Subunit-Dependent Modulation of Kainate Receptors by Extracellular Protons and Polyamines

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The Journal of Neuroscience, February 15, 2003, 23(4):1179

Subunit-Dependent Modulation of Kainate Receptors by Extracellular Protons and Polyamines
David D. Mott¹, Mark S. Washburn², Sunan Zhang¹, and Raymond J. Dingledine¹
¹ Department of Pharmacology, Emory University School of Medicine, Atlanta, Georgia 30322, and ² Merck Research Laboratories, San Diego, California 92121

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Synaptic activity causes significant fluctuations in proton concentrations in the brain. Changes in pH can affect neuronalexcitability by acting on ligand-gated channels, including thosegated by glutamate. We show here a subunit-dependent regulationof native and recombinant kainate receptors by physiologicallyrelevant proton concentrations. The effect of protons on kainatereceptors is voltage-independent and subunit dependent, with GluR5(Q),GluR6(Q), GluR6(R), and GluR6(R)/KA2 receptors being inhibitedand GluR6(R)/KA1 receptors beingpotentiated.
Mutation of two acidic residues (E396 and E397) to neutral amino acids significantly reduces the proton sensitivity of theGluR6(Q) receptor, suggesting that these residues influence protoninhibition. The endogenous polyamine spermine potentiated GluR6(R)kainate currents in a pH-dependent manner, producing an acidicshift in the IC₅₀ for proton inhibition. Spermine potentiationof GluR6(R) is voltage independent, does not affect receptor desensitization,and only slightly shifts the agonist affinity of the receptor.These results suggest that, similar to its action on NMDA receptors,spermine potentiates kainate receptors by relieving proton inhibitionof the receptor. Furthermore, they suggest that fluctuations inbrain pH during both normal and pathological processes could regulatesynaptic transmission and plasticity mediated by kainatereceptors.

Key words: polyamines; spermine; pH; kainate receptor; NMDA receptor; proton; epilepsy; neurodegeneration; GluR6

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Electrical activity in the brain results in significant pH shifts in neurons, glia, and the interstitial space. The magnitudeof pH fluctuations varies depending on the stimulus delivered,reaching several tenths of a pH unit during repetitive stimulation(Chessler and Kaila, 1992). During pathophysiological insults,such as spreading depression and ischemia, interstitial pH canfall to 6.5 and below for prolonged periods (Somjen, 1984; vonHanwehr et al., 1986). Many ligand-gated channels, including thosegated by glutamate, are sensitive to extracellular pH. Much attentionhas focused on the pH sensitivity of the NMDA class of glutamatereceptor (GluR) (Tang et al., 1990; Traynelis and Cull-Candy,1990). NMDA receptors that lack exon 5 and NR2C are half-maximallyinhibited by protons at approximately pH 7.3, suggesting thatactivity-dependent changes in interstitial pH could regulate theirfunction. In contrast, AMPA receptors are much less proton sensitive,with half-maximal inhibition at pH 6.1 (Lei et al., 2001). Thus,it seems likely that AMPA receptors would be inhibited by protonsonly during strong pathophysiological insults. Kainate receptorswere reported to be only weakly inhibited by protons (Tang etal., 1990; Traynelis and Cull-Candy, 1990). However, these earlystudies were hampered by the inability of investigators to separateresponses mediated by AMPA and kainate receptors. Only recently,with the development of more selective agonists and antagonists,as well as the use of recombinant receptor subunits, has it beenpossible to study kainate receptors inisolation.

The family of kainate receptors is composed of five different genes that code for the subunits GluR5, GluR6, GluR7, KA1, andKA2 (Chittajallu et al., 1999). These subunits can combine tocreate a variety of distinct kainate receptors that play differentfunctional roles. For example, in CA3 pyramidal cells of the hippocampus,GluR6-containing kainate receptors participate in synaptic transmissionat the mossy fiber-CA3 pyramidal cell synapse but not at commissuralsynapses (Castillo et al., 1997). In CA1 stratum radiatum interneurons,postsynaptic kainate receptors contain both GluR5 and GluR6 subunits;however, presynaptic kainate receptors that modulate synaptictransmission between these interneurons contain GluR6 but notGluR5 subunits (Mulle et al., 2000). KA1 and KA2 subunits appearto modify the pharmacological and physiological properties ofkainate receptors when coexpressed in heteromeric complexes (Herbet al., 1992; Swanson et al., 1998).

Given the highly specialized roles of different kainate receptors, it is important to understand whether receptor activationis modulated by endogenous agents in a subunit-dependent manner.In this study, we identified a prominent subunit-dependent regulationof recombinant kainate receptors by protons and polyamines. Protonsinhibit most tested kainate receptors but, surprisingly, potentiateGluR6/KA1 receptors. We focused on the mechanism by which protonsinhibit kainate receptors, finding strong similarity between theaction of protons on kainate and NMDA receptors. These resultssuggest that changes in interstitial pH may tonically regulatethe function of kainate receptors in a subunit-dependent manner.They also add another layer of complexity to our understandingof kainate receptor function in thebrain.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Primary hippocampal cell culture. Primary cultures of hippocampal neurons were prepared using a modified version of our methodfor preparing cortical cultures (Mott et al., 1998). Briefly,the hippocampi were dissected from the brains of embryonic day19 Sprague Dawley rat pups, dissociated by trituration, and suspendedin DMEM supplemented with L-glutamine (2 mM), penicillin (100U/ml)-streptomycin (100 µg/ml), and B27 supplement. Cells wereplated onto 12 mm glass coverslips precoated with poly-D-lysine(1 mg/ml, 12 hr exposure) and laminin (50 µg/ml, 1 hr exposure)and maintained at 37°C in a humidified 5% CO₂incubator.

Electrophysiological recording from primary hippocampal neurons. After 7-15 d in culture, a coverslip containing neurons wasplaced in the recording chamber and continually perfused withwarmed (30-32°C), bubbled (95% O₂-5% CO₂) artificial CSF (ACSF)at a rate of 2 ml/min. The ACSF contained the following (in mM):125 NaCl, 2.8 KCl, 25 NaHCO₃, 1.00 NaH₂PO₄, 2 CaCl₂, 1.5 MgSO₄,and 25 glucose at pH 7.3. Cells were observed with an uprightOlympus Optical (Melville, NY) BX50WI microscope equipped witha 40× water immersion differential interference contrast objectivecoupled to an infrared camera system (Hamamatsu, Tokyo, Japan).Neurons selected for recording were large and had a pyramidalappearance with two to three dendriticprocesses.

