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Detection of PCR amplification with Electrochemical DNA Biosensor

机译:电化学DNA生物传感器检测PCR扩增

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A novel assay for the Cyclic Voltammetry (CV) detection of PCR amplification to using Electrochemical DNA Biosensor was reported. The coupling of DNA electrochemical sensors have specialities of quick detection and cheapness and have the potential of the quantitative evaluation of the PCR amplification. The electrochemical sensor was obtained by immobilizing single-stranded oligonucleotides onto gold electrodes through mercaptan of the DNA bases using Nhydroxysulfosuccinimide (NHS) and N-(3-dimethylamion)propylN'-ethyl carbodiimidehydrochloride (EDC) as activation. The hybridization reaction that occurred on the electrode surface was evidenced by Cyclic Voltammetry (CV) analysis-using as [Co(phen)3](ClO4)3 indicator. The covalently immobilized singlestranded DNA could selectively hybridize with its complementary DNA in solution to form double-stranded DNA on the gold surface. A significant increase of the peak current of Cyclic Voltammetry (CV)) upon the hybridization of immobilized ssDNA with PCR amplification products in the solution was observed. This peak current change was used to monitor the amount of PCR amplification products. Factors such as DNA target concentration and hybridization conditions determining the sensitivity of the electrochemical assay were investigated.
机译:报道了一种使用电化学DNA生物传感器进行PCR扩增的循环伏安法(CV)检测的新方法。 DNA电化学传感器的耦合具有快速检测和廉价的特点,并具有定量评估PCR扩增潜力的潜力。电化学传感器是通过使用N羟基磺基琥珀酰亚胺(NHS)和N-(3-二甲基氨基)丙基N'-乙基碳二亚胺盐酸盐(EDC)作为活化剂通过DNA碱基的硫醇将单链寡核苷酸固定在金电极上而获得的。电极表面发生的杂交反应通过循环伏安法(CV)分析证明,用作[Co(phen)3](ClO4)3指示剂。共价固定的单链DNA可以在溶液中与其互补DNA选择性杂交,在金表面形成双链DNA。观察到溶液中固定的ssDNA与PCR扩增产物杂交后,循环伏安法(CV)的峰值电流显着增加。该峰值电流变化用于监测PCR扩增产物的量。研究了诸如DNA靶标浓度和杂交条件等因素,这些因素决定了电化学测定的灵敏度。

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