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Controlling Data Quality and Reproducibility of a High-Sensitivity Immunoassay Using Isotachophoresis in a Microchip

机译:在芯片中使用等速电泳来控制高灵敏度免疫分析的数据质量和重现性

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This report describes a method of controlling the sensitivity and reproducibility of a microchip-based immunoassay by using isotachophoresis to preconcentrate the antigen and antibody prior to binding. Gel electrophoresis separation is coupled to the preconcentration step to separate the immunocomplex products formed. The system employs a quartz-based LabChip that automates the metering, preconcentration, reaction, separation, and detection. The system also uses a handoff mechanism that switches the immunocomplex from the stacking mode to the separation mode. We show that the handoff timing affects the data quality and repeatability of the electropherograms, and we demonstrate an automatic handoff mechanism to precisely control the signal intensity and separation of peaks of interest. In so doing, the automatic handoff mechanism also improves the reproducibility of the assay. When applied to the homogeneous liquid-phase detection of alpha-fetoprotein, a common tumor marker, the system shows a greater than 200-fold stacking of specific analytes of interest.
机译:该报告描述了一种通过使用等速电泳在结合前预浓缩抗原和抗体来控制基于微芯片的免疫测定的灵敏度和可重复性的方法。凝胶电泳分离与预浓缩步骤相连,以分离形成的免疫复合物产物。该系统采用基于石英的LabChip,可自动进行计量,预浓缩,反应,分离和检测。该系统还使用切换机制,将免疫复合物从堆叠模式切换到分离模式。我们展示了切换时间会影响电泳图的数据质量和可重复性,并且我们展示了一种自动切换机制,可精确控制信号强度和目标峰的分离。这样做,自动切换机制也提高了测定的可重复性。当应用于常见肿瘤标志物甲胎蛋白的均相液相检测时,该系统显示出感兴趣的特定分析物的堆积超过200倍。

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