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基于亚微米间隙叉指电极和金增强的电化学生物传感器。

Electrical immunosensor based on a submicron-gap interdigitated electrode and gold enhancement.

机构信息

BioMonitoring Research Center, KRIBB, Daejeon 305-806, Republic of Korea.

出版信息

Biosens Bioelectron. 2011 Aug 15;26(12):4690-6. doi: 10.1016/j.bios.2011.05.027. Epub 2011 May 19.

DOI:10.1016/j.bios.2011.05.027
PMID:21684145
Abstract

We demonstrated that the detection of human interleukin 5 (IL5) with a higher sensitivity than the enzyme-linked immunosorbent assay (ELISA) was possible using mass-producible submicron-gap interdigitated electrodes (IDEs) combined with signal amplification by a gold nanoparticle (AuNP) and gold enhancement. IDEs, facing comb-shape electrodes, can act as simple and miniaturized devices for immunoassay. An IDE with a gap size of 400nm was fabricated by a stepper photolithography process and was applied for the immunoassay of human IL5. A biotinylated anti-human IL5 was immobilized on the streptavidin-modified IDE, and biotin-bovine serum albumin (BSA) and BSA were added sequentially to reduce non-specific binding between the streptavidin-immobilized IDE surface and other proteins. The immunoassay procedure included three main steps: the reaction of human IL5 to form antigen-antibody complexes, the binding of AuNP conjugation with an antibody against human IL5 for the sandwich immunoassay, and gold enhancement for electrical signal amplification. The measurement of electrical current at each step showed that the gold enhancement step was very critical in detection of the concentration of human IL5. Analysis by scanning electron microscope (SEM) showed that close to 1μm particles were formed from 10nm AuNP by the gold enhancement reaction using gold ions and hydroxylamine. Under optimized conditions, human IL5 could be analyzed at 1pgmL(-1) with a wide dynamic range (from 10(-3) to 100ngmL(-1) concentrations).

摘要

我们证明,使用大规模生产的亚微米间隙叉指电极(IDEs)结合金纳米粒子(AuNP)和金增强的信号放大,可以比酶联免疫吸附测定(ELISA)更灵敏地检测人白细胞介素 5(IL5)。面对梳状电极的 IDE 可以作为简单和小型化的免疫分析设备。通过步进光刻工艺制造了间隙尺寸为 400nm 的 IDE,并将其应用于人 IL5 的免疫分析。将生物素化的抗人 IL5 固定在链霉亲和素修饰的 IDE 上,并依次添加生物素-牛血清白蛋白(BSA)和 BSA,以减少链霉亲和素固定的 IDE 表面与其他蛋白质之间的非特异性结合。免疫分析过程包括三个主要步骤:人 IL5 的反应形成抗原-抗体复合物,AuNP 与抗人 IL5 的抗体结合进行夹心免疫分析,以及金增强进行电信号放大。每个步骤的电流测量表明,金增强步骤在检测人 IL5 浓度方面非常关键。扫描电子显微镜(SEM)分析表明,通过使用金离子和羟胺的金增强反应,10nm AuNP 形成了接近 1μm 的颗粒。在优化条件下,人 IL5 可以在 1pgmL(-1)的浓度下进行分析,具有较宽的动态范围(从 10(-3)到 100ngmL(-1)浓度)。

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