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基于酶催化靶标循环的尿液病原体电化学高灵敏检测的双重信号放大。

Dual signal amplification for highly sensitive electrochemical detection of uropathogens via enzyme-based catalytic target recycling.

机构信息

Key Laboratory on Luminescence and Real-Time Analysis, Ministry of Education, School of Chemistry and Chemical Engineering, Southwest University, Chongqing 400715, PR China.

出版信息

Biosens Bioelectron. 2011 Nov 15;29(1):184-8. doi: 10.1016/j.bios.2011.08.015. Epub 2011 Aug 19.

Abstract

We report an ultrasensitive electrochemical approach for the detection of uropathogen sequence-specific DNA target. The sensing strategy involves a dual signal amplification process, which combines the signal enhancement by the enzymatic target recycling technique with the sensitivity improvement by the quantum dot (QD) layer-by-layer (LBL) assembled labels. The enzyme-based catalytic target DNA recycling process results in the use of each target DNA sequence for multiple times and leads to direct amplification of the analytical signal. Moreover, the LBL assembled QD labels can further enhance the sensitivity of the sensing system. The coupling of these two effective signal amplification strategies thus leads to low femtomolar (5fM) detection of the target DNA sequences. The proposed strategy also shows excellent discrimination between the target DNA and the single-base mismatch sequences. The advantageous intrinsic sequence-independent property of exonuclease III over other sequence-dependent enzymes makes our new dual signal amplification system a general sensing platform for monitoring ultralow level of various types of target DNA sequences.

摘要

我们报告了一种超灵敏的电化学方法,用于检测尿路病原体序列特异性 DNA 靶标。该传感策略涉及一种双重信号放大过程,它将酶促靶标循环技术的信号增强与量子点(QD)层层组装标签的灵敏度提高相结合。基于酶的催化靶标 DNA 循环过程导致每个靶标 DNA 序列被多次使用,并导致分析信号的直接放大。此外,LBL 组装的 QD 标签还可以进一步提高传感系统的灵敏度。这两种有效的信号放大策略的结合导致了对靶 DNA 序列的低飞摩尔(5fM)检测。该策略还显示了靶 DNA 与单碱基错配序列之间的出色区分。外切酶 III 的有利的固有序列非依赖性特性优于其他序列依赖性酶,使得我们的新双重信号放大系统成为监测各种类型的超低水平靶 DNA 序列的通用传感平台。

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