Recordings were made using conventional whole-cell voltage-clamp techniques (Mott et al., 2001) with a MultiClamp 700A amplifier(Axon Instruments, Union City, CA). Pipettes (resistance ~5 M $Omega$ )were filled with the following solution (in mM): 110 CsGluconate,20 CsCl, 4 NaCl, 10 HEPES, 0.5 CaCl₂, 5 BAPTA, 2 MgATP, and 0.3NaGTP, pH 7.3 (285-295 mOsm). Cells were held in voltage clampat $-$ 70 mV throughout the experiment. Data were filtered at 1 kHzand digitized at 2 kHz using a Digidata 1200 (Axon Instruments)analog-to-digital board. During the experiment, the flow rateof ACSF was increased by means of a peristaltic pump (Minipuls3; Gilson, Middleton, WI) to 10 ml/min to decrease solution exchangetime. Kainate receptor-mediated currents were isolated by applicationof a drug mixture containing antagonists of AMPA receptors (GYKI52466, 100 µM), NMDA receptors (D-APV, 100 µM), and GABA_A receptors(bicuculline methochloride, 100 µM). In the presence of this drugmixture, kainate receptor-mediated currents were evoked by bathapplication of domoate (100 µM) for 90 sec. Agonist was bath appliedin these experiments to allow tight control over the pH of thesolution. pH levels in the recording chamber were monitored bymeans of a miniature pH probe (LAZAR Research Laboratories, LosAngeles, CA) and did not drift by >0.05 pH units from the desiredpH over the course of the experiment. Domoate was chosen as theagonist because it is weakly desensitizing and could be used insupramaximal concentrations (100 µM) to speed the onset of thecurrent. To test the effect of protons on native kainate receptors,ACSF at pH 6.3 was used. This ACSF contained the following (inmM): 147.5 NaCl, 2.8 KCl, 2.5 NaHCO₃, 1.00 NaH₂PO₄, 2 CaCl₂, 1.5MgSO₄, and 25 glucose. Neurons were allowed to equilibrate tothe desired pH level for 30-60 sec or until a stable baselinehad been reached before domoate application. Series resistance,input resistance, and baseline holding current were monitoredthroughout the experiment. Neurons in which any of these parametersvaried by >10% werediscarded.

Oocyte preparation and injection. Xenopus oocytes were prepared and injected as described previously (Mott et al., 1998).Briefly, stage V-VI oocytes were isolated from anesthetized frogs,enzymatically treated by gentle shaking with collagenase (typeIV, 1.7 mg/ml for 45-120 min; Worthington, Freehold, NJ) in acalcium-free Barth's solution and then (in some cases) manuallydefolliculated. Cells were injected with up to 50 ng of mRNA transcribedfrom linearized constructs in the pGEM-HE, pSGEM, or Bluescript(Stratagene, La Jolla, CA) vector. For heteromeric receptors,mRNA was injected at a 10:1 ratio (GluR2/GluR3), a 1:6 ratio (GluR6/KA1and GluR6/KA2), or a 1:3 ratio (NR1/NR2). Injected oocytes weremaintained at 17°C in Barth's solution containing gentamycin (100µg/ml), penicillin (10 U/ml), and streptomycin (10 µg/ml) for3-10 d, after which two-electrode voltage-clamp recordings weremade at room temperature (23-25°C) from cells continually perfusedin a standard frog Ringer's solution. This solution containedthe following (in mM): 90 NaCl, 1 KCl, 15 HEPES, and 0.4 CaCl₂and 0.1 MgCl₂. Recording pipettes were filled with 3 M CsCl plus0.4 M EGTA, pH 7.5, to chelate Ca²⁺ and thereby minimize the activation of calcium-dependent chloridecurrents. GluR6/KA1 and GluR6/KA2 receptors were activated withAMPA (0.3-1 mM), whereas homomeric receptors were activated bydomoate (3 µM) or kainate (30 µM). To reduce desensitization whenkainate was used as the agonist, oocytes were pretreated withconcanavalin-A (0.3 mg/ml for 3 min) and then washed for at least10 min before use. NMDA receptors were activated using NMDA (100µM) and glycine (10 µM), and AMPA receptors were activated withkainate (300 µM). When NMDA receptors were studied, the MgCl₂in the Ringer's solution was replaced with 0.4 mM BaCl₂. Currentswere elicited from a holding potential of $-$ 70 mV except when specified.Current signals were digitized at 1 kHz using a Digidata 1200analog-to-digital board (Axon Instruments). Current-voltage (I-V)curves during steady-state current responses were generated usingvoltage ramps from $-$ 100 to +50 mV over a period of 1.3 sec. Rampcurrents were analyzed by subtracting the average of the leakcurrent before and after agonist application from the currentobtained in the presence of agonist. At least three ramps wererecorded and averaged for each condition in each oocyte. To studythe effect of pH, oocytes were perfused with Ringer's solutionat the desired pH for 30-60 sec or until a stable baseline hadbeen reached before subsequent agonist application. Applicationof each of the agonists produced a stable, rapidly rising andnondesensitizing or weakly desensitizing current in the majorityof oocytes. Oocytes in which the current was not stable or inwhich the baseline holding current drifted by >10% werediscarded.

Human embryonic kidney 293 cell culture and transfection. Human embryonic kidney 293 (HEK 293) cells (CRL 1573; American TypeCulture Collection, Manassas, VA) were cultured in DMEM containinghigh glucose (25 mM) and added L-glutamine (2 mM), sodium pyruvate(1 mM), penicillin (100 U/ml)-streptomycin (100 µg/ml), and 10%fetal bovine serum according to Mott et al. (2001). Cells weremaintained in 60 mm culture plates at 37°C in a humidified atmospherecontaining 5% CO₂, grown to ~80% confluency (usually ~48 hr afterplating), harvested enzymatically using 0.25% trypsin, and dissociatedfurther by gentle trituration. For maintenance, cells were thenreplated in 60 mm culture dishes at a ratio of 1:5 with growthmedia. For transfection, cells were plated at a density of 10⁶ cells/ml on 12 mm glass coverslips coated first with poly-D-lysine(2-12 hr exposure; 100 mg/ml) and then with fibronectin (2-12hr exposure; 20 mg/ml). After 24-48 hr, cells were transfectedby the method of calcium phosphate precipitation as describedpreviously (Mott et al., 2001) with 0.1-1 mg/ml GluR6(Q) in thecytomegalovirus-based mammalian expression vector JG3.6 or GluR6(R)in pcDNA1amp. Cotransfection with the reporter gene green fluorescentprotein (0.2-0.4 mg/ml) was used to identify individually transfectedcells.

