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适体-分子印迹聚合物杂化受体用于前列腺特异性抗原的高灵敏电化学检测。

Aptamer-MIP hybrid receptor for highly sensitive electrochemical detection of prostate specific antigen.

机构信息

Department of Electronic & Electrical Engineering, University of Bath, Bath BA2 7AY, United Kingdom.

School of Pharmacy and Pharmaceutical Sciences, Cardiff University, Cardiff CF10 3NB, United Kingdom.

出版信息

Biosens Bioelectron. 2016 Jan 15;75:188-95. doi: 10.1016/j.bios.2015.08.043. Epub 2015 Aug 21.

DOI:10.1016/j.bios.2015.08.043
PMID:26318788
Abstract

This study reports the design and evaluation of a new synthetic receptor sensor based on the amalgamation of biomolecular recognition elements and molecular imprinting to overcome some of the challenges faced by conventional protein imprinting. A thiolated DNA aptamer with established affinity for prostate specific antigen (PSA) was complexed with PSA prior to being immobilised on the surface of a gold electrode. Controlled electropolymerisation of dopamine around the complex served to both entrap the complex, holding the aptamer in, or near to, it's binding conformation, and to localise the PSA binding sites at the sensor surface. Following removal of PSA, it was proposed that the molecularly imprinted polymer (MIP) cavity would act synergistically with the embedded aptamer to form a hybrid receptor (apta-MIP), displaying recognition properties superior to that of aptamer alone. Electrochemical impedance spectroscopy (EIS) was used to evaluate subsequent rebinding of PSA to the apta-MIP surface. The apta-MIP sensor showed high sensitivity with a linear response from 100pg/ml to 100ng/ml of PSA and a limit of detection of 1pg/ml, which was three-fold higher than aptamer alone sensor for PSA. Furthermore, the sensor demonstrated low cross-reactivity with a homologous protein (human Kallikrein 2) and low response to human serum albumin (HSA), suggesting possible resilience to the non-specific binding of serum proteins.

摘要

本研究报告了一种新的合成受体传感器的设计和评估,该传感器基于生物分子识别元件和分子印迹的融合,以克服传统蛋白质印迹所面临的一些挑战。与前列腺特异性抗原(PSA)具有既定亲和力的硫醇化 DNA 适体与 PSA 复合,然后固定在金电极表面上。多巴胺的受控电化学聚合围绕复合物进行,既可以捕获复合物,使适体保持在其结合构象中或附近,又可以将 PSA 结合位点定位在传感器表面上。去除 PSA 后,据推测,分子印迹聚合物(MIP)空腔将与嵌入的适体协同作用,形成混合受体(apta-MIP),显示出优于单独适体的识别特性。电化学阻抗谱(EIS)用于评估 PSA 随后与 apta-MIP 表面的再结合。apta-MIP 传感器具有高灵敏度,对 100pg/ml 至 100ng/ml PSA 的线性响应,检出限为 1pg/ml,比单独用于 PSA 的适体传感器高 3 倍。此外,该传感器对同源蛋白(人激肽释放酶 2)表现出低交叉反应性,对人血清白蛋白(HSA)的反应性低,表明对血清蛋白的非特异性结合具有一定的抵抗力。

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