Cooperation of the Conserved Aspartate 439 and Bound Amino Acid Substrate Is Important for High-Affinity Na+ Binding to the Glutamate Transporter EAAC1

doi:10.1085/jgp.200609678

Published online March 26, 2007
doi:10.1085/jgp.200609678
The Journal of General Physiology, Vol. 129, No. 4, 331-344
The Rockefeller University Press, 0022-1295 $30.00
© 2007 Tao et al.

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ARTICLE

Cooperation of the Conserved Aspartate 439 and Bound Amino Acid Substrate Is Important for High-Affinity Na⁺ Binding to the Glutamate Transporter EAAC1

Zhen Tao and Christof Grewer

University of Miami School of Medicine, Miami, FL 33136

Correspondence to Christof Grewer: cgrewer{at}med.miami.edu

The neuronal glutamate transporter EAAC1 contains several conservedacidic amino acids in its transmembrane domain, which are possiblyimportant in catalyzing transport and/or binding of co/countertransportedcations. Here, we have studied the effects of neutralizationby site-directed mutagenesis of three of these amino acid sidechains, glutamate 373, aspartate 439, and aspartate 454, onthe functional properties of the transporter. Transport wasanalyzed by whole-cell current recording from EAAC1-expressingmammalian cells after applying jumps in voltage, substrate,or cation concentration. Neutralization mutations in positions373 and 454, although eliminating steady-state glutamate transport,have little effect on the kinetics and thermodynamics of Na⁺and glutamate binding, suggesting that these two positions donot constitute the sites of Na⁺ and glutamate association withEAAC1. In contrast, the D439N mutation resulted in an approximately10-fold decrease of apparent affinity of the glutamate-boundtransporter form for Na⁺, and an $~$ 2,000-fold reduction in therate of Na⁺ binding, whereas the kinetics and thermodynamicsof Na⁺ binding to the glutamate-free transporter were almostunchanged compared to EAAC1_WT. Furthermore, the D439N mutationconverted L-glutamate, THA, and PDC, which are activating substratesfor the wild-type anion conductance, but not L-aspartate, intotransient inhibitors of the EAAC1_D439 anion conductance. Activationof the anion conductance by L-glutamate was biphasic, allowingus to directly analyze binding of two of the three cotransportedNa⁺ ions as a function of time and [Na⁺]. The data can be explainedwith a model in which the D439N mutation results in a dramaticslowing of Na⁺ binding and a reduced affinity of the substrate-boundEAAC1 for Na⁺. We propose that the bound substrate controlsthe rate and the extent of Na⁺ interaction with the transporter,depending on the amino acid side chain in position 439.

Abbreviations used in this paper: EAAC1, excitatory amino acidcarrier 1; EAAT, excitatory amino acid transporter; HEK, humanembryonic kidney; PDC, L-trans-2,4-pyrrolidine dicarboxcylicacid; RL, reentrant loop; TBOA, DL-threo-ß-benzyloxyaspartate;THA, D,L-threo-ß-hydroxyaspartic acid; TM, transmembranedomain.

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