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基于双链特异性核酸酶和杂交链式反应的双重扩增机制的用于灵敏检测 microRNA 的比率型电化学分析。

Ratiometric electrochemical assay for sensitive detecting microRNA based on dual-amplification mechanism of duplex-specific nuclease and hybridization chain reaction.

机构信息

College of Chemistry and Institute for Advanced Study, Nanchang University, Nanchang 330031, China.

College of Chemistry and Institute for Advanced Study, Nanchang University, Nanchang 330031, China.

出版信息

Biosens Bioelectron. 2018 Apr 15;102:211-216. doi: 10.1016/j.bios.2017.11.030. Epub 2017 Nov 8.

DOI:10.1016/j.bios.2017.11.030
PMID:29145074
Abstract

We propose a ratiometric electrochemical assay for detecting microRNA (miRNA) on the basis of dual-amplification mechanism by using distinguishable electrochemical signals from thionine (Thi) and ferrocene (Fc). The thiol-modified and ferrocene-labeled hairpin capture probes (CP) are first immobilized on an Au electrode via Au-S reaction. The target miRNA hybridizes with CP and unfolding the hairpin structure of CP to form miRNA-DNA duplexes. Then, kamchatka crab duplex specific nuclease (DSN) specifically cleaves the DNA in miRNA-DNA duplexes, leading to the release of miRNA and another cleaves cycle, meanwhile, numerous Fc leaves away from the electrode surface and leads to the signal-off of Fc. The residual fragment on electrode surface acts as a HCR primer to form dsDNA polymers through in situ HCR with the presence of the primer and two probes (HDNA and HDNA'), resulting in the capture of numerous DNA/Au NPs/Thi and the signal-on of Thi. The dual-amplification mechanism significantly amplifies the decrease of Fc signal and the increase of Thi signal for ratiometric readout (I/I), thus providing a sensitive method for the selective detection of miR-141 with a detection limit down to 11aM. The dual-signal ratiometric outputs have an intrinsic self-calibration to the effects from system, which is promising to be applied in biosensing and clinical diagnosis.

摘要

我们提出了一种基于双扩增机制的比率型电化学测定法来检测 microRNA(miRNA),该方法利用了来自硫堇(Thi)和二茂铁(Fc)的可区分电化学信号。巯基修饰和二茂铁标记的发夹捕获探针(CP)首先通过 Au-S 反应固定在 Au 电极上。靶 miRNA 与 CP 杂交并展开 CP 的发夹结构,形成 miRNA-DNA 双链体。然后,堪察加蟹双链体特异性核酸酶(DSN)特异性切割 miRNA-DNA 双链体中的 DNA,导致 miRNA 的释放和另一个切割循环,同时,大量的 Fc 离开电极表面,导致 Fc 的信号关闭。电极表面上的残留片段作为 HCR 引物,通过在引物和两个探针(HDNA 和 HDNA')存在下进行原位 HCR,形成 dsDNA 聚合物,导致大量的 DNA/Au NPs/Thi 的捕获和 Thi 信号的开启。双扩增机制显著放大了 Fc 信号的减少和 Thi 信号的增加,用于比率读取(I/I),从而提供了一种用于选择性检测 miR-141 的灵敏方法,检测限低至 11aM。双信号比率输出对系统的影响具有内在的自我校准,有望应用于生物传感和临床诊断。

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