Mutating a Conserved Proline Residue within the Trimerization Domain Modifies Na+ Binding to Excitatory Amino Acid Transporters and Associated Conformational Changes |
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| Authors: | Jasmin Hotzy Nicole Schneider Peter Kovermann Christoph Fahlke |
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| Affiliation: | From the ‡Institut für Neurophysiologie, Medizinische Hochschule Hannover, 30625 Hannover Germany.;the §Institute of Complex Systems, Zelluläre Biophysik (ICS-4), Forschungszentrum Jülich, 52428 Jülich, Germany, and ;the ¶Zentrum für Systemische Neurowissenschaften Hannover, 30559 Hannover, Germany |
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| Abstract: | Excitatory amino acid transporters (EAATs) are crucial for glutamate homeostasis in the mammalian central nervous system. They are not only secondary active glutamate transporters but also function as anion channels, and different EAATs vary considerably in glutamate transport rates and associated anion current amplitudes. A naturally occurring mutation, which was identified in a patient with episodic ataxia type 6 and that predicts the substitution of a highly conserved proline at position 290 by arginine (P290R), was recently shown to reduce glutamate uptake and to increase anion conduction by hEAAT1. We here used voltage clamp fluorometry to define how the homologous P259R mutation modifies the functional properties of hEAAT3. P259R inverts the voltage dependence, changes the sodium dependence, and alters the time dependence of hEAAT3 fluorescence signals. Kinetic analysis of fluorescence signals indicate that P259R decelerates a conformational change associated with sodium binding to the glutamate-free mutant transporters. This alteration in the glutamate uptake cycle accounts for the experimentally observed changes in glutamate transport and anion conduction by P259R hEAAT3. |
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| Keywords: | Anion Transport Ataxia Glutamate Neurological Diseases Neurotransmitter Transport Voltage Clamp Fluorometry |
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