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Synergetic performance of isothermal amplification techniques and lateral flow approach for nucleic acid diagnostics

机译:等温扩增技术的协同性能与核酸诊断的侧向流动方法

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摘要

The advancement in developing sensitive, rapid, and specific sensing tools is crucial in diagnostics and biotechnological applications. Although various isothermal amplification approaches exist for the detection and identification of nucleic acids, post-amplicon analysis is still based on traditional methods such as gel electrophoresis, colorimetry, turbidity, which could be non-specific and inconvenient. Thus, this review will first elaborate various isothermal amplification techniques (principle, merits, and demerits) and their potentials when combined with lateral flow approach for point-of-care nucleic acid diagnostics. Different methods for monitoring carryover contamination resulting from amplification product contamination will be discussed. Then, we will present recent advances in diagnostics with both target pre-amplification and CRISPR-Cas systems, which exhibit collateral cleavage of target nucleic acid and a reporter single strand nucleic acid within the vicinity. When the reporter is fluorophore-labeled, it provides a detectable signal by fluorescence or lateral flow biosensors. Lastly, we will discuss how CRISPR-Cas system based diagnostics could be more effective, affordable and portable for on-site detection.
机译:开发敏感,快速和特异性传感工具的进步在诊断和生物技术应用中至关重要。尽管存在用于检测和识别核酸的各种等温扩增方法,但扩增后分析仍然基于传统方法,例如凝胶电泳,比色法,浊度,这可能是非特异性和不方便的。因此,本综述首先将首先在与护理点核酸诊断结合的侧向流动方法结合时,首先详细说明各种等温放大技术(原理,优点和缺点)及其潜力。将讨论用于监测来自扩增产物污染的携带污染的不同方法。然后,我们将在靶预扩增和CRISPR-CAS系统中提出诊断的最新进展,其在附近表现出靶核酸的抵押品切割和附近的报告单链核酸。当报告器是荧光团标记时,它通过荧光或横向流动生物传感器提供可检测信号。最后,我们将讨论基于CAS系统的CASP-CAS系统如何更有效,可承受的,可用于现场检测。

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