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链置换诱导的酶免扩增用于核酸和蛋白质的无标记和无分离超灵敏原子荧光光谱检测

Strand Displacement-Induced Enzyme-Free Amplification for Label-Free and Separation-Free Ultrasensitive Atomic Fluorescence Spectrometric Detection of Nucleic Acids and Proteins.

机构信息

College of Chemistry, and ‡Analytical & Testing Center, Sichuan University , 29 Wangjiang Road, Chengdu, Sichuan 610064, China.

出版信息

Anal Chem. 2016 Dec 20;88(24):12386-12392. doi: 10.1021/acs.analchem.6b03633. Epub 2016 Nov 30.

DOI:10.1021/acs.analchem.6b03633
PMID:28193041
Abstract

In previous work, we have developed a simple strategy for a label-free and separation-free bioassay for target DNA and protein, with the limit of detection at the nM level only. Herein, taking advantage of atomic fluorescence spectrometric detection of metal ions and amplification of DNA, a label-free and separation-free ultrasensitive homogeneous DNA analytical platform for target DNA and protein detection was developed on the basis of an enzyme-free strand displacement signal amplification strategy for dramatically improved detectability. Using the T-Hg-T hairpin structure as the probe, the target DNA binds with HP (T-Hg-T hairpin structure) and released the Hg first; then, the P4 (help DNA) hybridizes with target-P3 complex and free the target DNA, which is used to trigger another reaction cycle. The cycling use of the target amplifies the mercury atomic fluorescence intensity for ultrasensitive DNA detection. Moreover, the enzyme-free strand displacement signal amplification analytical system was further extended for protein detection by introducing an aptamer-P2 arched structure with thrombin as a model analyte. The current homogeneous strategy provides an ultrasensitive AFS detection of DNA and thrombin down to the 0.3 aM and 0.1 aM level, respectively, with a high selectivity. This strategy could be a promising unique alternative for nucleic acid and protein assay.

摘要

在之前的工作中,我们开发了一种简单的无标记和无分离的靶 DNA 和蛋白质生物分析策略,检测限可达纳摩尔水平。在此基础上,利用金属离子原子荧光光谱检测和 DNA 扩增,我们基于无酶链置换信号放大策略,开发了一种无标记和无分离的超灵敏均相 DNA 分析平台,用于靶 DNA 和蛋白质检测,大大提高了检测的灵敏度。我们使用 T-Hg-T 发夹结构作为探针,靶 DNA 与 HP(T-Hg-T 发夹结构)结合并首先释放汞;然后,P4(辅助 DNA)与靶-P3 复合物杂交并释放靶 DNA,这用于触发另一个反应循环。靶标 DNA 的循环使用放大了汞原子荧光强度,从而实现了超灵敏的 DNA 检测。此外,通过引入带有凝血酶作为模型分析物的适体-P2 弓形结构,我们进一步扩展了无酶链置换信号放大分析系统,用于蛋白质检测。目前的均相策略为 DNA 和凝血酶的 AFS 检测提供了超灵敏的检测下限,分别达到 0.3 aM 和 0.1 aM 水平,具有高选择性。这种策略可能是核酸和蛋白质分析的一种有前途的独特替代方法。

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