植物病原体检测的进展:重组酶聚合酶扩增与 CRISPR/Cas 系统的整合。

IF 2.6 4区 生物学 Q3 BIOTECHNOLOGY & APPLIED MICROBIOLOGY 3 Biotech Pub Date : 2024-09-01 Epub Date: 2024-08-27 DOI:10.1007/s13205-024-04055-x
P Anbazhagan, B Parameswari, K Anitha, G V Chaitra, Bhaskar Bajaru, A Rajashree, S K Mangrauthia, Faisal Yousuf, V Celia Chalam, G P Singh
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引用次数: 0

摘要

植物病原体正在造成巨大的经济损失,因而成为全球农业的重大威胁。有效、及时的检测方法是应对植物病原体造成的损失的先决条件。在植物病原体检测领域,等温扩增技术,如重组酶聚合酶扩增(RPA)和环介导等温扩增(LAMP),已成为传统 PCR 的快速、精确和最灵敏的替代方法,但它们往往存在非特异性扩增率高和操作复杂的问题。近年来,聚类规则间隔短回文重复序列(CRISPR)和与 CRISPR 相关的核酸酶 Cas 系统,特别是 Cas12,已成为高灵敏度、特异性和快速病原体检测的强大工具。Cas12 可选择性地裂解单链 DNA(ssDNA),利用 Cas12 的附带活性,新型检测平台应运而生。其机理是形成一个由导向 RNA、Cas12 酶和底物靶核苷酸序列组成的三重复合分子。识别到目标后,Cas12 会不加区分地裂解 DNA 链,导致裂解的 ssDNA 报告释放荧光。将等温扩增方法与 CRISPR/Cas12 相结合,可实现一步检测测定,从而在 30 分钟内以单一温度快速鉴定病原体。这种集成的 RPA-CRISPR/Cas12a 方法无需提取 RNA 和转换 cDNA,可直接使用粗植物汁液作为模板。通过经济实惠的荧光可视化系统,这种便携式方法的灵敏度比传统技术高出 100 倍。本综述总结了用于检测植物病原体的 RPA-CRISPR/Cas12a 的最新进展,包括引物设计、田间便携性和灵敏度的提高。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Advances in plant pathogen detection: integrating recombinase polymerase amplification with CRISPR/Cas systems.

Plant pathogens are causing substantial economic losses and thus became a significant threat to global agriculture. Effective and timely detection methods are prerequisite for combating the damages caused by the plant pathogens. In the realm of plant pathogen detection, the isothermal amplification techniques, e.g., recombinase polymerase amplification (RPA) and loop-mediated isothermal amplification (LAMP), have emerged as a fast, precise, and most sensitive alternative to conventional PCR but they often comprise high rates of non-specific amplification and operational complexity. In recent advancements, clustered regularly interspaced short palindromic repeats (CRISPR) and CRISPR-associated nuclease Cas systems, particularly Cas12, have emerged as powerful tools for highly sensitive, specific, and rapid pathogen detection. Exploiting the collateral activities of Cas12, which selectively cleaves single-stranded DNA (ssDNA), novel detection platforms have been developed. The mechanism employs the formation of a triple complex molecule comprising guide RNA, Cas12 enzyme, and the substrate target nucleotide sequence. Upon recognition of the target, Cas12 indiscriminately cleaves the DNA strand, leading to the release of fluorescence from the cleaved ssDNA reporter. Integration of isothermal amplification methods with CRISPR/Cas12 enables one-step detection assays, facilitating rapid pathogen identification within 30 min at a single temperature. This integrated RPA-CRISPR/Cas12a approach eliminates the need for RNA extraction and cDNA conversion, allowing direct use of crude plant sap as a template. With an affordable fluorescence visualization system, this portable method achieves 100-fold greater sensitivity than conventional techniques. This review summarizes recent advances in RPA-CRISPR/Cas12a for detecting plant pathogens, covering primer design, field-level portability, and enhanced sensitivity.

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来源期刊
3 Biotech
3 Biotech Agricultural and Biological Sciences-Agricultural and Biological Sciences (miscellaneous)
CiteScore
6.00
自引率
0.00%
发文量
314
期刊介绍: 3 Biotech publishes the results of the latest research related to the study and application of biotechnology to: - Medicine and Biomedical Sciences - Agriculture - The Environment The focus on these three technology sectors recognizes that complete Biotechnology applications often require a combination of techniques. 3 Biotech not only presents the latest developments in biotechnology but also addresses the problems and benefits of integrating a variety of techniques for a particular application. 3 Biotech will appeal to scientists and engineers in both academia and industry focused on the safe and efficient application of Biotechnology to Medicine, Agriculture and the Environment.
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