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Integrated Tyramide and Polymerization-Assisted Signal Amplification for a Highly-Sensitive Immunoassay

机译:集成的乙酰胺和聚合辅助信号放大技术,可实现高度灵敏的免疫分析

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摘要

A novel strategy for ultrasensitive detection of model protein based on the integration of tyramide signal amplification (TSA) and polymerization-assisted signal amplification was proposed. The surface-initiated atom transfer radical polymerization (SI-ATRP) of glycidyl methacrylate (GMA) was triggered by the initiator-coupled protein immobilized on the electrode surface through sandwiched immunoreactions. Growth of long chain polymeric materials provided numerous epoxy groups for subsequent coupling of horseradish peroxidase (HRP), which in turn significantly increased the loading of quantum dots (QDs) labeled tyramide in the presence of hydrogen peroxide. As a result, electrochemiluminescence (ECL) and square-wave voltammetric (SWV) measurements showed 9.4- and 10.5-fold increase in detection signal in comparison with the unamplified method, respectively. To demonstrate the feasibility of this approach, human immunoglobulin G antigen (IgG) as a model target protein was employed and the detection limits were 0.73 and 0.09 pg mL~(-1) for ECL and SWV, respectively. The results showed that sensitivity of the presented immunoassay significantly increased by one-order of magnitude and offered great application promises in providing a sensitive, specific, and potent method for biological detection.
机译:提出了一种基于酪胺信号放大(TSA)和聚合辅助信号放大的超灵敏检测模型蛋白的新策略。甲基丙烯酸缩水甘油酯(GMA)的表面引发的原子转移自由基聚合(SI-ATRP)是通过夹心的免疫反应固定在电极表面的引发剂偶联蛋白触发的。长链聚合物材料的生长为辣根过氧化物酶(HRP)的后续偶联提供了许多环氧基,进而在过氧化氢的存在下显着增加了标记为酪酰胺的量子点(QD)的负载。结果,与未放大的方法相比,电化学发光(ECL)和方波伏安(SWV)测量分别显示检测信号增加9.4倍和10.5倍。为了证明这种方法的可行性,采用了人类免疫球蛋白G抗原(IgG)作为模型目标蛋白,ECL和SWV的检出限分别为0.73和0.09 pg mL〜(-1)。结果表明,所提出的免疫测定的灵敏度显着提高了一个数量级,并为提供灵敏,特异性和有效的生物检测方法提供了广阔的应用前景。

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