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Detection of Listeria monocytogenes through real-time PCR and biosensor methods

机译:通过实时荧光定量PCR和生物传感器方法检测单核细胞增生李斯特菌

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Listeria monocytogenes is a foodborne pathogen causing listeriosis, especially in sensitive individuals such as children, pregnant women and persons with compromised immune systems. This pathogen has been isolated from different food products, but milk products surely play a major role in the epidemiology of this foodborne disease. Identification traditionally involved culture methods based on selective enrichment and plating followed by the characterization of Listeria spp. based on colony morphology, sugar fermentation and haemolytic properties. These methods are the gold standard, but in the last years more rapid tests were developed based on antibodies (ELISA) or molecular techniques (PCR or DNA hybridization). More recently, molecular methods were developed that target RNA rather than DNA, such as RT-PCR, real time PCR or nucleic acid sequence-based amplification (NASBA). In this review, real-time PCR assays, protein chip methods and label-free SPR immunosensors were compared for their application in bacterial detection.
机译:单核细胞增生李斯特菌是引起李斯特菌病的食源性病原体,尤其是在敏感的个体,例如儿童,孕妇和免疫系统受损的人中。该病原体已从不同的食品中分离出来,但是乳制品无疑在这种食源性疾病的流行病学中起着重要作用。鉴定传统上涉及基于选择性富集和铺板的培养方法,然后表征李斯特菌。基于菌落形态,糖发酵和溶血特性。这些方法是黄金标准,但是在最近几年中,基于抗体(ELISA)或分子技术(PCR或DNA杂交)开发了更加快速的测试方法。最近,开发了靶向RNA而非DNA的分子方法,例如RT-PCR,实时PCR或基于核酸序列的扩增(NASBA)。在这篇综述中,实时荧光定量PCR检测,蛋白质芯片方法和无标记SPR免疫传感器在细菌检测中的应用进行了比较。

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