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Novel multiplex polymerase chain reaction and an oligonucleotide array for specific detection of the dominant foodborne bacterial pathogens in chicken meat

机译:新型多重聚合酶链反应和寡核苷酸阵列可特异性检测鸡肉中主要的食源性细菌病原体

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Oligonucleotide array hybridisation and multiplex polymerase chain reaction (m-PCR) can be used to screen and detect multiple foodborne pathogens. In our study, m-PCR and oligonucleotide array assays for the specific detection of the dominant foodborne bacterial pathogens, including?Escherichia coli,?Listeria monocytogenes,?Salmonella?spp., andShigella?spp., in chicken meat were developed. The combination of m-PCR and an oligonucleotide array targeting the 16S rRNA,?uspA,?prfA,?fimY, and?ipaH?genes displayed a high?discriminatory power among the aforementioned genera and species with low or no incidence of false negative results. Our combined methods could detect all 4 target bacteria at amounts as low as 1 ng of each from mixed genomic DNA extracted from pure cultures, which?is equivalent to 104-106?CFU/ml. After enrichment steps for the target bacteria,?E. coli,?L. monocytogenes, and?Salmonella?sp. could be detected simultaneously from fresh chicken samples. Combining the two methods could enhance accuracy and sensitivity for foodborne pathogen detection and identification. The problems of cross-reactivities from non-target bacteria isolated from an enrichment culture and the difficulties in result interpretation by m-PCR could be solved using our oligonucleotide array hybridisation method.
机译:寡核苷酸阵列杂交和多重聚合酶链反应(m-PCR)可用于筛选和检测多种食源性病原体。在我们的研究中,开发了用于特异性检测鸡肉中主要食源性细菌病原体(包括大肠杆菌,单核细胞增生李斯特菌,沙门氏菌和志贺氏菌)的m-PCR和寡核苷酸阵列测定法。 m-PCR和靶向16S rRNA,?uspA,?prfA,?fimY和?ipaH?基因的寡核苷酸阵列的组合在上述属和种中显示出较高的区分能力,假阴性结果发生率低或没有发生率。我们的联合方法可以从纯培养物提取的混合基因组DNA中检测到所有4种目标细菌,其每种细菌的量低至1 ng,这相当于104-106?CFU / ml。针对目标细菌的富集步骤后,大肠杆菌单核细胞增生和沙门氏菌。可以从新鲜鸡肉样品中同时检测到。结合使用这两种方法可以提高食源性病原体检测和鉴定的准确性和敏感性。使用我们的寡核苷酸阵列杂交方法可以解决从富集培养物中分离出的非目标细菌的交叉反应性问题以及通过m-PCR进行结果解释的困难。

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