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A Rapid PCR-Reverse Dot Blot Method for the Identification of Bacterial Intestial Pathogens in Blood Samples

机译:一种快速的PCR反向点印迹方法,用于鉴定血液样本中的细菌肠道病原体

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Intestinal infections which are the important public health concern worldwide, are caused by the bacterial intestinal pathogens. The aim of our study is to develop a simultaneous, rapid, sensitive and specific diagnostic assay by using a combined PCR-Reverse dot blot method for the identification of pathogen strains, including Bacillus cereus, Clostridium botulinum, Clostridium perfringen, Staphylococcus aureus, Listeria monocytogenes, Escherichia coli 0157:H7, Salmonella spp., Shigella spp., Vibrio cholerae, Vibrio parahaemolyticus, Yersinia enterocolitica va Brucella spp. Based on the 16S and 23S DNA regions, the two sets of universal primers and twelve specific probes were obtained for amplification and specific detection of those twelve bacterial species. The initial experimental results using bacterial cultures and 50 clinical samples confirmed the in silico hypothesis that was previously established in universal primers and probes design as well as identified with some basic conditions for PCR and Reverse Dot Blot hybridization reactions. Thus, this procedure being further tested for the other kinds of samples such as fecal samples or foods.
机译:肠道感染是全世界重要的公共卫生关注的肠道感染是由细菌肠道病原体引起的。我们的研究目的是通过使用组合的PCR反向点印迹方法来制定同时,快速,敏感和特异性的诊断测定方法,用于鉴定病原体菌株,包括芽孢杆菌,肉毒杆菌,梭菌菌株,流产大肠,金黄色葡萄球菌,李斯特菌单核细胞增生,大肠杆菌0157:H7,Salmonella SPP。,Shigella SPP,霍乱霍乱,Vibrio Parahaemolyticus,Yersinia Enterocolitica Va Brucella SPP。基于16S和23S DNA区域,获得两组通用引物和12种特异性探针,用于扩增和特异性检测那些12种细菌物种。使用细菌培养物和50个临床样品的初始实验结果证实了先前在环球引物和探针设计中建立的硅假设,以及用一些基本条件鉴定为PCR和反向点染色杂交反应。因此,该过程正在进一步测试其他种类的样品,例如粪便样品或食物。

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