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Lucifer Yellow as a Live Cell Fluorescent Probe for Imaging Water Transport in Subcellular Organelles

路西法黄 细胞器 生物物理学 化学 荧光 亚历山福禄 内体 磁导率 荧光显微镜 细胞内 生物化学 生物 量子力学 物理 缝隙连接
作者
Adriana María Chaurra Arboleda,Brittany M. Gutzman,Emily Taylor,P. Christine Ackroyd,Ken Christensen
出处
期刊:Applied Spectroscopy [SAGE]
卷期号:65 (1): 20-25 被引量:9
标识
DOI:10.1366/10-06095
摘要

While the water permeability of the plasma membranes of mammalian cells has been studied extensively, water transport across membranes of subcellular compartments (e.g., lysosomes, macropinosomes) has been difficult to study. Here we demonstrate a new method for measuring water flux in late endosomes and lysosomes of intact living cells using time-lapse fluorescence microscopy. Cells were loaded by fluid-phase uptake with a mixture of the Lucifer Yellow dextran (LY-dex), a D(2)O sensitive dye, and a D(2)O insensitive control dye, Alexa fluor 546 dextran (AF546-dex). LY-dex responded linearly to changes in D(2)O concentration and the LY-dex D(2)O sensitivity was not affected by changes in pH, physiological salt, and protein concentrations. The co-loaded control dye, AF546-dex, showed no signal changes as a function of D(2)O concentration. To measure membrane water flux, the LY-dex fluorescence in labeled organelles was recorded during rapid superfusion of cells with isotonic buffers prepared in D(2)O. The time constant of water exchange across the lysosomal membrane of intact cells was determined by fitting the data to a single exponential function. From these data, together with the measured area of the organelles, observed water permeability for intracellular CHO-K1 lysosomes was calculated to be 5.3 × 10(-3) ± 0.3 × 10(-3) cm/s. This work demonstrates the feasibility of measuring water flux into subcellular organelles in live cells using LY-dex.

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