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Microfluidics platform for single-shot dose-response analysis of chloride channel-modulating compounds

机译:微流控平台用于氯离子通道调节化合物的单次剂量响应分析

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摘要

We previously developed cell-based kinetics assays of chloride channel modulators utilizing genetically encoded yellow fluorescent proteins. Fluorescence platereader-based high-throughput screens yielded small-molecule activators and inhibitors of the cAMP-activated chloride channel CFTR and calcium-activated chloride channels, including TMEM16A. Here, we report a microfluidics platform for single-shot determination of concentration-activity relations in which a 1.5 × 1.5 mm square area of adherent cultured cells is exposed for 5–10 min to a pseudo-logarithmic gradient of test compound generated by iterative, two-component channel mixing. Cell fluorescence is imaged following perfusion with an iodide-containing solution to give iodide influx rate at each location in the image field, thus quantifying modulator effects over a wide range of concentrations in a single measurement. IC50 determined for CFTR and TMEM16A activators and inhibitors by single-shot microfluidics were in agreement with conventional plate reader measurements. The microfluidics approach developed here may accelerate the discovery and characterization of chloride channel-targeted drugs.
机译:我们以前利用遗传编码的黄色荧光蛋白开发了基于氯离子通道调节剂的基于细胞的动力学测定方法。基于荧光读板器的高通量筛选产生了小分子活化剂和cAMP活化氯通道CFTR和钙活化氯通道(包括TMEM16A)的抑制剂。在这里,我们报告了一种用于浓度-活性关系的单次测定的微流控平台,其中一个1.5×1.5 mm见方的贴壁培养细胞在5-10分钟内暴露于由迭代产生的测试化合物的拟对数梯度,两组分通道混合。在用含碘化物的溶液灌注后,对细胞荧光进行成像,以在图像场中的每个位置提供碘化物的流入速率,从而可以在单次测量中在很宽的浓度范围内量化调节剂的作用。通过单次微流控技术确定的CFTR和TMEM16A激活剂和抑制剂的IC50与常规酶标仪的测量结果一致。此处开发的微流控方法可能会加快针对氯离子通道的药物的发现和表征。

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