Cell volume measured by total internal reflection microfluorimetry: application to water and solute transport in cells transfected with water channel homologs

Cell volume measured by total internal reflection microfluorimetry: application to water and solute transport in cells transfected with water channel homologs

Total internal reflection (TIR) microfluorimetry was established as a method to measure continuously the volume of adherent cells and applied to measure membrane permeabilities in cells transfected with water channel homologs. Cytosol was labeled with the membrane-impermeant fluorophore calcein. Flu...

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Veröffentlicht in:Biophysical journal 1995-04, Vol.68 (4), p.1613-1620
Hauptverfasser: Farinas, J., Simanek, V., Verkman, A.S.
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Antiporters - genetics
Antiporters - metabolism
Aquaporin 1
Aquaporins
Biological Transport, Active
Biophysical Phenomena
Biophysics
Cell Line
Cell Membrane Permeability
Cell Size
Fluorometry - methods
Ion Channels - genetics
Ion Channels - metabolism
LLC-PK1 Cells
Models, Biological
Osmolar Concentration
Spodoptera
Swine
Transfection
Water - metabolism
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container_title Biophysical journal
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creator Farinas, J.
Simanek, V.
Verkman, A.S.
description Total internal reflection (TIR) microfluorimetry was established as a method to measure continuously the volume of adherent cells and applied to measure membrane permeabilities in cells transfected with water channel homologs. Cytosol was labeled with the membrane-impermeant fluorophore calcein. Fluorescence was excited by the TIR evanescent field in a thin section of cytosol (approximately 150 nm) adjacent to the cell-substrate interface. Because cytosolic fluorophore number per cell remains constant, the TIR fluorescence signal should be inversely related to cell volume. For small volume changes in Sf-9 and LLC-PK1 cells, relative TIR fluorescence was nearly equal to inverse relative cell volume; deviations from the ideal were modeled theoretically. To measure plasma membrane osmotic water permeability, Pf, the time course of osmotically induced cell volume change was inferred from the TIR fluorescence signal. LLC-PK1 cells expressing the CHIP28 water channel had an HgCl2-sensitive, threefold increase in Pf compared to nontransfected cells (Pf = 0.0043 cm/s at 10 degrees C). Solute permeability was measured from the TIR fluorescence time course in response to solute gradients. Glycerol permeability in Sf-9 cells expressing the water channel homolog GLIP was (1.3 +/- 0.2) x 10(-5) cm/s (22 degrees C), greater than that of (0.36 +/- 0.04) x 10(-5) cm/s (n = 4, p < 0.05) for control cells, indicating functional expression of GLIP. Water and urea permeabilities were similar in GLIP-expressing and control cells. The TIR method should be applicable to the study of water and solute permeabilities and cell volume regulation in cells of arbitrary shape and size.
doi_str_mv 10.1016/S0006-3495(95)80335-8
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1542-0086
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subjects Animals
Antiporters - genetics
Antiporters - metabolism
Aquaporin 1
Aquaporins
Biological Transport, Active
Biophysical Phenomena
Biophysics
Cell Line
Cell Membrane Permeability
Cell Size
Fluorometry - methods
Ion Channels - genetics
Ion Channels - metabolism
LLC-PK1 Cells
Models, Biological
Osmolar Concentration
Spodoptera
Swine
Transfection
Water - metabolism
title Cell volume measured by total internal reflection microfluorimetry: application to water and solute transport in cells transfected with water channel homologs
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