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利用多重聚合酶链反应快速、特异性鉴定四种土壤杆菌属菌种和生物型。

Rapid and specific identification of four Agrobacterium species and biovars using multiplex PCR.

作者信息

Puławska Joanna, Willems Anne, Sobiczewski Piotr

机构信息

Research Institute of Pomology and Floriculture, ul. Pomologiczna 18, 96-100 Skierniewice, Poland.

出版信息

Syst Appl Microbiol. 2006 Sep;29(6):470-9. doi: 10.1016/j.syapm.2005.11.002. Epub 2005 Dec 15.

Abstract

On the basis of 23S rRNA gene sequences, 1 universal forward and 4 taxon (species/biovar)-specific reverse primers were designed for multiplex PCR to aid in identification and differentiation of Agrobacterium rubi, Agrobacterium vitis and Agrobacterium biovars 1 and 2. In reactions with DNA of 119 bacterial strains belonging to: Agrobacterium, Allorhizobium, Mesorhizobium, Rhizobium, Sinorhizobium and Phyllobacterium, as well as phytopathogenic bacteria representing various genera, the primers developed for identification of A. vitis, A. rubi or Agrobacterium biovar 1 amplified only DNA of strains belonging to these taxa, producing fragments of the expected sizes: 478, 1006 and 184bp, respectively. However, in the case of the primer developed for identification of Agrobacterium biovar 2, the characteristic 1066bp PCR product was obtained not only with DNA of this biovar, but also with DNA of 3 atypical biovar 1 strains and some rhizobial strains. Differentiation between Agrobacterium biovar 2 and the other strains was possible using the restriction analysis of this product with endonuclease Alw26I. The method developed is an excellent tool for rapid classification of these 4 taxa of Agrobacterium.

摘要

基于23S rRNA基因序列,设计了1条通用正向引物和4条分类单元(种/生物变种)特异性反向引物用于多重PCR,以辅助鉴定和区分悬钩子土壤杆菌、葡萄土壤杆菌以及生物变种1和2。在与属于土壤杆菌属、异根瘤菌属、中生根瘤菌属、根瘤菌属、中华根瘤菌属和叶杆菌属的119株细菌菌株的DNA,以及代表各种属的植物病原菌的反应中,为鉴定葡萄土壤杆菌、悬钩子土壤杆菌或土壤杆菌生物变种1而开发的引物仅扩增属于这些分类单元的菌株的DNA,分别产生预期大小的片段:478bp、1006bp和184bp。然而,对于为鉴定土壤杆菌生物变种2而开发的引物,不仅用该生物变种的DNA,而且用3株非典型生物变种1菌株和一些根瘤菌菌株的DNA获得了特征性的1066bp PCR产物。使用Alw26I内切酶对该产物进行限制性分析,可以区分土壤杆菌生物变种2和其他菌株。所开发的方法是对这4个土壤杆菌分类单元进行快速分类的优秀工具。

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