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首页> 外文期刊>Journal of Clinical Microbiology >Spacer oligonucleotide typing of Mycobacterium bovis strains from cattle and other animals: a tool for studying epidemiology of tuberculosis.
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Spacer oligonucleotide typing of Mycobacterium bovis strains from cattle and other animals: a tool for studying epidemiology of tuberculosis.

机译:来自牛和其他动物的牛分枝杆菌菌株的间隔区寡核苷酸分型:研究结核病流行病学的工具。

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The spacer oligonucleotide typing (spoligotyping) method was evaluated for its ability to differentiate Mycobacterium bovis strains. This method detects the presence or absence of spacers of the direct repeat locus of the M. bovis genome. The spacers in the direct repeat locus are amplified by PCR and are detected by hybridization of the biotin-labelled PCR product with a membrane containing oligonucleotides derived from spacer sequences that have previously been bound to a membrane. One hundred eighty-two M. bovis isolates from domestic animals (cattle, goat, sheep, and cats) and wild animals (deer and wild boar) were spoligotyped, and the results were compared with those obtained by IS6110 restriction fragment length polymorphism analysis. Two rather homogeneous clusters of isolates containing 20 and 4 types, respectively, were identified by spoligotyping. The first cluster included isolates from cattle, cats, and feral animals. By spoligotyping, isolates from the Spanish wild boar and deer had the same pattern as some bovine isolates, suggesting transmission between these animals and cattle and highlighting the importance of the study of these reservoirs. The second cluster included all the caprine and ovine isolates. Within each cluster, the patterns of the different strains differed only slightly, suggesting that the spoligotypes may be characteristic of strains from particular animal species. Spoligotyping proved to be useful for studying the epidemiology of bovine M. bovis isolates, especially of those isolates containing only a single copy of IS6110. In view of our results, we suggest fingerprinting all M. bovis strains by the spoligotyping method initially and then by IS6110 restriction fragment length polymorphism typing of the strains belonging to the most common spoligotypes.
机译:评价了间隔区寡核苷酸分型(spoligotyping)方法区分牛分枝杆菌菌株的能力。该方法检测牛分枝杆菌基因组直接重复基因座的间隔子是否存在。通过PCR扩增直接重复基因座中的间隔子,并通过将生物素标记的PCR产物与含有源自先前已结合至膜的间隔子序列的寡核苷酸的膜杂交来检测。对来自家畜(牛,山羊,绵羊和猫)和野生动物(鹿和野猪)的182株牛分枝杆菌进行了盲纹定型,并将结果与​​通过IS6110限制性片段长度多态性分析获得的结果进行了比较。通过Spoligotyping鉴定出两个相当均一的分离株簇,分别包含20和4种类型。第一组包括来自牛,猫和野生动物的分离株。通过spoligotyping,西班牙野猪和鹿的分离株与某些牛分离株具有相同的模式,表明这些动物和牛之间的传播,并突出了研究这些水库的重要性。第二类包括所有的山羊和绵羊分离株。在每个簇中,不同品系的模式仅略有不同,这表明spoligotypes可能是特定动物物种品系的特征。寡核苷酸分型被证明对于研究牛牛分枝杆菌的流行病学是有用的,尤其是那些只包含一个IS6110单拷贝的菌株。鉴于我们的结果,我们建议首先通过分型方法对所有牛分枝杆菌菌株进行指纹识别,然后再对属于最常见的分型类型的菌株进行IS6110限制性片段长度多态性分型。

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