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首页> 外文期刊>African Journal of Microbiology Research >Study on rapid detection of seven common foodborne pathogens by gene chip
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Study on rapid detection of seven common foodborne pathogens by gene chip

机译:基因芯片快速检测七种常见食源性病原体的研究

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摘要

To develop a rapid, effective, specific, and sensitive method to detect foodborne pathogens, 13 sets of primers were designed to amplify the conservative and specific genes of rfbE, fliC, invA, hilA, ipaH, femA, nuc, hlyA, prfA, tuf, speB, tlh and tdh, respectively. Establishment of foodborne pathogens detection chips was conducted by spotting the target genes on the chips by Nano-PlotterTM NP 1.2 printing system. The DNA of 7 standard pathogenic strains and 147 strains extracts from food samples was amplified and labeled for hybridization. The results demonstrated that enterhemorrhagic Escherichia coli O157:H7, Salmonella enteritidis, Shigella flexner, Staphylococcus aureus, Listeria monocytogenes, β-hemolytic streptococcus, and Vibrio parahaemolyticus could correctly be identified by the designed gene chip at an optimal temperature of 58°C and were proved as a potential method with good stability and sensitivity (5 pg/μl of template DNA).
机译:要开发出一种检测食源性病原体的快速,有效,具体和敏感的方法,设计了13套引物,用于扩增RFBE,FLIC,INVA,HILA,IPAH,FEMA,NUC,Hlya,PRFA,TUF的保守和特异性基因,SPEB,TLH和TDH分别。通过将纳米Plottertm NP 1.2印刷系统发现碎片上的靶基因进行食源性病原体检测芯片的建立。 7标准致病菌菌株和147株从食物样品提取物的DNA被扩增并标记以杂交。结果表明,Enterhemorlagic大肠杆菌O157:H7,Salmonella Enteritidis,Shigella Flexiner,金黄色葡萄球菌,Histeria单核细胞增生,β-溶血性链球菌和Vibrio Parahaemolyticus可以通过设计的最佳温度识别58°C,并且是被证明是具有良好稳定性和灵敏度的潜在方法(5 pg /μl模板DNA)。

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