的能力。由错配的核苷酸引入的双螺旋pi堆栈的扰动会降低电子流,并且可以通过测量电荷转移的衰减来检测。与包含至少一个CYP3A4 * 1B等位基因的DNA样品相比,通过观察到的5μC电荷衰减,开发的方法可以识别CYP3A4 * 1A纯合子。

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