Electrophysiological recording from HEK 293 cells. Transfected HEK 293 cells plated on a glass coverslips were transferredto a perfusion chamber on the stage of an inverted microscope(Diaphot; Nikon, Tokyo, Japan) and continually perfused at a rateof 0.5 ml/min with 23°C media containing the following (in mM):150 NaCl, 3 KCl, 10 HEPES, 1 CaCl₂, and 0.4 MgCl₂. Whole-cellrecordings of agonist-evoked membrane currents were performedunder voltage-clamp conditions (Mott et al., 2001) with electrodescontaining the following (in mM): 110 D-gluconic acid, 110 CsOH,30 CsCl, 4 NaCl, 5 HEPES, 5 BAPTA, 0.5 CaCl₂, 2 MgCl₂, 2 NaATP,and 0.3 NaGTP at pH 7.3 (osmolality was 290 mOsm). Recording electrodeswere made from borosilicate glass (inner diameter, 1.15; outerdiameter, 1.65) fire polished to resistance of 4-6 M $Omega$ . The membranepotential was held between $-$ 60 and $-$ 75 mV unless otherwise specified.Current recordings were amplified (Axopatch 200; Axon Instruments),filtered (1-3 kHz, $-$ 3 dB), and digitized at 3-13 kHz using a Digidata1200 analog-to-digital board. Tip potentials were measured aftereach patch experiment, and experiments with slow or multiphasicexchange time courses were excluded. For whole-cell recordings,cells were lifted off of the bottom of the dish to facilitatesolutionexchange.

Slow solution changes were performed by exchanging the total volume of the recording chamber. Rapid solution changes wereperformed with a piezoelectric-driven double-barreled perfusionsystem (model P-272.00; Physik Instrumente, Waldbronn, Germany)(Mott et al., 2001). The application pipette was pulled from thetaglass tubing (2 mm outer diameter, 0.3 mm wall thickness, 0.22mm septum; Hilgenberg, Malsfeld, Germany) and had a tip diameterof 200-300 µm, with the inner diameter of each barrel being 80-120µm. A solenoid valve typically controlled flow in each side ofthe theta tubing. Control solution flowed continuously throughone barrel, whereas the agonist solution flowed through the otherbarrel only during drug application. The agonist application barrelwas preflushed for 1-2 sec before piezo-driven application toclear diluted solution and moved by means of a piezoelectric devicecausing the recorded cell or membrane patch to be transientlyexposed to the agonist-containing solution. The time course ofsolution exchange across the laminar flow interface was estimatedat the end of each experiment by liquid junction potential measurementsand was found to possess a 20-80% rise time of 300-500 µsec. Thesolution flowing through the application pipette could be changedby means of a rotary valve connected to each barrel. Between solutionchanges, the agonist application barrel was flushed for 20-60sec to remove the previous solution. Unless otherwise stated,agonist was applied at intervals at which the receptors were shownto completely recover (4× mean tau; 99%) from desensitization(15 sec for glutamate and 45 sec for kainate). All experimentswere performed using 1-3 mM glutamate or 300 µM kainate, unlessotherwiseindicated.

Data analysis. Analysis was performed using pClamp (Axon Instruments), Origin (Microcal Software, Northampton, MA), and Prismsoftware (GraphPad Software, San Diego, CA) packages. Statisticalcomparisons were performed using the appropriate Student's t test.A two-way ANOVA with Bonferroni post hoc test to compare selectedmeans was performed for the analysis of the data presented inFigure 4D. Values are given as mean ±SE.

Materials. GluR6(Q) and GluR6(R) in pGEM-HE and the pSGEM vector were a generous gift from M. Mayer (National Institutes ofHealth, Bethesda, MD). GluR6(Q) in JG3.6 was generously providedby S. Heinemann (Salk Institute, San Diego, CA), as were GluR5,KA1 and KA2 plasmids. NR1 and NR2 were generously provided byS. Nakanishi (Kyoto University, Kyoto, Japan). Philanthotoxin-433(PhTx-433) was a generous gift from A. Mueller (NPS Pharmaceuticals,Salt Lake City, UT). Kainate, spermine, spermidine, GYKI 52466,and glycine were purchased from Sigma (St. Louis, MO). Domoate,AMPA, D-APV, bicuculline methochloride, and NMDA were purchasedfrom Tocris Cookson (St. Louis, MO). All tissue culture reagentswere obtained from Invitrogen (Gaithersburg, MD). Molecular biologyreagents, restriction enzymes, and fibronectin were purchasedfrom Promega (Madison, WI), Pharmacia (Piscataway, NJ), or BoehringerMannheim (Indianapolis,IN).

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Inhibition of native and recombinant kainate receptors by protons

Kainate receptors expressed in cultured hippocampal neurons can be activated in a weakly desensitizing manner by domoate (Lermaet al., 1993). We made use of this finding to test the protonsensitivity of native kainate receptors in cultured hippocampalneurons. Activation of pharmacologically isolated kainate receptorswith domoate (100 µM) at pH 7.3 and a holding potential of $-$ 70mV produced inward currents. Decreasing the pH to 6.3 significantlyreduced the amplitude of this current (Fig. 1A). Returning thepH to 7.3 rapidly restored the current amplitude. These data indicatethat protons inhibit native kainate receptors in cultured hippocampalneurons.

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Figure 1. Protons inhibit native and recombinant kainate receptors in a subunit-dependent manner. A, Pharmacologically isolated kainate currents from a cultured hippocampal neuron during application of domoate (100 µM) at pH 7.3, pH 6.3, and after wash at pH 7.3. The bar graph on the right compares the averaged effect of acidic pH on kainate receptor-mediated currents in cultured hippocampal neurons (n = 4; **p < 0.01). Responses were normalized relative to the initial control current at pH 7.3 (dotted line). B, Dose-response curves to protons for GluR6(Q) (filled circles; n = 7) and NR1a/NR2B NMDA receptors (open circles; n = 5-8 oocytes per pH level) expressed in oocytes. The pH levels at which proton inhibition of GluR6(Q) (IC₅₀ of pH 6.9 ± 0.03) and NR1a/NR2B receptors (IC₅₀ of pH 7.42 ± 0.06) were half-maximal were both within a biologically relevant range of proton concentrations (gray bar in this and subsequent figures). The dotted line indicates the extrapolated maximum current used for normalization (see Results). The inset shows sample recordings of domoate currents from GluR6(Q) receptors at different pH levels. The gray bars denote application of the indicated pH, whereas the black bars indicate domoate (3 µM) application. C, Dose-response curve to protons for GluR6(Q)/KA2 receptors expressed in oocytes. Protons inhibited this receptor in a biphasic manner with IC₅₀ values at pH 8.9 ± 0.8 (a) and 5.8 ± 0.1 (b; n = 11). The proton inhibition curve for GluR6(Q) is plotted for comparison. The dotted line indicates the extrapolated maximum current used for normalization (see Results). The inset shows sample currents from GluR6(Q)/KA2 receptors activated by AMPA at different pH levels. The gray bars denote application of the indicated pH, whereas the black bars indicate (s)-AMPA (300 µM) application. D, The bar graph compares the pH level necessary to produce half-maximal inhibition (IC₅₀) of each of the indicated kainate receptors expressed in oocytes. Because the proton inhibition curve for GluR6(Q)/KA2 is biphasic (C), both IC₅₀ values are indicated. The number of oocytes used for each receptor is as follows (oocytes per point on the proton inhibition curve): GluR5(Q), 8; GluR6(Q), 6-20; GluR6(R), 4-20; GluR6(Q)/KA2, 5-7. E, Comparison of the effect of protons on selected NMDA, kainate, and AMPA receptors expressed in oocytes. Current amplitudes at pH 6.8 are expressed as a percentage of the amplitude at pH 7.5 (dotted line). The number of oocytes used is as follows: NR1a/NR2A, 7; NR1a/NR2B, 6; NR1a/NR2C, 6; NR1a/NR2D, 5; GluR6(Q), 15; GluR6(R), 7; GluR5(Q), 8; GluR6(Q)/KA2, 10; GluR3, 11; GluR2/GluR3, 4.

