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Genetic characterization of Erwinia amylovora strains by amplified fragment length polymorphism

机译:扩增片段长度多态性对解淀粉欧文氏菌的遗传鉴定

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Aims: Erwinia amylovora is one of the most important pathogens of pear and apple and is subject to strict quarantine regulations worldwide, although its patterns of dispersal are largely unknown. Previous attempts to fingerprint E. amylovora strains by molecular techniques have detected very little polymorphism because of the high genetic homogeneity of this bacterium. Our aim was to establish and test a typing method to quantify genetic diversity among strains of this plant pathogen. Methods and Results: Twenty-two strains from different hosts and geographical locations were examined by PCR fingerprinting with four primers and by amplified fragment length polymorphism (AFLP) with four selected combinations of primers with a single base extension. PCR fingerprinting revealed little polymorphism producing the same amplification patterns for 17 strains, while the combined AFLP patterns yielded 78 polymorphic bands (34% of total bands) and allowed the differentiation of all but two strains. Clustering of strains in the resulting dendrogram was not correlated with host, year or country of isolation, and questions previous genealogies based on PFGE patterns. Conclusions: The AFLP technique allowed the detection of an unprecedented number of genetic markers in E. amylovora and proved to be the most useful tool so far for discriminating among strains of this pathogen. The results obtained in this study strongly suggest the occurrence of multiple introductions of the pathogen in Spain and other European countries. Significance and Impact of the Study: A major limitation in understanding the ecology of fire blight is the lack of typing techniques with a high power of discrimination. This study demonstrates the high resolution and the usefulness of the AFLP technique to differentiate among E. amylovora strains.
机译:目的:解淀粉欧文氏菌是梨和苹果最重要的病原体之一,尽管其传播方式在很大程度上尚不清楚,但全世界都受到严格的检疫法规的约束。由于该细菌的高遗传同质性,以前通过分子技术对支链淀粉菌菌株进行指纹鉴定的尝试几乎没有检测到多态性。我们的目标是建立和测试一种分型方法,以量化这种植物病原体菌株之间的遗传多样性。方法和结果:通过使用四个引物的PCR指纹图谱和使用四个具有单碱基延伸的引物组合的扩增片段长度多态性(AFLP)检测了来自不同宿主和地理位置的22个菌株。 PCR指纹图谱显示几乎没有多态性,可对17个菌株产生相同的扩增模式,而组合的AFLP模式可产生78个多态性条带(占总条带的34%),并允许除两个菌株外的所有菌株进行分化。结果树状图中菌株的聚类与寄主,年份或隔离国家无关,并根据PFGE模式质疑以前的家谱。结论:AFLP技术可以检测出支链淀粉中史无前例的遗传标记,并被证明是迄今为止区分该病原体的最有用工具。这项研究获得的结果强烈表明,西班牙和其他欧洲国家多次引入病原体。研究的意义和影响:了​​解火疫病的主要局限性在于缺乏具有高判别力的打字技术。这项研究证明了高分辨率和AFLP技术的区别在支链淀粉中的菌株。

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