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首页> 外文期刊>Veterinary Microbiology >Validation of an open-formula, diagnostic real-time PCR method for 20-h detection of Salmonella in animal feeds.
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Validation of an open-formula, diagnostic real-time PCR method for 20-h detection of Salmonella in animal feeds.

机译:用于动物饲料中沙门氏菌20小时检测的开放式诊断实时PCR方法的验证。

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A comparative study of a 20-h, non-commercial, open-formula PCR method and the standard culture-based method NMKL 187, for detection of Salmonella, was performed according to the validation protocol from the Nordic organisation for validation of alternative microbiological methods (NordVal) on 81 artificially or naturally contaminated animal feed samples. The PCR method is based on culture enrichment in buffered peptone water for 16 +or- 2h followed by a magnetic beads based semi automated DNA extraction and real-time PCR analysis, including an internal amplification control. The limit of detection (LOD50) was found to be 7.19 and 7.24 CFU/sample for the PCR method and NMKL187, respectively. A very good correlation between results obtained by the two methods was found (Cohen's kappa = 0.92). The relative accuracy, relative sensitivity and relative specificity were found to be 97.5%, 102.0% and 96.6%, respectively. This method is the fastest open PCR based analysis protocol for detection of Salmonella in feed samples. Implementing rapid methods such as the one validated in this study can speed up Salmonella testing of feed for food-producing animals. All rights reserved, Elsevier.
机译:根据北欧的验证方案,对20小时非商业性开放式PCR方法与基于标准培养物的NMKL 187检测沙门氏菌的方法进行了比较研究。组织对81种人工或自然污染的动物饲料样品的替代微生物方法(NordVal)进行验证。 PCR方法基于缓冲蛋白ept水中的培养物富集16 +或2h,然后进行基于磁珠的半自动DNA提取和实时PCR分析,包括内部扩增对照。 PCR方法和NMKL187的检出限(LOD50)分别为7.19和7.24 CFU /样品。发现通过两种方法获得的结果之间具有很好的相关性(科恩卡帕值= 0.92)。发现相对准确度,相对灵敏度和相对特异性分别为97.5%,102.0%和96.6%。此方法是用于检测饲料样品中沙门氏菌的最快的基于开放式PCR的分析方案。实施快速的方法(如本研究中验证的方法)可以加快食品生产动物饲料的沙门氏菌检测。保留所有权利,Elsevier。

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