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用于高灵敏度检测生物制剂多重PCR产物的电微阵列。

Electrical microarrays for highly sensitive detection of multiplex PCR products from biological agents.

作者信息

Elsholz Bruno, Nitsche Andreas, Achenbach John, Ellerbrok Heinz, Blohm Lars, Albers Jörg, Pauli Georg, Hintsche Rainer, Wörl Ralf

机构信息

Fraunhofer Institute for Silicon Technology, Biotechnical Microsystems, Itzehoe, Germany.

出版信息

Biosens Bioelectron. 2009 Feb 15;24(6):1737-43. doi: 10.1016/j.bios.2008.09.003. Epub 2008 Sep 12.

Abstract

For the sensitive detection of amplicons derived from diagnostic PCR, a novel electrical low-density microarray is applied and compared to state-of-the-art quantitative real-time PCR. The principle of the electrochemical method and the effective use for analysis are described. Interdigitated array gold electrodes (IDA-E) embedded into a silicon chip are the core technology of the fully automated compact biosensor system, basing on enzyme coupled electrochemical detection. The biointerface is built up with thiol-modified capture oligonucleotides on gold and mediates the specific recognition of hybridised target DNA amplified with uniplex or multiplex PCR. In here we show the potential of the designed electrical microarray to function as an advanced screening method for the parallel detection of a panel of the four pathogens Bacillus anthracis, Yersinia pestis, Francisella tularensis and ortho pox viruses (genus), which are among the most relevant biowarfare agents. PCR products, generated from 10 to 50 gene equivalents, have been detected reproducibly. The experiments with varying pathogen amounts showed the good reliability and the high sensitivity of the method, equivalent to optical real-time PCR detection systems. Without PCR the total assay time amounts to 27 min. The advantage of the combination of multiplex-PCR with electrical microarray detection avoiding intensive PCR probe labelling strategies is illustrated.

摘要

为了灵敏检测诊断性聚合酶链反应(PCR)产生的扩增子,应用了一种新型的低密度电微阵列,并与最先进的定量实时PCR进行比较。描述了电化学方法的原理及其在分析中的有效应用。嵌入硅芯片的叉指阵列金电极(IDA-E)是基于酶联电化学检测的全自动紧凑型生物传感器系统的核心技术。生物界面通过金表面的硫醇修饰捕获寡核苷酸构建,介导对单重或多重PCR扩增的杂交靶DNA的特异性识别。在此,我们展示了所设计的电微阵列作为一种先进筛选方法用于平行检测炭疽芽孢杆菌、鼠疫耶尔森菌、土拉弗朗西斯菌和正痘病毒(属)这四种病原体的潜力,这些病原体是最相关的生物战剂。从10到50个基因当量产生的PCR产物已被重复检测。不同病原体数量的实验表明该方法具有良好的可靠性和高灵敏度,与光学实时PCR检测系统相当。不进行PCR时,总检测时间为27分钟。说明了多重PCR与电微阵列检测相结合的优势,避免了繁琐的PCR探针标记策略。

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