To explore this finding in greater detail, we examined the effect of protons on recombinant kainate receptors. Steady-statedomoate-evoked (3 µM) currents in oocytes injected with the unedited(Q) variant of GluR6 were decreased when the pH was lowered andwere potentiated when the pH was raised above pH 7.5. Proton inhibitionof these currents was rapidly reversible during washout. A compositeinhibition curve describing the effect of protons on GluR6(Q)receptors was produced by recording the domoate current from eachoocyte over a pH range from 9.0 to 5.2 and then expressing thiscurrent as a percentage of the current at pH 7.5. The resultsfrom each oocyte were then normalized to the extrapolated maximumresponse in that oocyte, combined, and plotted in Figure 1B. TheIC₅₀ determined from the fitted curve for GluR6(Q) was approximatelypH 6.9 (~126 nM H⁺), whereas that for NR1a/NR2B receptors was approximately pH 7.4.These data indicate that, as with NMDA receptors, GluR6 receptorsare tonically inhibited by protons at pH 7.3.

It is unlikely that ionization of domoate contributed to the pH-dependent effects of this agonist. The three carboxylic acidsof domoic acid have p_Ka values of 2.1, 3.7, and 5.0, with theamino group in the pentameric ring having a p_Ka of 9.8. Thesevalues are all outside of the pH range tested in these experiments.Furthermore, a supramaximal concentration of domoate was usedin all experiments to minimize any potential effects of changesin the ionization of thisagonist.

Subunit dependence of proton inhibition

Kainate receptors of distinct subunit composition play different functional roles. Differential proton sensitivity of thesereceptors may provide a novel method of regulating kainate receptor-mediatedneurotransmission. Therefore, we examined the proton sensitivityof kainate receptors of different subunit composition. GluR5(Q)kainate receptors were inhibited by protons with an IC₅₀ of pH6.9 ± 0.04. This value was similar to that of GluR6(Q), suggestingthat GluR5 kainate receptors would also be tonically inhibitedby ambient proton concentrations. GluR5 and GluR6 subunits aresubject to RNA editing, which converts a single amino acid residuein the channel pore from a glutamine (Q) into an arginine (R)(Sommer et al., 1991). Editing at this Q/R site in GluR6 did notaffect proton inhibition [GluR6(R) IC₅₀ of 7.0 ± 0.04] (Fig. 1D).

We examined the proton sensitivity of a heteromeric kainate receptor by expressing the GluR6(Q) subunit in combination withKA2 subunits. GluR6(Q)/KA2 receptors were selectively activatedby bath application of (s)-AMPA (300 µM) (Herb et al., 1992).Protons inhibited current at these receptors, but the proton inhibitioncurve was biphasic, with IC₅₀ values at approximately pH 8.9 and5.8, respectively (Fig. 1C,D). When compared with GluR6(Q) receptors,GluR6(Q)/KA2 receptors were equally sensitive to low proton concentrations(pH $>=$ 7.5) and less sensitive to higher proton concentrations (pH<7.5). Interestingly, although the current at GluR6(Q)/KA2 receptorswas inhibited by ~25% between pH 7.5 and 6.8, the extent of protoninhibition did not significantly change as the pH was alteredover this range. It is unlikely that ionization of AMPA contributesto the pH-dependent effects of this agonist because the p_Ka valuesfor AMPA (p_Ka1 = 1.9; p_Ka2 = 5.1; and p_Ka3 = 10.1) fall outsideof the tested pHvalues.

The current amplitude at pH 6.8 as a percentage of the current at pH 7.5 gives a measure of proton inhibition over a biologicallyrelevant portion of the pH range. This type of comparison betweenkainate, NMDA, and AMPA receptors of selected subunit compositionreveals that homomeric kainate receptors (GluR5 and GluR6) haveintermediate proton sensitivity between that of NMDA and AMPAreceptors, with NR1a/NR2C NMDA receptors being less proton sensitivethan all tested kainate receptors except GluR6(Q)/KA2 (Fig. 1E).

Protons potentiate current at GluR6(Q)/KA1 receptors

In contrast to the strong inhibition produced by protons on homomeric or heteromeric GluR6(Q)/KA2-containing kainate receptors,protons potentiated kainate receptors containing GluR6(Q)/KA1subunits. Proton potentiation of current at these receptors becamestronger as proton concentrations were increased from 1 nM (pH9.0) up to 1 µM (pH 6.0). At proton concentrations above 1 µM(pH <6.0), potentiation of the kainate current was reversed (Fig.2A,B). Proton potentiation was rapidly reversible during washout.Protons potentiated GluR6(Q)/KA1 receptors with an EC₅₀ of pH7.1 ± 0.03, indicating that these receptors were more sensitiveto protons than other tested kainate receptors. In two of theeight oocytes tested, the current was also slightly potentiatedat very alkaline pH values (Fig. 2A), suggesting that protonsmay act at more than one site on these receptors.

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Figure 2. Protons potentiate kainate current at GluR6/KA1 receptors. A, GluR6(Q)/KA1 currents activated by (s)-AMPA (300 µM) in oocytes at different pH levels. Note the increased current amplitude at pH 6.0. Also in this oocyte note the atypical increase in current at pH 9.0. B, Dose-response curve to protons at GluR6(Q)/KA1 receptors expressed in oocytes (n = 8). The dotted line indicates the current amplitude at pH 9.0 used for normalization. The proton inhibition curve for GluR6(Q) is indicated for comparison (dashed line).

