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首页> 外文期刊>FEMS Microbiology Letters >Development of PCR assay based on ITS2 rDNA polymorphism for the detection and differentiation of Fusarium sporotrichioides
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Development of PCR assay based on ITS2 rDNA polymorphism for the detection and differentiation of Fusarium sporotrichioides

机译:基于ITS2 rDNA多态性的PCR检测试剂盒的开发用于孢子孢镰刀菌的检测和鉴别

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摘要

A polymerase chain reaction assay was developed for detection of Fusarium sporotrichioides, a plant pathogen in many parts of the world. Based on small nucleotide differences in ITS2 (Internal Transcribed Spacer) rDNA of our local isolate of F sporotrichioides (Accession No. AY510069) and other isolates found in NCBI/GeneBank database, species specific primer FspITS2K was selected. Primer pair FspITS2K and P28SL amplified a fragment of 288 bp containing a portion of ITS2 and 28S rDNA of all the F. sporotrichioides isolates tested, originated from different hosts and regions of the world but did not amplify any other species of Fusarium and plant's DNA. To use the PCR assay in seed health testing, a protocol was setup for the rapid and effective preparations of fungal DNA from wheat seeds. The method developed may be useful for the rapid detection and identification of F. sporotrichioides both from culture and from plant tissue. (C) 2004 Federation of European Microbiological Societies. Published by Elsevier B.V. All rights reserved.
机译:开发了一种聚合酶链反应测定法,用于检测世界许多地方的植物病原体镰孢镰刀菌。根据我们的F孢子虫局部分离株(保藏号AY510069)和在NCBI / GeneBank数据库中发现的其他分离株的ITS2(内部转录间隔区)rDNA的微小核苷酸差异,选择了物种特异性引物FspITS2K。引物对FspITS2K和P28SL扩增了一个288 bp的片段,其中包含来自世界各地的不同宿主和地区的所有受试孢子虫分离株的ITS2和28S rDNA的一部分,但未扩增任何其他镰刀菌和植物DNA。为了在种子健康测试中使用PCR分析,建立了从小麦种子中快速有效制备真菌DNA的方案。所开发的方法可用于从培养物和植物组织中快速检测和鉴定孢子丝孢菌。 (C)2004年欧洲微生物学会联合会。由Elsevier B.V.发布。保留所有权利。

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