Transport direction determines the kinetics of substrate transport by the glutamate transporter EAAC1

Zhang, Zhou; Tao, Zhen; Gameiro, Armanda; Barcelona, Stephanie; Braams, Simona; Rauen, Thomas; Grewer, Christof

doi:10.1073/pnas.0704570104

Cited by 64 publications

(84 citation statements)

References 24 publications

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“…Because the mutants are locked in an exchange mode, we cannot experimentally test this alternative. This is because one or more sodium ions can bind before substrate on the extracellular side (33,34), and all three sodium ions unbind after the substrate on the intracellular side (35). Therefore many labeled substrate molecules can be exchanged for intracellular unlabeled substrate molecules without any accompanying sodium translocation.…”

Section: Discussionmentioning

confidence: 99%

The equivalent of a thallium binding residue from an archeal homolog controls cation interactions in brain glutamate transporters

Teichman

Kanner

2009

Proc. Natl. Acad. Sci. U.S.A.

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Glutamate transporters maintain low synaptic concentrations of neurotransmitter by coupling uptake to flux of other ions. Their transport cycle consists of two separate translocation steps, namely cotransport of glutamic acid with three Na ؉ followed by countertransport of K ؉ . Two Tl ؉ binding sites, presumed to serve as sodium sites, were observed in the crystal structure of a related archeal homolog and the side chain of a conserved aspartate residue contributed to one of these sites. We have mutated the corresponding residue of the eukaryotic glutamate transporters GLT-1 and EAAC1 to asparagine, serine, and cysteine. Remarkably, these mutants exhibited significant sodium-dependent radioactive acidic amino acid uptake when expressed in HeLa cells. Reconstitution experiments revealed that net uptake by the mutants in K ؉ -loaded liposomes was impaired. However, with Na ؉ and unlabeled L-aspartate inside the liposomes, exchange levels were around 50 -90% of those by wild-type. In further contrast to wild-type, where either substrate or K ؉ stimulated the anion conductance by the transporter, substrate but not K ؉ modulated the anion conductance of the mutants expressed in oocytes. Both with wild-type EAAC1 and EAAC1-D455N, not only sodium but also lithium could support radioactive acidic amino acid uptake. In contrast, with D455S and D455C, radioactive uptake was only observed in the presence of sodium. Thus the conserved aspartate is required for transporter-cation interactions in each of the two separate translocation steps and likely participates in an overlapping sodium and potassium binding site.cation binding site ͉ obligate exchange mutant ͉ sodium selectivity G lutamate transporters are key elements in the termination of the synaptic actions of the neurotransmitter and keep its synaptic concentrations below neurotoxic levels. Glutamate transport is an electrogenic process (1, 2) consisting of two sequential translocation steps: (i) Cotransport of the neurotransmitter with three sodium ions and a proton (3, 4) and (ii) the countertransport of one potassium ion (5-7). The mechanism involving two half-cycles (Fig. 1A) is supported by the fact that mutants impaired in the interaction with potassium are ''locked'' in an obligatory exchange mode (7,8). Glutamate transporters mediate two distinct types of substrate-induced steady-state current: An inward-rectifying or ''coupled'' current, reflecting electrogenic sodium-coupled glutamate translocation, and an ''uncoupled'' sodium-dependent current, which is carried by chloride ions and further activated by substrates of the transporter (9-11). Nontransportable substrate analogs, expected to ''lock'' the transporter in an outward-facing conformation (stippled part of Fig. 1 A), are not only competitive inhibitors of the two types of substrate-induced current, but also inhibit the basal sodium-dependent anion conductance (12,13).Recently a high-resolution crystal structure of a glutamate transporter homolog, Glt Ph , from the archeon Pyrococcus horikoshii was pu...

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Section: Discussionmentioning

confidence: 99%

The equivalent of a thallium binding residue from an archeal homolog controls cation interactions in brain glutamate transporters

Teichman

Kanner

2009

Proc. Natl. Acad. Sci. U.S.A.

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“…TBOA does not bind to EAAC1 in the absence of Na ϩ and may bind, but only weakly, in the presence of extracellular K ϩ . Therefore, TBOA binding was promoted by including a small amount of Na ϩ (2 mM in the presence of extracellular K ϩ and 5 mM in the presence of extracellular NMG ϩ ) in the TBOA-containing solution, as described previously (22). This small amount of Na ϩ did not elicit nonspecific currents.…”

Section: Methodsmentioning

confidence: 99%

“…Under these ionic conditions, 200 M TBOA is a supersaturating concentration (about 100-fold K m ), so the TBOA binding site should be saturated at all voltages. The K m for TBOA under these conditions has been experimentally determined previously (22).…”

Section: Methodsmentioning

confidence: 99%

Charge Compensation Mechanism of a Na+-coupled, Secondary Active Glutamate Transporter

Grewer

Zhang

Mwaura

et al. 2012

Journal of Biological Chemistry

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“…ϩ Binding Suggested by Kinetic Modeling-Coupled glutamate transport can be modeled as binding/unbinding transitions between distinct states (32,43). EAAT-associated anion channel properties are included in these models by connecting several states of the transport cycle with open conformations of the EAAT-associated anion channel (Fig.…”

Section: C-terminal Modulation Of Kmentioning

confidence: 99%

Regulation of Glial Glutamate Transporters by C-terminal Domains

Leinenweber

Machtens

Begemann

et al. 2011

Journal of Biological Chemistry

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Excitatory amino acid transporter 2 (EAAT2) is a high affinity glutamate transporter predominantly expressed in astroglia. Human EAAT2 encompasses eight transmembrane domains and a 74-amino acid C-terminal domain that resides in the cytoplasm. We examined the role of this region by studying various C-terminal truncations and mutations using heterologous expression in mammalian cells, whole-cell patch clamp recording and confocal imaging. Removal of the complete C terminus (K498X EAAT2) results in loss of function because of intracellular retention of truncated proteins in the cytoplasm. However, a short stretch of amino acids (E500X EAAT2) within the C terminus results in correctly processed transporters. E500X reduced glutamate transport currents by 90%. Moreover, the voltage and substrate dependence of E500X EAAT2 anion currents was significantly altered. WT and mutant EAAT2 anion channels are modified by external Na ؉ in the presence as well as in the absence of L-glutamate. Whereas Na

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Transport direction determines the kinetics of substrate transport by the glutamate transporter EAAC1

Cited by 64 publications

References 24 publications

The equivalent of a thallium binding residue from an archeal homolog controls cation interactions in brain glutamate transporters

The equivalent of a thallium binding residue from an archeal homolog controls cation interactions in brain glutamate transporters

Charge Compensation Mechanism of a Na+-coupled, Secondary Active Glutamate Transporter

Regulation of Glial Glutamate Transporters by C-terminal Domains

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