Whereas the mechanism of proton inhibition of kainate receptors is unknown, proton inhibition of NMDA receptors has been wellcharacterized. Protons inhibit NMDA receptors by binding to anallosteric site on the extracellular face of the receptor anddecreasing the single-channel opening frequency (Traynelis andCull-Candy, 1990). Protons do not alter the rate or extent ofNMDA receptor desensitization nor do they alter agonist affinityat the receptor (Tang et al., 1990; Traynelis and Cull-Candy,1990, 1991). Proton inhibition of NMDA receptors is voltage independentand does not involve a shift in the reversal potential of thecurrent. Finally, polyamines potentiate current at NR1a/NR2B NMDAreceptors primarily by relieving proton inhibition (Trayneliset al., 1995). Using NMDA receptors as a model, we examined themechanism of proton inhibition of kainate receptors. We focusedour attention on GluR6 kainatereceptors.

Protons do not alter GluR6 receptor desensitization kinetics

Protons do not alter desensitization of NMDA receptors (Traynelis and Cull-Candy, 1991). In contrast, protons inhibit AMPAreceptors by enhancing receptor desensitization (Ihle and Patneau,2000; Lei et al., 2001). We examined the effect of protons onthe desensitization kinetics of GluR6(Q) kainate receptors expressedin HEK 293 cells to determine whether the mechanism of protoninhibition of kainate receptors was similar to that of NMDA orAMPA receptors. Rapid application of a supramaximal concentrationof glutamate (3 mM, pH 7.3) produced a strongly desensitizingresponse in whole-cell recordings of GluR6(Q) currents in thesecells. The rapid monophasic rise of the current ( $tau$ _rise = 720 ±80 µsec) and the sharp current peak suggest that GluR6 receptorsare activated synchronously. At pH 7.3, desensitization of thecurrent was well fitted by a single exponential component, with $tau$ _desens = 6.4 ± 0.3 msec and a peak/steady-state current ratioof 410 ± 30 (n = 8). Alkaline pH (pH 8.5) increased, whereas acidicpH (pH 6.0) decreased peak current amplitude. However, neitheralkaline nor acidic pH altered GluR6(Q) current kinetics, as canbe seen when the current traces are scaled and superimposed (Fig.3A). Closer examination of desensitization kinetics of GluR6(Q)revealed that alkaline pH did not significantly alter $tau$ _desensor the peak/steady-state current ratio (Fig. 3B,C). These datasuggest that, similar to NMDA receptors, proton inhibition ofGluR6 kainate receptors is not caused by changes in the extentor rate of onset of desensitization.

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Figure 3. Protons do not alter desensitization kinetics or voltage dependence of GluR6 kainate receptors. A, The GluR6(Q) current produced by rapid application of glutamate (3 mM) to HEK 293 cells held at $-$ 70 mV was potentiated by 60% at alkaline pH (pH 8.5) in one cell and inhibited by 85% at acidic pH (pH 6.0) in another cell. The lack of change in response kinetics at altered pH can be seen when the currents are scaled and superimposed. The graph on the right shows the amplitude of the GluR6(Q) current in response to rapid application of glutamate during the course of one experiment as the pH was increased to 8.5 and then returned to 7.3. On average, pH 8.5 caused a 15 ± 5% (p < 0.05; n = 5) increase in GluR6(Q) current amplitude. B, Superimposition of GluR6(Q) currents in response to rapid application of glutamate at pH 7.3 and 8.5. Monoexponential fits of the current decay demonstrate that, despite the increased current amplitude, the desensitization kinetics of the current did not change. C, Top, Desensitization of GluR6(Q) currents was almost complete. Steady-state current amplitudes were determined from monoexponential fits of current decay and averaged only ~0.24% of peak amplitude (n = 4). Alkaline pH (pH 8.5) produced a small but nonsignificant decrease in steady-state/peak current ratio. Bottom, The time constant of current decay ( $tau$ _decay) did not change as the pH was increased from pH 7.3 to 8.5 (n = 4). D, In oocytes, the domoate (3 mM) current at GluR6(R) receptors at three different pH levels was outwardly rectifying during voltage ramps from $-$ 100 to +50 mV as evident in these sample traces (dotted lines). The slope of the linear portion of the I-V curve, calculated by regression analysis, is shown (thick lines).

Proton inhibition of kainate receptors is voltage insensitive

The voltage sensitivity of proton inhibition of kainate receptors was examined to determine whether protons inhibit thesereceptors by acting at a site within the transmembrane electricfield. Domoate currents at pH 6.0, 7.5, and 9.0 were recordedfrom GluR6(R)-injected oocytes as the holding potential was rampedfrom $-$ 100 to +50 mV. Domoate currents reversed close to 0 mV atall pH levels tested (pH 9, I_REV $-$ 2 ± 8 mV; pH 7.5, I_REV $-$ 2 ±8 mV; pH 6.0, I_REV $-$ 1 ± 8 mV; n = 4) and were approximately linearlydependent on voltage over the range from $-$ 80 to $-$ 20 mV. The slopeof this region of the current-voltage curve was dependent on pHin a manner quantitatively similar to that of steady-state currentsin these same oocytes. The average slope increased by 70 ± 40%when the pH was raised to pH 9.0 and decreased by 40 ± 18% whenthe pH was lowered to pH 6.0 (Fig. 3D), whereas the steady-statecurrent at $-$ 70 mV increased by 60 ± 17% at pH 9.0 and decreasedby 50 ± 4% at pH 6.0 (n = 4). Finally, the lack of an increasein outward rectification of the current at pH 6.0 [rectificationratio-100/50 (RR_-100/50), 1.2 ± 0.1, pH 7.5; 1.3 ± 0.1, pH 6.0;n = 4] suggested that proton inhibition of GluR6(R) kainate receptorsis voltageinsensitive.

Mutations in GluR6(Q) reduce proton inhibition

Site-directed mutagenesis has identified a number of acidic amino acid residues on the NR1 NMDA receptor subunit that arecritical for proton inhibition of that receptor (Williams et al.,1995; Masuko et al., 1999). Two residues of particular interestare glutamate 342 and aspartate 343. These neighboring residuesare located in the N terminus of the NR1 subunit in the regionconnecting the two lobes of the LIVBP-like domain. Sequence alignmentof NR1a, NR2A-NR2D with GluR5-GluR7 reveals that, in seven ofeight subunits, E342 is conserved, whereas the neighboring residueat position 343 is acidic (either aspartate or glutamate, differingonly in NR2C) (alignments adapted from those of Armstrong et al.,1998; Paoletti et al., 2000; Perin-Dureau et al., 2002). In GluR6,these amino acids correspond to residues E396 and E397. To determinewhether similar residues in kainate and NMDA receptors are importantfor proton inhibition, we examined the effect of mutation of eachof these residues as well as three nearby unconserved acidic residues(D388, D390, and E400) on proton inhibition of GluR6(Q) receptors(Fig. 4A). In all cases, aspartate was mutated to asparagine andglutamate to glutamine. Proton inhibition curves were constructedas described previously for each of the mutant receptors. Mutationof the three unconserved residues (D388N, D390N, and E400Q) hadno effect on proton inhibition in GluR6. In contrast, mutationof the two conserved residues caused a significant decrease inproton sensitivity of GluR6(Q) (Fig. 4B-D). Of the two mutations,E396Q caused a greater decrease in the IC₅₀ for proton inhibition(5.6-fold) than did E397Q (2.8-fold). Despite their reduced protoninhibition, mutant GluR6 receptors showed no evidence for potentiation,suggesting that proton potentiation of GluR6/KA1 receptors wasunique to the KA1 subunit and not a property of the GluR6 subunitthat was masked by the stronger proton inhibition.

