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首页> 外文期刊>Research in Microbiology >Comparison of 16SrDNA and toxR genes as targets for detection of Vibrio anguillarum in Dicentrarchus labrax kidney and liver.
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Comparison of 16SrDNA and toxR genes as targets for detection of Vibrio anguillarum in Dicentrarchus labrax kidney and liver.

机译:比较16SrDNA和toxR基因作为检测Dicentrarchus labrax肾脏和肝脏中鳗弧菌的靶标。

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Vibrio anguillarum is a pathogen that causes high mortality in marine and freshwater fish. The aim of this study was to develop a real-time PCR assay for identification and quantification of V. anguillarum in fish tissue. The assay was carried out using two target genes, 16SrDNA and toxR, to evaluate the influence of differences in the operon copy number in quantitative assessment, both in pure cultures of V. anguillarum serovar O1 (strain 975/I), as a reference, and in the liver and kidney of a sea bass (Dicentrarchus labrax) specimen. Real-time PCR analysis showed high specificity for both target genes, with a detection limit of approximately 1-10 bacterial cells per reaction in pure culture and 10/100 V. anguillarum cells per reaction in fish tissue, which corresponds to 2 x 10(2)/2 x 10(3) cells g(-1) fish tissue. Moreover, both genes showed high specificity but differing sensitivity due to the different operon copy number; as a result, it is possible to target the high copy number gene to improve sensitivity. Our results suggest that the protocol we tested can be used as a sensitive and specific molecular method for the detection of the fish pathogen V. anguillarum in fish tissue.
机译:鳗弧菌是引起海洋和淡水鱼类高死亡率的病原体。这项研究的目的是开发一种实时PCR分析方法,用于鉴定和定量鱼类组织中的鳗弧菌。该分析是使用两个靶基因16SrDNA和toxR进行的,以评估定量评估中操纵子拷贝数差异的影响,这两种情况均以纯鳗弧菌血清O1(菌株975 / I)作为参考,以及鲈鱼(Dicentrarchus labrax)标本的肝脏和肾脏中。实时PCR分析显示了对两种靶基因的高特异性,在纯培养物中每个反应的检出限约为1-10个细菌细胞,在鱼组织中每个反应的检出限为10/100 V.鳗鱼细胞,相当于2 x 10( 2)/ 2 x 10(3)个细胞g(-1)鱼组织。此外,由于操纵子拷贝数不同,两个基因均显示出高特异性,但敏感性不同。结果,可以靶向高拷贝数基因以提高灵敏度。我们的结果表明,我们测试的方案可以用作检测鱼组织中鱼病原体V. anguillarum的灵敏且特异的分子方法。

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