๐”– Bobbio Scriptorium
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Flux measurement in single cells by fluorescence microphotolysis

โœ Scribed by R. Peters


Book ID
104684308
Publisher
Springer
Year
1984
Tongue
English
Weight
833 KB
Volume
11
Category
Article
ISSN
1432-1017

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โœฆ Synopsis


Fluorescence microphotolysis--widely employed for diffusion studies--can be used to measure transfer (flux) of fluorescent solutes through membranes in single cells and organelles. This article analyses the methodological basis of flux measurements, provides experimental tests, and discusses potential applications. The principle of the method is to equilibrate cells, organelles or vesicles with a fluorescent solute, to deplete the interior of individual cells etc. of fluorescein by the pulse of a high-intensity microbeam, and to monitor influx of solute by microfluorometry. Simple equations are given and a computer curve fitting program is described by which rate constants of influx and membrane permeability coefficients can be derived from fluorescence measurements. The permeability of individual "leaky" human erythrocyte ghosts to fluorescein-isothiocyanate-labelled bovine serum albumin has been measured under various conditions. Multiple exposure to the high-intensity microbeam had no effect on permeability within experimental error. Flux measurements have been also performed on individual vesicles of 1-2 micron radius which had been derived from ghosts. The potential application of the method to sub-lightmicroscopic vesicles and to organelles within living cells is discussed.


๐Ÿ“œ SIMILAR VOLUMES


Single-cell flux measurement by continuo
โœ M. Scholz; K. Schulten; R. Peters ๐Ÿ“‚ Article ๐Ÿ“… 1985 ๐Ÿ› Springer ๐ŸŒ English โš– 679 KB

Continuous fluorescence microphotolysis (CFM) was adapted to flux measurements in single cells. The principle of the method is simple: Cells are equilibrated with a fluorescent solute, an individual cell is continuously irradiated by a laser beam focussed down to approximately the diameter of the ce