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Figure 4. Mutation of two critical acidic residues, E396 and E397, in GluR6(Q) reduces proton sensitivity of the receptor. A, Sequence alignment of a portion of the LIVBP-like domain in the NR1 subunit with the analogous portion of the GluR6 subunit. Amino acids in the NR1 subunit reported to alter either proton inhibition or spermine potentiation are indicated (filled circles) as are residues in the GluR6 subunit that were mutated in this study (open circles). Only mutations at E396 and E397 (asterisks) reduced proton inhibition of GluR6(Q). A proposed schematic diagram of the GluR6 subunit, based on the structure of the NR1 subunit, is shown on the right, indicating the position of the LIVBP-like domain in the N terminus and the locations of residues E396 and E397 in this domain. B, Sample recordings of steady-state domoate (3 mM) currents evoked at three different pH levels in an oocyte expressing wild-type GluR6(Q) receptors or mutant GluR6(Q) receptors in which residue 396 has been mutated from glutamate to glutamine (E396Q). Note the reduced effect of protons on the mutated receptor. C, Dose-response curve for protons at wild-type (filled circles; n = 7) and mutant E396Q (open circles; n = 10) GluR6(Q) receptors. D, The graph shows the half-maximal concentration of protons (IC₅₀) necessary to inhibit wild-type and five mutant GluR6(Q) receptors expressed in oocytes. Only mutations at E396 and E397 significantly reduced proton inhibition (**p < 0.01). The number of oocytes used is shown in parentheses. E, Proton inhibition curve for mutant GluR6Q(E396Q)/KA2 receptors expressed in oocytes (left). Protons inhibited this receptor in a biphasic manner, with IC₅₀ values at pH 9.0 ± 0.4 (a) and 5.4 ± 0.1 (b; n = 7, n = 6-14 oocytes per point). The proton inhibition curve for wild-type GluR6(Q)/KA2 receptors has been overlaid for comparison. Note the increased prominence of the first component (a) of proton inhibition in the mutant receptor. The IC₅₀ values for proton inhibition of mutant and wild-type GluR6(Q)/KA2 receptors are compared in the bar graph (right). The GluR6Q(E396Q) mutation significantly reduced the affinity of only the second component (b) of proton inhibition.

Expression of the mutant GluR6Q(E396Q) subunit with the KA2 subunit allowed examination of the effect of this mutation onthe heteromeric GluR6(Q)/KA2 receptor. The mutant GluR6Q(E396Q)/KA2receptor was inhibited by protons in a biphasic manner, with IC₅₀values at pH 9.0 ± 0.4 and 5.4 ± 0.1 (Fig. 4E). The IC₅₀ for thefirst component of inhibition was similar to that of the wild-typereceptor, whereas that for the second component of inhibitionwas significantly reduced (*p < 0.05). Although the IC₅₀ valuefor the first component of inhibition was unchanged, this componentwas much more prominent in the proton inhibition curve of themutant receptor. Thus, these receptors were significantly moreinhibited at pH 6.8-7.5 than were wild-typereceptors.

Polyamines potentiate GluR6(R) and inhibit GluR6(Q) current

Small endogenous polyamines, such as spermine, potentiate current through recombinant NMDA receptors. Traynelis et al. (1995)reported that spermine potentiates NMDA responses primarily byrelieving tonic proton block of these receptors present at physiologicalpH levels. A minor role may also be played by the small polyamine-inducedchanges in receptor desensitization that have been reported previously(Lerma, 1992; Rumbaugh et al., 2000). If the mechanism of protoninhibition of NMDA and kainate receptors is similar, then polyaminesmay potentiate GluR6 kainate receptors in a comparable manner.Therefore, to further compare proton inhibition of kainate andNMDA receptors, we tested the effect of polyamines on kainatecurrent through GluR6receptors.

The effect of polyamines on the GluR6 receptor-mediated current was dependent on the editing state of the Q/R site on thereceptor (Fig. 5A). Spermine (1 mM) markedly facilitated the steady-statecurrent at edited GluR6(R) receptors at pH 7.5. Potentiation byspermine was reversible and concentration dependent, with an EC₅₀of 282 µM [95% confidence interval (C.I.), 191-416 µM; n = 7].This potentiation was mimicked by the polyamine spermidine (1mM; 151 ± 2.5% of control; n = 3) but not by the polyamine arthropodtoxin PhTx-433 (1 µM; 92 ± 6.0%; n = 4). These findings suggestsimilarity in the action of spermine on NMDA and kainate receptors.

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Figure 5. Spermine potentiates GluR6(R) and inhibits GluR6(Q) kainate receptors. A, Sample currents at pH 7.5 from oocytes show potentiation by 1 mM spermine at GluR6(R) receptors and inhibition by the same concentration of spermine at GluR6(Q) receptors. The graph on the right shows the dose-response curve for spermine potentiation at GluR6(R) receptors and spermine inhibition at GluR6(Q) receptors. The amplitude of the control current in the absence of spermine is indicated (dotted line). Currents were evoked by 30 µM kainate. B, At pH 7.3, currents evoked by rapid application of 3 mM glutamate to HEK 293 cells expressing GluR6(R) receptors were potentiated by 1 mM spermine, whereas currents at GluR6(Q) receptors were inhibited. The graph on the right shows that, relative to control (dotted line), spermine produced a significant potentiation of GluR6(R) current (n = 6; *p < 0.05) and a significant inhibition of GluR6(Q) current (n = 5; **p < 0.01) at pH 7.3.

In contrast to GluR6(R) receptors, the unedited (Q) form of the receptor was strongly inhibited by extracellular polyaminesat pH 7.5 (Bähring et al., 1997). Spermine (1 mM) and spermidine(1 mM) reversibly inhibited kainate currents through GluR6(Q)receptors to 14 ± 4% (n = 13) and 72 ± 3% (n = 5) of control,respectively. Inhibition by spermine was reversible and concentrationdependent (IC₅₀ of 66 µM; 95% C.I., 25-171 µM; n = 7) (Fig. 5A).In contrast to its lack of effect on GluR6(R) receptors, PhTx-433reduced domoate currents at GluR6(Q) receptors to 13 ± 3% of control(n = 5). The time course for block and recovery of GluR6(Q) receptorsby polyamines and polyamine toxins was similar to that reportedfor GluR2-lacking AMPA receptors (Washburn and Dingledine, 1996).

