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扩增片段长度多态性指纹图谱:一种检测木薯细菌性萎蔫病菌遗传变异的有效技术。

AFLP fingerprinting: an efficient technique for detecting genetic variation of Xanthomonas axonopodis pv. manihotis.

作者信息

Restrepo Silvia, Duque Myriam, Tohme Joe, Verdier Valérie

机构信息

Biotechnology Unit, Centro Internacional de Agricultural Tropical (CIAT), AA 6713, Cali, Colombia.

Institut Français de Recherche Scientifique pour le Développement en Coopération (ORSTOM), Genetrop, Unité de Phytopathologie, BP5045, 34032 Montpellier, France.

出版信息

Microbiology (Reading). 1999 Jan;145 ( Pt 1):107-114. doi: 10.1099/13500872-145-1-107.

Abstract

Xanthomonas axonopodis pv. manihotis (Xam) is the causative agent of cassava bacterial blight (CBB), a worldwide disease that is particularly destructive in South America and Africa. CBB is controlled essentially through the use of resistant varieties. To develop an appropriate disease management strategy, the genetic diversity of the pathogen's populations must be assessed. Until now, the genetic diversity of Xam was characterized by RFLP analyses using ribotyping, and plasmid and genomic Xam probes. We used AFLP (amplified fragment length polymorphism), a novel PCR-based technique, to characterize the genetic diversity of Colombian Xam isolates. Six Xam strains were tested with 65 AFLP primer combinations to identify the best selective primers. Eight primer combinations were selected according to their reproducibility, number of polymorphic bands and polymorphism detected between Xam strains. Forty-seven Xam strains, originating from different Colombian ecozones, were analysed with the selected combinations. Results obtained with AFLP are consistent with those obtained with RFLP, using plasmid DNA as a probe. Some primer combinations differentiated Xam strains that were not distinguished by RFLP analyses, thus AFLP fingerprinting allowed a better definition of the genetic relationships between Xam strains.

摘要

木薯细菌性枯萎病菌(Xanthomonas axonopodis pv. manihotis,简称Xam)是木薯细菌性枯萎病(CBB)的病原体,这种病害在全球范围内都有发生,在南美洲和非洲尤其具有破坏性。CBB主要通过使用抗病品种来控制。为了制定合适的病害管理策略,必须评估病原菌群体的遗传多样性。到目前为止,Xam的遗传多样性是通过使用核糖体分型、质粒和基因组Xam探针的RFLP分析来表征的。我们使用AFLP(扩增片段长度多态性),一种基于PCR的新技术,来表征哥伦比亚Xam分离株的遗传多样性。用65种AFLP引物组合对6株Xam菌株进行测试,以确定最佳的选择性引物。根据其可重复性、多态性条带数量以及在Xam菌株之间检测到的多态性,选择了8种引物组合。用选定的组合对来自哥伦比亚不同生态区的47株Xam菌株进行了分析。使用质粒DNA作为探针,AFLP获得的结果与RFLP获得的结果一致。一些引物组合区分了RFLP分析无法区分的Xam菌株,因此AFLP指纹图谱能够更好地定义Xam菌株之间的遗传关系。

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