Non-gel based techniques for plant pathogen genotyping.

Acta microbiologica Polonica Pub Date : 2003-01-01
Kamel A Abd-Elsalam
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Abstract

The introduction of real-time PCR technology has significantly improved and simplified the quantification of nucleic acids, and this technology has become an invaluable tool for many scientists working in different disciplines. Particularly in the field of molecular diagnostics and genotyping, real-time PCR-based assays have gained favour in the recent past. Rapid real-time PCR diagnosis can result in appropriate control measures and eradication procedures in a faster and more accurate way than traditional methods based on pathogen isolation. Real-time quantitative PCR represents a highly sensitive and powerful technique for the gel-free detection of nucleic acids. In this review, the main chemistries used for the detection of PCR product during real-time PCR, as well as advantages and limitations of real-time PCR will be depicted. Furthermore, the existing literature as it applies to plant pathogens detection in the routine and research laboratory will be reviewed in order to focus on one of the many areas in which the application of real-time PCR has provided significant methodological benefits.

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植物病原体基因分型的非凝胶技术。
实时PCR技术的引入大大改善和简化了核酸的定量,该技术已成为许多从事不同学科的科学家的宝贵工具。特别是在分子诊断和基因分型领域,基于实时聚合酶链反应的分析在最近的过去获得了青睐。与基于病原体分离的传统方法相比,快速实时PCR诊断可以更快、更准确地产生适当的控制措施和根除程序。实时定量PCR是一种高灵敏度和强大的无凝胶核酸检测技术。本文将介绍实时聚合酶链反应中用于检测PCR产物的主要化学物质,以及实时聚合酶链反应的优点和局限性。此外,现有的文献,因为它适用于植物病原体检测在常规和研究实验室将进行审查,以集中在其中一个领域,实时PCR的应用已经提供了显著的方法学上的好处。
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