Polyamines had similar effects on GluR6 receptors expressed in mammalian cells. We examined the effect of spermine (1 mM)on currents evoked by rapid application of glutamate to HEK 293cells transfected with either GluR6(R) or GluR6(Q) receptors.In cells held at $-$ 70 mV at pH 7.3, spermine produced a significantpotentiation of the current at GluR6(R) receptors and a significantinhibition of current at GluR6(Q) receptors (Fig. 5B). These effectswere reversible during washout ofspermine.

Polyamines potentiate NMDA receptors primarily by hindering protonation of residues critical for proton inhibition. Similarityin the mechanism underlying polyamine potentiation of NMDA andGluR6(R) kainate receptors would suggest additional structuralparallels in the regions of the two receptors responsible forproton inhibition. We therefore examined the mechanism of polyaminepotentiation ofGluR6(R).

Spermine potentiation is voltage insensitive

Spermine potentiation of NMDA receptors is voltage insensitive, suggesting that spermine acts at a site outside the transmembraneelectric field (Williams, 1994). To determine whether sperminepotentiation of kainate receptors shares similar voltage independence,we examined the effect of spermine on glutamate currents overa range of membrane potentials from $-$ 100 to +100 mV. Glutamate-evokedGluR6(R) currents in the absence and presence of spermine wereexamined in HEK 293 cells at pH 6.0, a pH level at which spermineproduces a strong potentiation (Fig. 6A,B). GluR6(R) currentsoutwardly rectified (RR_-100/60, 1.3 ± 0.2) and reversed at $-$ 3.5± 1.7 mV (n = 6). Spermine markedly potentiated responses at allmembrane potentials but did not alter the reversal potential ( $-$ 5.9± 1.1 mV) or rectification of the current (RR_-100/60, 1.4 ± 0.2;n = 6). For each experiment, the I-V curve in spermine was normalizedto that in control, and the resulting curves were combined toyield an averaged plot of the voltage dependence of spermine potentiation(Fig. 6C). The slope of these averaged curves was not significantlydifferent from zero, indicating the lack of any voltage dependenceof spermine potentiation.

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Figure 6. Spermine potentiation of GluR6(R) receptors is voltage independent, does not affect agonist potency, and does not alter receptor desensitization. A, Current responses (I) recorded at pH 6.0 from GluR6(R) receptors expressed in an HEK 293 cell in response to rapid application of glutamate as the holding potential (V) was stepped from $-$ 100 to +100 mV. B, The graph shows the I-V curve for GluR6(R) receptors in the absence and presence of spermine in the same cell as in A. The slope of the linear portion of the I-V curve increases in spermine by an amount (65%) similar to the increase in the peak current (58%) at $-$ 60 mV. C, The amplitude of the GluR6(R) current in the presence of 1 mM spermine and in wash was expressed as a fraction of the control current at each holding potential. When the data were fit by linear regression, the slopes of the resulting curves (0, 0.0006, and 0.0002 mV/fraction control current for control, spermine, and wash, respectively; n = 5) did not differ from zero, indicating voltage independence. D, The graph shows the dose-response curve for kainate on GluR6(Q) receptors expressed in oocytes in the absence (filled circles) and presence (open circles) of 1 mM spermine at pH 7.5. The dotted line indicates the amplitude of the maximal kainate response in the absence of spermine. E, Currents (superimposed in the absence and presence of spermine) at GluR6(R) receptors expressed in HEK 293 cells in response to rapid application of 3 mM glutamate showed strong potentiation by 1 mM spermine at pH 6.0. Monoexponential fits of the current decay revealed little effect of spermine on the onset rate of desensitization. F, Spermine did not affect either the steady-state/peak current ratio (top; n = 6) or the desensitization time constant ( $tau$ _decay; bottom; n = 6) of the GluR6(R) current in HEK 293 cells.

Spermine does not alter the agonist potency for GluR6(R)

Spermine may potentiate GluR6(R) current by enhancing the agonist potency for the receptor. To test this possibility, we examinedthe effect of spermine (1 mM) on the EC₅₀ for kainate activationof GluR6(R). Concentration-response curves to kainate in the absenceand presence of spermine revealed a substantial increase in themaximal kainate response in the presence of spermine but no significantdifference in the EC₅₀ for kainate (control, EC₅₀ of 0.7 µM; 95%C.I., 0.6-0.8 µM; n = 6; spermine, EC₅₀ of 0.5 µM; 95% C.I., 0.3-0.8µM; n = 6) (Fig. 6D). Therefore, we conclude that spermine doesnot potentiate the receptor by enhancing agonistpotency.

Spermine does not potentiate kainate responses by altering receptor desensitization

A spermine-induced decrease in either the rate or extent of receptor desensitization could also contribute to the potentiation.To test this possibility, we examined desensitization of GluR6(R)receptors expressed in HEK 293 cells. Whole-cell currents producedby rapid application of a supramaximal concentration of glutamate(3 mM) were examined at pH 6.0 in the presence and absence of1 mM spermine. In the continual presence of agonist, GluR6(R)currents desensitized rapidly and monoexponentially ( $tau$ _desens =6.5 ± 0.4 msec; n = 6) (Fig. 6E). Desensitization was virtuallycomplete, with the steady-state current representing only ~0.6%of the peak current. Spermine potentiated the peak current (Fig.5B) but had no effect on the onset rate of desensitization orthe steady-state to peak current ratio (Fig. 6E,F). Desensitizationof the receptor in the presence of spermine was monoexponential,with $tau$ _desens (6.4 ± 0.5 msec; n = 6) similar to that observedin the absence of spermine. These data indicate that sperminedoes not potentiate GluR6(R) by altering desensitization of thereceptor.

Potentiation by spermine is pH dependent

To determine whether spermine potentiates GluR6(R) by relieving proton inhibition, we examined spermine potentiation overa range of pH values. Potentiation produced by spermine was greatestat acidic pH levels when proton inhibition of the domoate currentwas strongest (Fig. 7A). This potentiation became progressivelysmaller at more basic pH levels as proton inhibition weakened.Similarly, at GluR6(R) receptors in HEK 293 cells, the currentinduced by rapid application of glutamate was more strongly potentiatedby spermine at pH 6.0 than at pH 7.5 (Fig. 7B). It is unlikelythat ionization of spermine can account for this pH-dependentpotentiation because the p_Ka4 value for spermine (p_Ka4 = 8.3)falls outside of the range over which spermine has its maximaleffects. These data indicate the strong pH dependence of sperminepotentiation.

