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使用种特异性引物通过聚合酶链反应检测禾顶囊壳菌变种

Detection of Gaeumannomyces graminis Varieties Using Polymerase Chain Reaction with Variety-Specific Primers.

作者信息

Fouly H M, Wilkinson H T

机构信息

Department of Natural Resources and Environmental Sciences, University of Illinois at Urbana-Champaign, Urbana 61801.

出版信息

Plant Dis. 2000 Sep;84(9):947-951. doi: 10.1094/PDIS.2000.84.9.947.

Abstract

The polymerase chain reaction (PCR) was used for detection of Gaeumannomyces graminis, the causal agent of take-all disease in wheat, oats, and turfgrass. NS5 and NS6 universal primers amplified the middle region of 18S ribosomal DNA of Gaeumannomyces species and varieties. Primers GGT-RP (5' TGCAATGGCTTCGTGAA 3') and GGA-RP (5' TTTGTGTGTGAC CATAC 3') were developed by sequence analysis of cloned NS5-NS6 fragments. The primer pair NS5:GGT-RP amplified a single 410-bp fragment from isolates of G. graminis var. tritici, a single 300-bp fragment from isolates of G. graminis var. avenae, and no amplification products from isolates of G. graminis var. graminis or other species of Gaeumannomyces. The primer pair NS5:GGA-RP amplified a single 400-bp fragment from isolates of varieties tritici and avenae. Two sets of primer pairs (NS5:GGT-RP and NS5:GGA-RP) were used in PCR reactions to detect and identify the varieties tritici and avenae either colonizing wheat, oats, or grass roots, or in culture. No amplification products were observed using DNA extracted from plants infected with eight other soilborne fungal pathogens or from uninoculated plants.

摘要

聚合酶链反应(PCR)用于检测禾顶囊壳菌,它是小麦、燕麦和草坪草全蚀病的致病因子。NS5和NS6通用引物扩增了禾顶囊壳菌物种和变种18S核糖体DNA的中间区域。通过对克隆的NS5-NS6片段进行序列分析,开发了引物GGT-RP(5' TGCAATGGCTTCGTGAA 3')和GGA-RP(5' TTTGTGTGTGAC CATAC 3')。引物对NS5:GGT-RP从小麦禾顶囊壳变种的分离株中扩增出一个410 bp的片段,从燕麦禾顶囊壳变种的分离株中扩增出一个300 bp的片段,而从禾顶囊壳变种或其他禾顶囊壳菌物种的分离株中未扩增出产物。引物对NS5:GGA-RP从小麦变种和燕麦变种的分离株中扩增出一个400 bp的片段。两组引物对(NS5:GGT-RP和NS5:GGA-RP)用于PCR反应,以检测和鉴定定殖于小麦、燕麦或草根中的小麦变种和燕麦变种,或用于检测培养物中的这些变种。使用从感染其他八种土传真菌病原体的植物或未接种植物中提取的DNA未观察到扩增产物。

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