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一种用于多重酶联免疫吸附测定的紧凑型微流控几何结构。

A compact microfluidic geometry for multiplexing enzyme-linked immunosorbent assays.

机构信息

Department of Chemistry, University of Wyoming, Laramie, Wyoming, USA.

出版信息

Electrophoresis. 2022 Jul;43(13-14):1399-1407. doi: 10.1002/elps.202100311. Epub 2022 Apr 26.

DOI:10.1002/elps.202100311
PMID:35355289
Abstract

We have previously reported a novel approach to implementing multiplex enzyme-linked immunosorbent assay (ELISA) in connected microchannels by exploiting the slow diffusion of the enzyme reaction product across the different assay segments. This work builds on that report by implementing the noted assay in segments arranged along the circumference of a circular channel layout to reduce the footprint size and sample volume requirement. Using the current design, a 5-plex cytokine ELISA was demonstrated in a 1.5 × 1.5-cm region, which corresponded to a reduction in the footprint area by about a factor of 3 compared to that reported in our previous study. Additionally, the selective coating of our assay segments with the target molecules was realized in this work using electroosmosis instead of hydrodynamic flow as was the case in the previous report. This aspect of our experimental design is particularly significant as it permits the use of cross-sectional channel dimensions significantly shorter than those employed in the current work. Moreover, the use of an electric field for coating purposes enables the integration of functionalities such as electrokinetic preconcentration of analyte molecules during the sample incubation period that can further enhance the capabilities of our assay method.

摘要

我们之前报道了一种在连通微通道中实现多重酶联免疫吸附测定(ELISA)的新方法,该方法利用酶反应产物在不同测定段之间的缓慢扩散。这项工作是在前一份报告的基础上进行的,即在圆形通道布局的圆周上布置了所述测定段,以减小足迹尺寸和样品体积需求。使用当前设计,在 1.5×1.5 平方厘米的区域内实现了 5 重细胞因子 ELISA,与我们之前的研究相比,足迹面积减小了约 3 倍。此外,与之前的报告不同,本工作使用电动渗透而不是流体动力学流动来实现我们的测定段与目标分子的选择性涂层。我们实验设计的这一方面非常重要,因为它允许使用比当前工作中使用的横截面通道尺寸短得多的通道尺寸。此外,电场的使用为涂层目的提供了便利,能够在样品孵育期间实现分析物分子的电动浓缩等功能,从而进一步增强我们的测定方法的能力。

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