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Droplet-based microfluidics platform for measurement of rapid erythrocyte water transport

机译:基于液滴的微流控平台用于快速测量红细胞的水传输

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摘要

Cell membrane water permeability is an important determinant of epithelial fluid secretion, tissue swelling, angiogenesis, tumor spread and other biological processes. Cellular water channels, the aquaporins, are important drug targets. Water permeability is generally measured from the kinetics of cell volume change in response to an osmotic gradient. Here, we developed a microfluidics platform in which cells expressing a cytoplasmic, volume-sensing fluorescent dye are rapidly subjected to an osmotic gradient by solution mixing inside a ~ 0.1 nL droplet surrounded by oil. Solution mixing time was < 10 ms. Osmotic water permeability was deduced from a single, time-integrated fluorescence image of an observation area in which time after mixing is determined by spatial position. Water permeability was accurately measured in aquaporin-expressing erythrocytes with half-times for osmotic equilibration down to < 50 ms. Compared with conventional water permeability measurements using costly stopped-flow instrumentation, the microfluidics platform here utilizes sub-microliter blood sample volume, does not suffer from mixing artifact, and replaces challenging kinetic measurements by a single image capture using a standard laboratory fluorescence microscope.
机译:细胞膜透水性是上皮液分泌,组织肿胀,血管生成,肿瘤扩散和其他生物学过程的重要决定因素。细胞水通道,水通道蛋白,是重要的药物靶标。一般根据响应于渗透梯度的细胞体积变化的动力学来测量水渗透性。在这里,我们开发了一种微流控平台,其中表达细胞质,体积敏感的荧光染料的细胞通过在溶液周围混合的〜0.1 nL小滴内迅速混合,进行渗透梯度渗透。溶液混合时间<10 ms。从观察区域的单个时间积分荧光图像推导渗透水渗透率,其中混合后的时间由空间位置确定。在表达水通道蛋白的红细胞中,渗透时间精确到一半(小于50毫秒),可精确测量其水渗透性。与使用昂贵的停流仪器进行的常规透水性测量相比,此处的微流体平台利用了亚微升的血液样本量,不会出现混合伪影,并通过使用标准实验室荧光显微镜的单次图像捕获来替代具有挑战性的动力学测量。

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