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Molecular intraspecific characterization of Photobacterium damselae ssp damselae strains affecting cultured marine fish

机译:影响养殖海水鱼类的淡色杆菌ssp damselae菌株的分子种内表征

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Aims:The aim of this study was to analyse the intraspecific variability of Photobacterium damselae ssp. damselae strains isolated from different cultured marine fish species using molecular typing methods.Methods and Results:Twenty P. damselae ssp. damselae strains isolated from marine fish species were used in this study. Phenotypic characterization of the strains was carried out using standard microbiological methods. Genetic characterization was conducted using three PCR-based methods [random amplified polymorphic DNA (RAPD), enterobacterial repetitive intergenic consensus-PCR (ERIC-PCR) and repetitive extragenic palindromic-PCR (REP-PCR)]. Dice coefficient and the unweighted pair group method with average linkage were used for numerical analyses of banding patterns. At phenotypic level, the strains analysed showed seven different profiles, which could not be related to the host fish species, geographic area or outbreak of disease. Isolates were grouped into nine and eight clusters using the RAPD technique with primers 5 and 4, respectively. In both cases, the main cluster grouped 45% of strains. The techniques ERIC-PCR and REP-PCR were more discriminatory, both resulting in 14 different clusters, which grouped 15-20% of the isolates.Conclusions:In this study, the techniques tested are confirmed as good tools for molecular typing, because they allow discrimination between P. damselae ssp. damselae strains isolated within the same outbreak. In addition, ERIC-PCR and REP-PCR methods were more adequate for rapid typing of P. damselae ssp. damselae than RAPD, allowing the discrimination at strain level.Significance and Impact of the Study:The results, in agreement with previous studies, confirmed the high intraspecific variability among isolated P. damselae ssp. damselae strains at both phenotypic and genetic levels. This suggests the existence of different clonal lineages that coexist in the same geographic area, within a short period of time (2-3 years). The discrimination at strain level can be useful to study the traceability of infections.
机译:目的:本研究的目的是分析damselae ssp。细菌的种内变异性。用分子分型方法从不同养殖海水鱼种中分离出丹苏拉菌株。方法与结果:二十个丹参体育本研究使用从海水鱼类中分离出的丹苏拉菌株。使用标准的微生物学方法对菌株进行表型鉴定。使用三种基于PCR的方法[随机扩增多态DNA(RAPD),肠细菌重复性基因间共有PCR(ERIC-PCR)和重复性基因外回文PCR(REP-PCR)]进行基因表征。使用骰子系数和具有平均连锁度的非加权对群方法进行带状谱图的数值分析。在表型水平上,所分析的菌株显示出七个不同的特征,这与宿主鱼类的种类,地理区域或疾病爆发无关。使用RAPD技术分别将引物5和4分离为9个和8个簇。在这两种情况下,主群均占菌株的45%。 ERIC-PCR和REP-PCR技术具有更高的歧视性,都产生了14个不同的簇,将15-20%的分离株分组。允许区分P. damselae ssp。在同一次暴发中分离出的年轻女孩菌株。此外,ERIC-PCR和REP-PCR方法更适合快速进行damselae ssp的快速分型。该研究的意义和影响:该结果与以前的研究一致,证实了分离的假单胞菌种中的种内变异性很高。在表型和遗传水平上的Damselae菌株。这表明在短时间内(2-3年),在同一地理区域中共存不同克隆世系。在菌株水平上的区分对于研究感染的可追溯性可能是有用的。

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