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一种紧凑的微流控平台,用于通过离心偏光吸收光谱法快速多重检测呼吸道病毒。

A compact microfluidic platform for rapid multiplex detection of respiratory viruses via centrifugal polar-absorbance spectroscopy.

机构信息

School of Medical Technology, Zhengzhou Academy of Intelligent Technology, Beijing Institute of Technology, Beijing, 100081, China; School of Biomedical Engineering, Tsinghua University, Beijing, 100084, China.

School of Biomedical Engineering, Tsinghua University, Beijing, 100084, China.

出版信息

Talanta. 2024 Dec 1;280:126733. doi: 10.1016/j.talanta.2024.126733. Epub 2024 Aug 21.

DOI:10.1016/j.talanta.2024.126733
PMID:39173249
Abstract

Nucleic acid detection technology has become a crucial tool in cutting-edge research within the life sciences and clinical diagnosis domains. Its significance is particularly highlighted during the respiratory virus pandemic, where nucleic acid testing plays a pivotal role in accurately detecting the virus. Isothermal amplification technologies have been developed and offer advantages such as rapidity, mild reaction conditions and excellent stability. Among these methods, recombinase polymerase amplification (RPA) has gained significant attention due to its simple primer design and resistance to multiple reaction inhibitors. However, the detection of RPA amplicons hinders the widespread adoption of this technology, leading to a research focus on cost-effective and convenient detection methods for RPA nucleic acid testing. In this study, we propose a novel computational absorption spectrum approach that utilizes the polar GelRed dye to efficiently detect RPA amplicons. By exploiting the asymmetry of GelRed molecules upon binding with DNA, polar electric dipoles are formed, leading to precipitate formation through centrifugal vibration and electrostatic interaction. The quantification of amplicon content is achieved by measuring the residual GelRed concentration in the supernatant. Our proposed portable and integrated microfluidic device successfully detected five respiratory virus genes simultaneously. The optimized linear detection was achieved and the sensitivity for all the targets reached 10 copies/μL. The total experiment could be finished in 27 min. The clinical experiments demonstrated the practicality and accuracy. This cost-effective and convenient detection scheme presents a promising biosensor for rapid virus detection, contributing to the advancement of RPA technology.

摘要

核酸检测技术已成为生命科学和临床诊断领域的前沿研究的重要工具。在呼吸道病毒大流行期间,核酸检测在准确检测病毒方面发挥着关键作用,凸显了其重要性。等温扩增技术得到了发展,并具有快速、温和的反应条件和出色的稳定性等优势。在这些方法中,由于其引物设计简单且能抵抗多种反应抑制剂,重组酶聚合酶扩增(RPA)引起了广泛关注。然而,RPA 扩增子的检测阻碍了这项技术的广泛应用,导致人们研究重点集中在用于 RPA 核酸检测的经济高效且方便的检测方法上。在本研究中,我们提出了一种新颖的计算吸收光谱方法,该方法利用极性 GelRed 染料来高效检测 RPA 扩增子。通过利用 GelRed 分子与 DNA 结合时的不对称性,形成极性电偶极子,通过离心振动和静电相互作用形成沉淀。通过测量上清液中剩余的 GelRed 浓度来定量扩增子含量。我们提出的便携式集成微流控装置成功地同时检测了五种呼吸道病毒基因。实现了优化的线性检测,所有目标的灵敏度均达到 10 拷贝/μL。整个实验可以在 27 分钟内完成。临床实验证明了其实用性和准确性。这种经济高效且方便的检测方案为快速病毒检测提供了一种有前途的生物传感器,推动了 RPA 技术的发展。

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