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通过干涉测量法测量上皮细胞层中的细胞体积和质膜渗透水通透性。

Cell volume and plasma membrane osmotic water permeability in epithelial cell layers measured by interferometry.

作者信息

Farinas J, Verkman A S

机构信息

Department of Medicine, University of California, San Francisco 94143-0521, USA.

出版信息

Biophys J. 1996 Dec;71(6):3511-22. doi: 10.1016/S0006-3495(96)79546-2.

Abstract

The development of strategies to measure plasma membrane osmotic water permeability (Pf) in epithelial cells has been motivated by the identification of a family of molecular water channels. A general approach utilizing interferometry to measure cell shape and volume was developed and applied to measure Pf in cell layers. The method is based on the cell volume dependence of optical path length (OPL) for a light beam passing through the cell. The small changes in OPL were measured by interferometry. A mathematical model was developed to relate the interference signal to cell volume changes for cells of arbitrary shape and size. To validate the model, a Mach-Zehnder interference microscope was used to image OPL in an Madin Darby Canine Kidney (MDCK) cell layer and to reconstruct the three-dimensional cell shape (OPL resolution < lambda/25). As predicted by the model, a doubling of cell volume resulted in a change in OPL that was proportional to the difference in refractive indices between water and the extracellular medium. The time course of relative cell volume in response to an osmotic gradient was computed from serial interference images. To measure cell volume without microscopy and image analysis, a Mach-Zehnder interferometer was constructed in which one of two interfering laser beams passed through a flow chamber containing the cell layer. The interference signal in response to an osmotic gradient was analyzed to quantify the time course of relative cell volume. The calculated MDCK cell plasma membrane Pf of 6.1 x 10(-4) cm/s at 24 degrees C agreed with that obtained by interference microscopy and by a total internal reflection fluorescence method. Interferometry was also applied to measure the apical plasma membrane water permeability of intact toad urinary bladder; Pf increased fivefold after forskolin stimulation to 0.04 cm/s at 23 degrees C. These results establish and validate the application of interferometry to quantify cell volume and osmotic water permeability in cell layers.

摘要

由于发现了一个分子水通道家族,人们开始致力于开发测量上皮细胞质膜渗透水通透性(Pf)的策略。一种利用干涉测量法测量细胞形状和体积的通用方法被开发出来,并应用于测量细胞层中的Pf。该方法基于穿过细胞的光束的光程长度(OPL)对细胞体积的依赖性。通过干涉测量法测量OPL的微小变化。开发了一个数学模型,将干涉信号与任意形状和大小的细胞的细胞体积变化联系起来。为了验证该模型,使用马赫-曾德尔干涉显微镜对Madin Darby犬肾(MDCK)细胞层中的OPL进行成像,并重建三维细胞形状(OPL分辨率<λ/25)。正如模型所预测的,细胞体积加倍导致OPL的变化与水和细胞外介质之间的折射率差异成正比。根据连续干涉图像计算出响应渗透梯度时相对细胞体积的时间进程。为了在不使用显微镜和图像分析的情况下测量细胞体积,构建了一个马赫-曾德尔干涉仪,其中两束干涉激光中的一束穿过包含细胞层的流动室。分析响应渗透梯度的干涉信号,以量化相对细胞体积的时间进程。在24℃下计算得到的MDCK细胞质膜Pf为6.1×10^(-4) cm/s,与通过干涉显微镜和全内反射荧光法获得的结果一致。干涉测量法还被应用于测量完整蟾蜍膀胱顶端质膜的水通透性;在23℃下,福斯可林刺激后Pf增加了五倍,达到0.04 cm/s。这些结果确立并验证了干涉测量法在量化细胞层中细胞体积和渗透水通透性方面的应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9625/1233838/cd03a2a2989c/biophysj00042-0602-a.jpg

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