应用场效应晶体管集成微流控系统检测c反应蛋白的双适体分析

W. Kao, C. Chu, Wen-Hsin Chang, Yu-Lin Wang, Gwo-Bin Lee
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引用次数: 3

摘要

c反应蛋白(C-reactive protein, CRP)是一种众所周知的评价心血管疾病风险的生物标志物,其快速准确的诊断对于监测心血管疾病至关重要。本研究提出了用场效应晶体管(FET)检测CRP的双适体试验。这是第一次使用两个特定于CRP的适体来形成一个三明治实验,这样就可以通过FET设备检测CRP浓度。此外,微流控系统被用于自动化双适体三明治分析,使整个诊断过程可以自动化。除了来自FET装置的电信号外,荧光信号也被用来证实这一测定。实验结果表明,第一适体(1st aptamer)和第二适体(c aptamer)可以与靶CRP特异性结合。此外,如果将结合的CRP和第二适体洗脱,则集成了FET的微流控芯片可以重复使用。此外,为了防止干扰物质如蛋白质、细胞和任何非特异性分子在固定第1个适体后仍粘附在FET器件的栅极区上,我们使用乙醇胺作为阻断剂来防止非特异性粘附。实验结果证实,使用乙醇胺阻断可以成功地阻止非特异性结合。
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Dual-aptamer assay for C-reactive protein detection by using field-effect transistors on an integrated microfluidic system
Rapid and accurate diagnosis of C-reactive protein (CRP) is crucial for monitoring cardiovascular diseases because it is a well-known biomarker for evaluating risks of cardiovascular diseases. This study presents a dual-aptamer assay for detection of CRP by using field-effect transistors (FET). This is the first time that two aptamers, which are specific to CRP, were used to form a sandwich assay such that the CRP concentration could be detected by FET devices. Furthermore, a microfluidic system was used to automate the dual-aptamer sandwich assay such that the entire diagnosis process could be automated. In addition to electric signals from the FET device, fluorescent signals were also used to confirm this assay. Experimental results revealed that the first aptamer (1st aptamer) and the second aptamer (c aptamer) could be specifically binded with target CRP. Furthermore, the microfluidic chip integrated with FET can be re-used if the binded CRP and 2nd aptamer was eluted. Besides, in order to prevent the interference materials like proteins, cells and any nonspecific molecules from adhering onto the gate region of the FET device even after immobilization of 1st aptamer, we used ethanolamine as the blocking agent to prevent nonspecific adhesion. The experimental results confirmed that blocking using ethanolamine could successfully prevent nonspecific binding.
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