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Program in Neuroscience, Department of Biological Sciences, Ohio University, Athens, Ohio 45701
In this study, Zn2+ transport in rat cortical neurons was characterized by successfully combining radioactive tracer experiments with spectrofluorometry and fluorescence microscopy. Cortical neurons showed a time-dependent and saturable transport of 65Zn2+ with an apparent affinity of 15-20 µM. 65Zn2+ transport was pH dependent and was decreased by extracellular acidification and increased by intracellular acidification. Compartmentalization of newly transported Zn2+ was assessed with the Zn2+-selective fluorescent dye zinquin. Resting cortical neurons showed uniform punctate labeling that was found in cell processes and the soma, suggesting extrasynaptic compartmentalization of Zn2+. Depletion of intracellular Zn2+ with the membrane-permeant chelator N,N,N',N'-tetrakis(2-pyridylmethyl)-ethylenediamine (TPEN) resulted in the complete loss of punctate zinquin labeling. After Zn2+ depletion, punctate zinquin labeling was rapidly restored when cells were placed in 30 µM Zn2+, pH 7.4. However, rapid restoration of punctate zinquin labeling was not observed when cells were placed in 30 µM Zn2+, pH 6.0. These data were confirmed in parallel 65Zn2+ transport experiments.
pH; zinquin; carboxyseminaphthorhodofluor-1 fluorescence; ion transport; transition elements; primary culture
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