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Ultrasensitive detection and rapid identification of multiple foodborne pathogens with the naked eyes

机译:用肉眼超灵敏检测和快速鉴定多种食源性病原体

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摘要

In this study, a novel approach for ultrasensitive detection and rapid high-throughput identification of a panel of common foodborne pathogens with the naked eyes is presented. As a proof-of-concept application, a multiple pathogen analysis array is fabricated through immobilizing three specific polyT-capture probes which can respectively recognize rfbE gene (Escherichia coli O157:H7), invA gene (Salmonella enterica), inlA gene (Listeria monocytogenes) on the plastic substrates. PCR has been developed for amplification and labeling target genes of rfbE, invA, inlA with biotin. The biotinated target DNA is then captured onto the surface of plastic strips through specific DNA hybridization. The succeeding staining of biotinated DNA duplexes with avidin-horseradish peroxidise (AV-HRP) and biotinated anti-HRP antibody greatly amplifies the detectable signal through the multiple cycle signal amplification strategy, and thus realizing ultrasensitive and specific detection of the above three pathogens in food samples with the naked eyes. Results showed approximately 5 copies target pathogenic DNA could be detected with the naked eyes. This simple but very efficient colorimetric assay also show excellent anti-interference capability and good stability, and can be readily applied to point-of-care diagnosis. (C) 2015 Elsevier B.V. All rights reserved.
机译:在这项研究中,提出了一种新的方法,可以用肉眼对一组常见食源性病原体进行超灵敏检测和快速高通量鉴定。作为概念验证的应用,通过固定三种可以分别识别rfbE基因(大肠杆菌O157:H7),invA基因(肠炎沙门氏菌),inlA基因(单核细胞增生李斯特氏菌)的特异性polyT捕获探针来制造多病原体分析阵列。 )放在塑料基材上。已经开发出PCR,以用生物素扩增和标记rfbE,invA,inlA的靶基因。然后通过特异性DNA杂交将生物素化的目标DNA捕获到塑料条的表面上。通过抗生物素蛋白辣根过氧化物酶(AV-HRP)和生物素化抗HRP抗体对生物素化DNA双链体进行成功的染色,通过多周期信号放大策略极大地放大了可检测信号,从而实现了食品中上述三种病原体的超灵敏和特异性检测肉眼观察样品。结果表明,用肉眼可检测到约5份靶病原DNA。这种简单但非常有效的比色测定法还显示出出色的抗干扰能力和良好的稳定性,可轻松应用于即时诊断。 (C)2015 Elsevier B.V.保留所有权利。

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