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基于纳米电极组合的用于乳糜泻诊断的灵敏电化学发光免疫传感器。

A Sensitive Electrochemiluminescence Immunosensor for Celiac Disease Diagnosis Based on Nanoelectrode Ensembles.

机构信息

Department of Molecular Sciences and Nanosystems, University Ca'Foscari of Venice , via Torino 155, 30172 Venezia Mestre, Italy.

Institut des Sciences Moléculaires, CNRS UMR 5255, University of Bordeaux, ENSCBP , 33607 Pessac, France.

出版信息

Anal Chem. 2015 Dec 15;87(24):12080-7. doi: 10.1021/acs.analchem.5b02801. Epub 2015 Nov 24.

Abstract

We report here the design of a novel immunosensor and its application for celiac disease diagnosis, based on an electrogenerated chemiluminescence (ECL) readout, using membrane-templated gold nanoelectrode ensembles (NEEs) as a detection platform. An original sensing strategy is presented by segregating spatially the initial electrochemical reaction and the location of the immobilized biomolecules where ECL is finally emitted. The recognition scaffold is the following: tissue transglutaminase (tTG) is immobilized as a capturing agent on the polycarbonate (PC) surface of the track-etched templating membrane. It captures the target tissue transglutaminase antibody (anti-tTG), and finally allows the immobilization of a streptavidin-modified ruthenium-based ECL label via reaction with a suitable biotinylated secondary antibody. The application of an oxidizing potential in a tri-n-propylamine (TPrA) solution generates an intense and sharp ECL signal, suitable for analytical purposes. Voltammetric and ECL analyses evidenced that the ruthenium complex is not oxidized directly at the surface of the nanoelectrodes; instead ECL is generated following the TPrA oxidation, which produces the TPrA•+ and TPrA• radicals. With NEEs operating under total overlap diffusion conditions, high local fluxes of these reactive radicals are produced by the nanoelectrodes in the immediate vicinity of the ECL labels, so that they efficiently generate the ECL signal. The radicals can diffuse over short distances and react with the Ru(bpy)32+ label. In addition, the ECL emission is obtained by applying a potential of 0.88 V versus Ag/AgCl, which is about 0.3 V lower than when ECL is initiated by the electrochemical oxidation of Ru(bpy)3(2+). The immunosensor provides ECL signals which scale with anti-tTG concentration with a linearity range between 1.5 ng·mL–1 and 10 μg·mL–1 and a detection limit of 0.5 ng·mL–1. The sensor is finally applied to the analysis of anti-tTG in human serum samples, showing to be suitable to discriminate between healthy and celiac patients.

摘要

我们在此报告了一种基于电致化学发光(ECL)读出的新型免疫传感器的设计及其在乳糜泻诊断中的应用,该传感器使用膜模板金纳米电极组件(NEE)作为检测平台。我们提出了一种原始的传感策略,通过将初始电化学反应和固定化生物分子的位置分隔开来,在空间上分隔开来,最终在该位置发出 ECL。识别支架如下:组织转谷氨酰胺酶(tTG)作为捕获剂固定在聚碳酸酯(PC)的轨迹蚀刻模板膜的表面上。它捕获靶组织转谷氨酰胺酶抗体(抗-tTG),最后通过与合适的生物素化二级抗体反应允许固定链霉亲和素修饰的基于钌的 ECL 标记。在三丙胺(TPrA)溶液中施加氧化电势会产生强烈而尖锐的 ECL 信号,适用于分析目的。伏安法和 ECL 分析表明,钌络合物不能在纳米电极的表面上直接氧化;相反,在 TPrA 氧化后生成 ECL,生成 TPrA•+和 TPrA•自由基。在 NEE 下操作时,在 ECL 标记附近的纳米电极附近会产生高局部通量的这些反应性自由基,从而有效地产生 ECL 信号。自由基可以短距离扩散并与 Ru(bpy)32+标记物反应。此外,通过施加相对于 Ag/AgCl 为 0.88 V 的电势获得 ECL 发射,这比通过电化学氧化 Ru(bpy)3(2+)引发 ECL 时低约 0.3 V。免疫传感器提供与抗-tTG 浓度成比例的 ECL 信号,线性范围为 1.5 ng·mL-1至 10 μg·mL-1,检测限为 0.5 ng·mL-1。该传感器最终应用于人血清样品中抗-tTG 的分析,表明它适用于区分健康人和乳糜泻患者。

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