利用 DNA 酶-HCR 级联扩增技术检测 CSFV 的策略。

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-10-15 DOI:10.1039/d4ay01209g
Xiuen Cao, Jiajing Cai, Zhilin He, Haofei Ji, Ruowei Sun, Xun Zhang, Chuanpin Chen, Qubo Zhu
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引用次数: 0

摘要

杂交链式反应(HCR)是一种等温扩增技术,广泛用于检测核酸和小分子。尽管效果显著,但传统线性 HCR 的动力学速度相对较慢,灵敏度也不够高。为解决这一难题,我们创新性地将 HCR 与 DNA 酶技术相结合,以提高核酸检测能力。在这种新方法中,目标分子的存在会触发 DNA 酶的形成,从而导致底物 S 的裂解、HCR 的启动以及 DNA 纳米线和标记 DNA 酶的产生。新生成的 DNA 酶不断裂解底物 S,促进 HCR 的连续扩增,并显著增强荧光信号。该系统提供了一种简单、灵敏、选择性强且用途广泛的核酸检测方法,检测限低至 5 pM。在对传统猪瘟病毒(CSFV)样本进行测试时,该系统显示出与 RT-qPCR 相当的检测准确性,并表现出卓越的重复性。
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A strategy for detecting CSFV using DNAzyme-HCR cascade amplification.

The Hybridization Chain Reaction (HCR) is an isothermal amplification technique widely used for sensing nucleic acids and small molecules. Despite its effectiveness, conventional linear HCR exhibits relatively slow kinetics and insufficient sensitivity. To address this challenge, we have innovatively combined HCR with DNAzyme technology to enhance nucleic acid detection. In this novel approach, the presence of a target molecule triggers the formation of DNAzyme, leading to the cleavage of substrate S, the initiation of HCR, and the production of DNA nanowires and labeled DNAzyme. The newly generated DNAzyme continuously cleaves substrate S, promoting sequential HCR amplification and significantly enhancing the fluorescence signal. This system offers a simple, sensitive, selective, and versatile method for nucleic acid detection, with a detection limit as low as 5 pM. When tested on classical swine fever virus (CSFV) samples, the system demonstrated detection accuracy comparable to RT-qPCR and exhibited superior repeatability.

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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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