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用双酶功能化纳米二氧化硅微球进行肝癌患者血清中甲胎蛋白的电导免疫分析。

Conductometric immunoassay of alpha-fetoprotein in sera of liver cancer patients using bienzyme-functionalized nanometer-sized silica beads.

机构信息

Institute of Biomedical Analytical Technology and Instrumentation, Key Laboratory of Biomedical Information Engineering of Ministry of Education, School of Life Science and Technology, Xi'an Jiaotong University, Xi'an 710049, Shaanxi, China.

出版信息

Analyst. 2018 Dec 17;144(1):265-273. doi: 10.1039/c8an01791c.

Abstract

A conductometric immunoassay protocol was designed for the sensitive detection of a liver cancer biomarker, alpha-fetoprotein (AFP), in biological fluids by using enzyme-conjugated nanometer-sized enzyme-doped silica beads. Initially, urease molecules were doped into nanosilica particles by using the reverse micelle method. Thereafter, arginase-labeled anti-AFP antibodies were covalently conjugated onto the surface of the synthesized nanoparticles. The immunoreaction was carried out in a monoclonal anti-AFP capture antibody-coated microplate with a sandwich-type assay format by using bienzyme-functionalized silica nanobeads as the recognition elements. Upon l-arginine introduction, the substrate was cleaved into urea and l-ornithine on the basis of the arginase enzymatic reaction, and the as-produced urea was then decomposed into ammonia (NH4+) and bicarbonate (HCO3-) ions by the doped urease, thus causing the variation in the local conductivity of the detection solution on an interdigitated conductometric transducer. Under optimal conditions, the developed immunosensing system exhibited good conductometric responses toward target AFP within a dynamic linear range of 0.01-100 ng mL-1 at a relatively low detection limit of 4.8 pg mL-1 based on the 3sB criterion. Importantly, good reproducibility, high specificity and acceptable method accuracy were acquired for the analysis of human serum specimens in liver cancer patients.

摘要

设计了一种基于电导的免疫分析方法,用于在生物流体中灵敏检测肝癌生物标志物甲胎蛋白(AFP),该方法使用酶标记的纳米尺寸酶掺杂硅纳米球作为识别元件。首先,采用反胶束法将脲酶分子掺杂到纳米硅颗粒中。然后,将标记有精氨酸酶的抗 AFP 抗体通过共价键连接到合成的纳米粒子表面。免疫反应在包被有单克隆抗 AFP 捕获抗体的微孔板中进行,采用双酶功能化硅纳米珠作为识别元件,建立三明治型检测模式。在引入 l-精氨酸后,根据精氨酸酶的酶反应将底物切割成尿素和 l-鸟氨酸,产生的尿素随后被掺杂的脲酶分解成氨(NH4+)和碳酸氢盐(HCO3-)离子,从而导致检测溶液在叉指式电导传感器上的局部电导率发生变化。在最佳条件下,所开发的免疫传感系统在 0.01-100ngmL-1 的动态线性范围内对 AFP 表现出良好的电导响应,检测限低至 4.8pgmL-1(基于 3sB 准则)。重要的是,该方法用于分析肝癌患者的人血清标本时,具有良好的重现性、高特异性和可接受的方法准确性。

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