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Fast immunoassay for microfluidic western blotting by direct deposition of reagents onto capture membrane

机译:通过直接沉积试剂将试剂直接沉积在捕获膜上的微流体蛋白质印迹快速免疫测定

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摘要

Western blotting is a widely used protein assay platform, but the technique requires long analysis times and multiple manual steps. Microfluidic systems are currently being explored for increased automation and reduction of analysis times, sample volumes, and reagent consumption for western blots. Previous work has demonstrated that proteins separated by microchip electrophoresis can be captured on membranes by dragging the microchip outlet across the membrane. This process reduces the separation and transfer time of a western blot to a few minutes. To further improve the speed and miniaturization of a complete western blot, a microscale immunoassay with direct deposition of immunoassay reagents has been developed. Flow deposition of antibodies is used to overcome diffusion limited binding kinetics so that the entire immunoassay can be completed in 1 h with detection sensitivity comparable to incubation steps requiring 20 h. The use of low microliter per min flow rates with antibody reagents applied directly and locally to the membrane where the target proteins have been captured, reduced antibody consumption similar to 30-fold. The complete western blot was applied to the detection of GAPDH and beta-tubulin from A431 cell lysate.
机译:Western Blotting是一种广泛使用的蛋白质测定平台,但该技术需要长分析时间和多个手动步骤。目前正在探索微流体系统,以增加自动化和减少西方印迹的分析时间,样本量和试剂消耗。以前的工作表明,通过将微芯片出口拖动在膜上,可以在膜上捕获通过微芯片电泳分离的蛋白质。该过程将Western印迹的分离和转移时间降低到几分钟内。为了进一步提高完全Western印迹的速度和小型化,已经开发了一种具有直接沉积免疫测定试剂的微米免疫测定。抗体的流量沉积用于克服扩散有限的结合动力学,使得整个免疫测定可以在1小时内完成,检测灵敏度与需要20小时的孵育步骤相当。使用低微升的每分钟流速与抗体试剂直接和局部施用于捕获靶蛋白的膜,降低抗体消耗与30倍。将完全的Western印迹应用于来自A431细胞裂解物的GAPDH和β-管蛋白的检测。

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