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首页> 外文期刊>Applied and Environmental Microbiology >Toward an International Standard for PCR-Based Detection of Food-Borne Thermotolerant Campylobacters: Assay Development and Analytical Validation
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Toward an International Standard for PCR-Based Detection of Food-Borne Thermotolerant Campylobacters: Assay Development and Analytical Validation

机译:迈向基于PCR的食品耐高温弯曲杆菌细菌检测国际标准:分析开发和分析验证

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As part of a European research project (FOOD-PCR), we developed a standardized and robust PCR detection assay specific for the three most frequently reported food-borne pathogenic Campylobacter species, C. jejuni, C. coli, and C. lari. Fifteen published and unpublished PCR primers targeting the 16S rRNA gene were tested in all possible pairwise combinations, as well as two published primers targeting the 23S rRNA gene. A panel of 150 strains including target and nontarget strains was used in an in-house validation. Only one primer pair, OT1559 plus 18-1, was found to be selective. The inclusivity and exclusivity were 100 and 97%, respectively. In an attempt to find a thermostable DNA polymerase more resistant than Taq to PCR inhibitors present in chicken samples, three DNA polymerases were evaluated. The DNA polymerase Tth was not inhibited at a concentration of 2% (vol/vol) chicken carcass rinse, unlike both Taq DNA polymerase and DyNAzyme. Based on these results, Tth was selected as the most suitable enzyme for the assay. The standardized PCR test described shows potential for use in large-scale screening programs for food-borne Campylobacter species under the assay conditions specified.
机译:作为欧洲研究项目(FOOD-PCR)的一部分,我们针对三种最常报告的食源性致病性 Cam> lobacter C菌种开发了一种标准化且稳定的PCR检测方法。空肠 C。大肠杆菌 C。拉里。以所有可能的成对组合测试了15种已公开和未公开的针对16S rRNA基因的PCR引物,以及两种针对23S rRNA基因的公开引物。在内部验证中使用了包括目标和非目标菌株在内的150株菌株。仅发现一对引物,OT1559加18-1具有选择性。包容性和排他性分别为100%和97%。为了找到对鸡样品中存在的PCR抑制剂比 Taq 更耐高温的DNA聚合酶,评估了三种DNA聚合酶。不同于 Taq DNA聚合酶和DyNAzyme,DNA聚合酶T th 在浓度为2%(体积/体积)的鸡car体冲洗液中均不受抑制。根据这些结果,选择T th 作为最适合该测定的酶。所描述的标准化PCR测试显示了在指定的检测条件下对食源性弯曲杆菌属细菌进行大规模筛选程序的潜力。

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