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Electrochemical detection of DNA hybridization using biometallization

机译:使用生物金属化技术对DNA杂交进行电化学检测

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We demonstrate the amplified detection of a target DNA based on the enzymatic deposition of silver. In this method, the target DNA and a biotinylated detection DNA probe hybridize to a capture DNA probe tethered onto a gold electrode. Neutravidin-conjugated alkaline phosphatase binds to the biotin of the detection probe on the electrode surface and converts the nonelectroactive substrate of the enzyme, p-aminophenyl phosphate, into the reducing agent, p-aminophenol. The latter, in turn, reduces metal ions in solutions leading to deposition of the metal onto the electrode surface and DNA backbone. Ibis process, which we term biometallization, leads to a great enhancement in signal due to the accumulation of metallic silver by a catalytically generated enzyme product and, thus, the electrochemical amplification of a biochemically amplified signal. The anodic stripping current of enzymatically deposited silver provides a measure of the extent of hybridization of the target oligomers. This biometallization process is highly sensitive, detecting as little as 100 aM (10 zmol) of DNA. We also successfully applied this method to the sequence-selective discrimination between perfectly matched and mismatched target oligonucleotides including a single-base mismatched target.
机译:我们展示了基于银的酶促沉积对靶DNA的扩增检测。在这种方法中,目标DNA和生物素化的检测DNA探针与拴在金电极上的捕获DNA探针杂交。中性抗生物素蛋白缀合的碱性磷酸酶与电极表面上检测探针的生物素结合,并将酶的非电活性底物对氨基苯磷酸转化为还原剂对氨基苯酚。后者继而还原溶液中的金属离子,导致金属沉积在电极表面和DNA主链上。宜必思过程(我们称为生物金属化)由于信号产生的酶产物积聚金属银而导致信号的极大增强,因此,生物化学放大信号的电化学放大。酶沉积的银的阳极剥离电流提供了靶低聚物的杂交程度的量度。这种生物金属化过程非常敏感,可检测到100 aM(10 zmol)的DNA。我们还成功地将此方法应用于完全匹配和不匹配的目标寡核苷酸(包括单碱基不匹配的目标)之间的序列选择性判别。

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