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一种结合 CRISPR/Cas12a 和链置换扩增以及多重信号读取的通用核酸检测平台。

A universal nucleic acid detection platform combing CRISPR/Cas12a and strand displacement amplification with multiple signal readout.

机构信息

College of Basic Medicine and Forensic Medicine, Henan University of Science and Technology, Luoyang, 471023, China.

College of Basic Medicine and Forensic Medicine, Henan University of Science and Technology, Luoyang, 471023, China.

出版信息

Talanta. 2024 Jun 1;273:125922. doi: 10.1016/j.talanta.2024.125922. Epub 2024 Mar 18.

DOI:10.1016/j.talanta.2024.125922
PMID:38503121
Abstract

Rapid and sensitive detection of nucleic acids has become crucial in various fields. However, most current nucleic acid detection methods can only be used in specific scenarios, such as RT-qPCR, which relies on fluorometer for signal readout, limiting its application at home or in the field due to its high price. In this paper, a universal nucleic acid detection platform combing CRISPR/Cas12a and strand displacement amplification (CRISPR-SDA) with multiple signal readout was established to adapt to different application scenarios. Nucleocapsid protein gene of SARS-CoV-2 (N gene) and hepatitis B virus (HBV) DNA were selected as model targets. The proposed strategy achieved the sensitivity of 53.1 fM, 0.15 pM, and 1 pM for N gene in fluorescence mode, personal glucose meter (PGM) mode and lateral flow assay (LFA) mode, respectively. It possessed the ability to differentiate single-base mismatch and the presence of salmon sperm DNA with a mass up to 10-fold of the targets did not significantly interfere with the assay signal. The general and modular design idea made CRISPR-SDA as simple as building blocks to construct nucleic acid sensing methods to meet different requirements by simply changing the SDA template and selecting suitable signal report probes, which was expected to find a breadth of applications in nucleic acids detection.

摘要

快速灵敏地检测核酸在各个领域变得至关重要。然而,大多数当前的核酸检测方法只能在特定场景下使用,例如 RT-qPCR,它依赖于荧光计进行信号读取,由于其价格高昂,限制了其在家庭或现场的应用。在本文中,建立了一种通用的核酸检测平台,将 CRISPR/Cas12a 和链置换扩增 (CRISPR-SDA) 与多种信号读取相结合,以适应不同的应用场景。选择 SARS-CoV-2 的核衣壳蛋白基因 (N 基因) 和乙型肝炎病毒 (HBV) DNA 作为模型靶标。所提出的策略在荧光模式、个人血糖仪 (PGM) 模式和侧向流动测定 (LFA) 模式下分别实现了对 N 基因的灵敏度为 53.1 fM、0.15 pM 和 1 pM。它具有区分单碱基错配的能力,并且存在多达 10 倍于目标物的鲑鱼精 DNA 不会显著干扰测定信号。通用和模块化的设计理念使 CRISPR-SDA 像构建块一样简单,可以通过简单地改变 SDA 模板和选择合适的信号报告探针来构建核酸传感方法,以满足不同的要求,预计在核酸检测中会有广泛的应用。

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引用本文的文献

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Coupling CRISPR-Cas and a personal glucose meter with an enzymatic reporter for portable detection of human papillomavirus in biological samples.将CRISPR-Cas与个人血糖仪相结合,并配备酶促报告基因,用于生物样本中人类乳头瘤病毒的便携式检测。
Theranostics. 2025 Feb 3;15(7):2870-2882. doi: 10.7150/thno.106490. eCollection 2025.
2
Applications of CRISPR/Cas as a Toolbox for Hepatitis B Virus Detection and Therapeutics.CRISPR/Cas 在乙型肝炎病毒检测和治疗中的应用。
Viruses. 2024 Oct 2;16(10):1565. doi: 10.3390/v16101565.
3
Recent Developments in Personal Glucose Meters as Point-of-Care Testing Devices (2020-2024).
即时检测用个人血糖仪的最新进展(2020-2024 年)。
Biosensors (Basel). 2024 Aug 27;14(9):419. doi: 10.3390/bios14090419.