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On Genotyping Bacterial Strains of the Genera Pectobacterium and Pseudomonas: Pathogens of Bacterioses in Potatoes

机译:关于属植物胶囊和假单胞菌的基因分型细菌菌株:土豆中菌的病原体

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Molecular-genetic research methods make it possible to identify phytopathogens with comprehensive characteristics of their hereditary material. We suggest a genotyping method based on the use of two restriction endonucleases for the cleavage of bacteria's genomic DNA. Taq DNA polymerase added to the reaction mixture provides labeling of DNA fragments with biotinylated deoxycytosinetriphosphate (Bio-dCTP). The label is only incorporated into DNA having 3-prime recessed ends formed by the first enzyme. The second restriction endonuclease produces only blunt ends of fragments that are unable to incorporate the label. As a result of the DDSL (double digest selective label) reaction, 20-50 distinct DNA fragments are visualized on the filter, the amount and distribution of which are specific for each bacterial strain. This research was carried out using two pairs of restriction enzymes (XbaI/DraI and XbaI/Eco24I). The results indicate the same discriminatory capacity of these enzymes. Some advantage was noted for the XbaI/DraI combination, which makes it possible to detect differences in the region of longer DNA fragments in genetic profiles. The genetic profile generated by the BcuI/Eco32I pair of enzymes in Ps. fluorescens 894 was significantly different from that of Ps. xanthochlora, which could be anticipated while comparing these two species. In general, the results of genotyping agreed with the data on the origin of bacterial strains. In particular, microorganisms with the same genetic profile, D822 and D828, G399 and G400, as well as C960 and C966, were obtained from affected tubers of the same experimental field. This suggests the possibility of the contact spread of the pathogen. In some cases, the identity of strains was observed, despite their different geographic origin. This fact confirms contamination that occurred in the past during the use of the foreign seed potato.
机译:分子遗传研究方法可以鉴定具有遗传物质的综合特征的植物病变。我们建议一种基于使用两种限制性内切核酸酶的基因分型方法,用于细菌的基因组DNA的切割。加入到反应混合物中的Taq DNA聚合酶提供与生物素化的脱氧胞嘧啶四磷酸(Bio-DCTP)的DNA片段的标记。标记仅掺入具有由第一酶形成的3-初始凹陷端的DNA。第二限制性内切核酸酶仅产生不能掺入标记的片段的钝端。作为DDSL(双摘要选择标签)反应的结果,在过滤器上可视化20-50个不同的DNA片段,其量和分布对于每种细菌菌株是特异性的。使用两对限制酶(XBAI / DRAI和XBAI / ECO24i)进行该研究。结果表明这些酶的相同歧视能力。 Xbai / Drai组合注意了一些优点,这使得可以检测遗传谱中较长DNA片段区域的差异。 BCUI / Eco32i对PS中的遗传谱。荧光荧光素894与PS的荧光素显着不同。 Xanthochlora,可以在比较这两个物种的同时预期。通常,基因分型结果与细菌菌株的起源的数据同意。特别地,具有相同遗传谱,D822和D828,G399和G400以及C960和C966的微生物是从相同实验领域的受影响的块茎获得的。这表明病原体的接触扩散的可能性。在某些情况下,尽管其不同的地理来源,观察到菌株的身份。这一事实证实了过去在使用外国种子马铃薯期间发生的污染。

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