Inhibition by K+ of Na+‐Dependent D‐Aspartate Uptake into Brain Membrane Saccules
- 1 September 1986
- journal article
- research article
- Published by Wiley in Journal of Neurochemistry
- Vol. 47 (3) , 825-830
- https://doi.org/10.1111/j.1471-4159.1986.tb00685.x
Abstract
Na+‐dependent uptake of dicarboxylic amino acids in membrane saccules, due to exchange diffusion and independent of ion gradients, was highly sensitive to inhibition by K+. The IC50 was 1–2 mM under a variety of conditions (i.e., whole tissue or synaptic membranes, frozen/thawed or fresh, D‐[3H]aspartate (10–1000 nM) or L‐[3H]glutamate (100 nM), phosphate or Tris buffer, NaCl or Na acetate, presence or absence of Ca2+ and Mg2+). The degree of inhibition by K+ was also not affected on removal of ion gradients by ionophores, or by extensive washing with H2O and reloading of membrane saccules with glutamate and incubation medium in the presence or absence of K+ (3 mM, i.e., IC70). Rb+, NH4+, and, to a lesser degree Cs+, but not Li+, could substitute for K+. [K+] showed a competitive relationship to [Na+]2. Incubation with K+ before or after uptake suggested that the ion acts in part by allowing net efflux, thus reducing the internal pool of amino acid against which D‐[3H]aspartate exchanges, and in part by inhibiting the interaction of Na+ and D‐[3H]aspartate with the transporter. The current model of the Na+‐dependent high‐affinity acidic amino acid transport carrier allows the observations to be explained and reconciled with previous seemingly conflicting reports on stimulation of acidic amino acid uptake by low concentrations of K+. The findings correct the interpretation of recent reports on a K+‐induced inhibition of Na+‐dependent “binding” of glutamate and aspartate, and partly elucidate the mechanism of action.Keywords
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