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首页> 外文期刊>Journal of Electroanalytical Chemistry: An International Journal Devoted to All Aspects of Electrode Kinetics, Interfacial Structure, Properties of Electrolytes, Colloid and Biological Electrochemistry >Electrogenerated chemiluminescence biosensing method for highly sensitive detection of DNA hydroxymethylation: Combining glycosylation with Ru (phen)(3)(2+)-assembled graphene oxide
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Electrogenerated chemiluminescence biosensing method for highly sensitive detection of DNA hydroxymethylation: Combining glycosylation with Ru (phen)(3)(2+)-assembled graphene oxide

机译:用于高敏感性检测DNA羟甲基的电化学化学发光的生物传感方法:将糖基化与Ru(Phen)(3)(2 +)组装的石墨烯组合

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摘要

We developed a novel electrogenerated chemiluminescence (ECL) biosensing method for quantitative detection of DNA hydroxymethylation (5-hydroxymethylcytosine, 5-hmC) using T4 beta-glucosyltransferase (beta-GT) and graphene oxide (GO) for enzymatic and chemical modification of the 5-hmC. beta-GT selectively glucosylated the hydroxymethyl group of 5-lnC to improve selectivity, whereas GO, which loads substantial amounts of the ECL reagent, was used as the signal amplification element to enhance assay sensitivity. The ECL bioassay involved the capture of DNA containing 5-hmC, which was chemically modified with a glucose moiety, through hybridization with complimentary 5'-thiol-modified DNA on a glassy carbon electrode (GCE) under the catalysis of beta-GT. The dichlorotris (1,10-phenanthroline) ruthenium -assembled GO (Ru(phen)(3)(2+)/GO) composite was coupled to the electrode surface via a bridging agent, and provided excellent ECL signal. The bridging agent used was 3-aminophenylboronic acid (APBA), boronic acid and its derivatives can interact with 1,2-or 1,3-diols (such as glucose) to generate 5-or 6 -membered cyclic boronate esters. The obtained ECL intensity was positively correlated with the concentration of DNA containing 5-hmC, the linear range was from 0.01 pM to 1.00 nM, with a low limit of detection of 3.84 fM. Our results demonstrate that use of enzymatic and chemical modification in combination with highly sensitive ECL is a facile and promising approach for DNA hydroxymethylation analysis.
机译:我们开发了一种新的电化学化学发光(ECL)生物传感方法,用于使用T4β-葡糖基转移酶(Beta-GT)和石墨烯(GO)来定量检测DNA羟甲基(5-羟甲基胞嘧啶,5-HMC),并为5的酶和化学改性进行酶促-hmc。 β-GT选择性地葡萄糖苷化5-LNC的羟甲基以改善选择性,而转载大量的EC1试剂的转移为信号放大元件以增强测定敏感性。 ECL生物测定涉及含有5-HMC的DNA的捕获,通过在β-GT的催化下与玻璃状碳电极(GCE)的互补5'-硫醇改性DNA杂交来化学改性。二氯(1,10-菲咯啉)钌 - 致密的去(Ru(phO)(3)(2 +)/去)复合物通过桥接剂偶联到电极表面,并提供优异的ECL信号。所用的桥接剂是3-氨基苯基硼酸(APBA),硼酸及其衍生物可以与1,2-或1,3-二醇(例如葡萄糖)相互作用以产生5-或60-0℃的环状硼酸酯。所获得的ECL强度与含有5-HMC的DNA的浓度呈正相关,线性范围为0.01pm至1.00nm,检测限为3.84 fm。我们的结果表明,使用酶和化学改性与高度敏感的ECL结合的使用是DNA羟甲基甲基化分析的容易和有希望的方法。

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