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Detection and Enumeration of Vibrio vulnificus by Direct Colony Immunoblot

机译:直接菌落免疫印迹法检测和计数弧菌弧菌

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A direct colony immunoblot method (DCI) for the enumeration of Vibrio vulnificus was developed. Bacterial colonies were transferred from agar plates to membranes, which were then dried and blocked with bovine serum albumin. Subsequently, the membranes were treated with anti- V. vulnificus H antibodies, washed and incu-bated with peroxidase-conjugated goat anti-rabbit IgG. After a final wash, the membranes were exposed to a sub-strate mixture containing H_2O_2 which resulted in the development of a purple color by V. vulnificus colonies. The DCI detected all clinical and environmental V. vulnificus strains tested and did not cross-react with other Vibrio species including V. cholerae, V. parahaemolyticus, or V.fluvialis. The DCI was then compared to the DNA hybridiza-tion procedure (DNAH) using V. vulnificus agar plates inoculated with mixed cultures of V. vulnificus and V. para-haemolyticus and V. vulnificus-seeded oyster homogenatcs. Both DCI and DNAH delected 1 to 2 log colony forming units (CFU)/mL V. vulnificus mixed with 4 log CFU/mL V. parahaemolyticus. Both methods were comparable and demonstrated no significant statistical differences when enumerating V. vulnificus in mixed cultures or in oyster homogenates seeded with levels of V. vulnificus from 2 to 8 log CFU/mL. The DCI demonstrated clearer color devel-opment and was less time consuming than the DNAH.
机译:开发了一种直接菌落免疫印迹法(DCI),用于计数弧菌。将细菌菌落从琼脂平板转移到膜上,然后干燥并用牛血清白蛋白封闭。随后,将膜用抗V. vulnificus H抗体处理,洗涤并用过氧化物酶偶联的山羊抗兔IgG诱导。在最终洗涤之后,将膜暴露于含有H_2O_2的底物混合物,其导致创伤弧菌菌落形成紫色。 DCI检测到所有测试过的临床和环境创伤弧菌菌株,并且未与其他霍乱弧菌物种(包括霍乱弧菌,副溶血弧菌或流感弧菌)发生交叉反应。然后,用接种了V. vulnificus和V. para-haemolyticus以及V. vulnificus的牡蛎苗均质混合培养的V. vulnificus琼脂平板,将DCI与DNA杂交程序(DNAH)进行比较。 DCI和DNAH均以1-2个对数菌落形成单位(CFU)/ mL创伤弧菌与4 logCFU / mL副溶血弧菌混合。两种方法均具有可比性,并且在混合培养物中或在接种V. vulnificus的水平为2至8 log CFU / mL的牡蛎匀浆中计数V. vulnificus时,无统计学差异。 DCI显示出比DNAH更清晰的色彩开发,并且耗时更少。

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