首页> 外文会议>Micro(MEMS) and Nanotechnologies for Defense and Security; Proceedings of SPIE-The International Society for Optical Engineering; vol.6556 >Microfluidic device detection of waterborne pathogens through static light scattering of latex immunoagglutination using proximity optical fibers
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Microfluidic device detection of waterborne pathogens through static light scattering of latex immunoagglutination using proximity optical fibers

机译:使用邻近光纤通过乳胶免疫凝集的静态光散射来检测水性病原体的微流控设备

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Microfluidic device detections of E. coli K12 in deionized (DI) water and E. coli in field water sample were demonstrated through static light scattering of latex immunoagglutination using proximity optical fibers. This method is a fully-automated, one-step detection, and requires neither sample pre-treatment nor cell culturing often required in many on-chip detections. We have used highly carboxylated polystyrene submicron latex particles without surfactants to enhance diffusional mixing and prevent non-specific bindings towards successful demonstration of latex immunoagglutination in microfluidic device. Detection of E. coli was performed by taking microscopic images from the view cell of a microfluidic device and counting the fractions of non-agglutinated and agglutinated particles. The limit of detection (LOD) was ca. 150 CFU ml~(-1) with this method for both E. coli K12 in DI water and E. coli in field water sample, indicating no non-specific bindings. Improved LOD of < 4.3 CFU ml~(-1) was achieved by measuring forward static light scattering from microfluidic device, using proximity optical fibers and a USB-powered miniature spectrometer. The total assay time for sample preparation (mostly dilutions) and on-chip assay (mostly injections and short incubation time) was < 10 min.
机译:通过使用邻近光纤的乳胶免疫凝集的静态光散射,证明了去离子(DI)水中的大肠杆菌K12和野外水样品中的大肠杆菌的微流体装置检测效果。该方法是全自动的一步式检测,不需要样品预处理,也不需要许多芯片检测中通常需要的细胞培养。我们已经使用了不含表面活性剂的高度羧化的聚苯乙烯亚微米胶乳颗粒,以增强扩散混合并防止非特异性结合,从而成功地证明了微流体装置中胶乳免疫凝集的成功。大肠杆菌的检测是通过从微流控设备的观察室拍摄显微图像并计数未凝集和凝集的颗粒的分数来进行的。检出限(LOD)为。用此方法对去离子水中的大肠杆菌K12和田间水样中的大肠杆菌均进行150 CFU ml〜(-1)处理,表明没有非特异性结合。通过使用邻近光纤和USB供电的微型光谱仪测量微流控设备的前向静态光散射,可以实现LOD <4.3 CFU ml〜(-1)的改进。样品制备(主要是稀释液)和芯片上分析(主要是进样和较短的孵育时间)的总分析时间少于10分钟。

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