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Figure 7. Spermine potentiates GluR6(R) receptors by relieving proton inhibition. A, Sample traces (top) showing potentiation of domoate currents by 1 mM spermine at GluR6(R) receptors in an oocyte as the pH was increased to 9.0 and decreased to 6.0. Note that the amount of potentiation increased at more acidic pH levels. The graph on the bottom shows the averaged effect of spermine on GluR6(R) (n = 8-30 oocytes per point) and GluR6(Q) (n = 6-17 oocytes per point) receptors over a range of pH values. Data are expressed relative to the current amplitude in the absence of spermine (dotted line). B, Potentiation of GluR6(R) current by 1 mM spermine at pH 7.3 (top; n = 6) and pH 6.0 (bottom; n = 10). Currents were evoked by rapid application of 3 mM glutamate onto GluR6(R) receptors expressed in HEK 293 cells. Note that spermine produced a greater potentiation of the glutamate current at pH 6.0 than at pH 7.3. C, Dose-response curve for protons at GluR6(R) receptors in oocytes in the absence (filled circles) and presence (open circles) of 1 mM spermine (n = 4-20 oocytes per point). Spermine caused a strong rightward shift in the proton IC₅₀ at the receptor, indicating that the polyamine potentiated these receptors by reducing proton inhibition. D, Dose-response curve for protons at GluR6(Q) receptors in the absence (filled circles) and presence (open circles) of 1 mM spermine (n = 7). Note that spermine shifted the curve only at acidic pH levels. In C and D, currents were evoked by 3 µM domoate.

To further determine whether spermine relieved proton inhibition of GluR6(R), we examined the effect of spermine on the IC₅₀for proton inhibition of the GluR6(R) receptor expressed in oocytes(Fig. 7C). Spermine (1 mM) produced a 22-fold acidic shift inthe IC₅₀ for proton inhibition of the receptor (control, IC₅₀of pH 6.9 ± 0.03, n = 5-20; spermine, IC₅₀ of pH 5.6 ± 0.06, n= 4-18), shifting the proton sensitivity of the receptor out ofthe physiological range. These results suggest that, as with NMDAreceptors, spermine potentiation of GluR6(R) is primarily causedby a relief of proton inhibition of thereceptor.

At GluR6(Q) spermine consistently inhibited domoate currents at all but the most acidic pH levels (Fig. 7A). However, at pH6.0, spermine inhibition was reduced, and, in two of six oocytes,spermine potentiation was observed. Consequently, spermine shiftedthe proton inhibition curve for GluR6(Q) only at the most acidiclevels, having no effect at more alkaline pH values (Fig. 7D).These results are consistent with the interpretation that boththe edited (R) and unedited (Q) variants of the GluR6 receptorare potentiated by spermine in a pH-sensitive manner. However,in GluR6(Q) receptors, the potentiation is masked by a coexistentspermine-induced inhibition at all but the most acidic pH levels.The incomplete editing of GluR6 kainate receptors in the rat brain(Chittajallu et al., 1999) and the opposing effects of polyamineson these editing states suggests that kainate receptors can beexpressed with a high degree of specialization to meet the specificneeds of their synapticmicroenvironment.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The principal finding of the present study is that kainate receptors, like NMDA receptors, are tonically regulated by protonsat ambient pH (pH 7.3), and the extent and direction of this modulationis dependent on the subunit composition of the receptor. For example,we found that homomeric GluR6 receptors and heteromeric GluR6(Q)/KA2receptors are ~20-25% inhibited at resting pH (pH 7.3), whereasheteromeric GluR6/KA1 receptors are ~30% facilitated. Tonic regulationof kainate receptors by protons is important because it suggeststhat both the alkaline and acid shifts in interstitial pH thataccompany neuronal activity could modulate kainate receptor function.In addition, we found that the endogenous polyamine spermine potentiatesthe GluR6 kainate receptor primarily by relieving this protoninhibition. Given the specialized roles of kainate receptors ofdifferent subunit composition (Castillo et al., 1997; Mulle etal., 2000), our results suggest that these endogenous modulatoryagents may differentially regulate distinct kainate receptorsand thereby exert selective influence over discrete aspects ofkainate neurotransmission. These modulatory sites may also providenovel sites for the development of context-dependent and region-selectiveneuroprotective agents (Mott et al., 1998).

The mechanism underlying the differential effect of protons on distinct kainate receptors is unknown. Swanson et al. (2002)reported that each subunit in a heteromeric kainate receptor contributesan independent agonist-activated conductance to the overall channelresponse. According to this suggestion, activation or inhibitionof individual subunits would shift the conductance state of thechannel in a manner similar to that of AMPA receptors (Rosenmundet al., 1998). The biphasic nature of the proton inhibition curvefor GluR6/KA2 and the proton potentiation observed for GluR6/KA1suggest the possibility that protons can act with different affinitieson individual subunits in heteromeric kainate receptors. The biphasicproton inhibition curve for GluR6/KA2 may therefore representselective and independent inhibition of first the higher-affinityKA2 subunit, which reduces the channel conductance, followed byinhibition of the lower-affinity GluR6 subunit, which inhibitsthe receptor altogether. In support of this idea, we found thatreplacement of the GluR6 subunit in the heteromeric GluR6/KA2receptor with a mutated GluR6 subunit [GluR6Q(E396Q)] with loweredproton sensitivity altered the IC₅₀ of the low-affinity, but notthe high-affinity, component of the biphasic proton inhibitioncurve. Although this model represents the most straightforwardinterpretation of our results, we realize that other more complexscenarios can beimagined.

Although protons may alter kainate receptor gating by inhibiting individual subunits within the receptor, it appears thatthe proton sensitivity and possibly even the degree of protonationof the individual subunits is influenced by their interactionwith other subunits in the receptor. This idea is supported bytwo findings. First, neither of the two proton IC₅₀ values ofthe GluR6/KA2 receptor match the IC₅₀ of homomeric GluR6. Second,replacement of wild-type GluR6 with mutant GluR6 in the GluR6/KA2receptor significantly increases the prominence of the first componentof inhibition. Subunit interaction may therefore contribute tothe overall proton sensitivity of the receptor and influence thetonic level of proton inhibition at ambient pH. Additional experimentswill be necessary to explore thesepossibilities.

The mechanism by which protons inhibit kainate receptors appears to be similar to that by which protons inhibit NMDA receptors(Traynelis and Cull-Candy, 1991). This conclusion is strengthenedby four observations. First, as with NMDA receptors, proton inhibitionof kainate receptors is voltage independent, supporting the conclusionthat protons do not inhibit kainate receptors by acting at a sitewithin the receptor channel. Second, similar to their effect onNMDA receptors, protons do not alter the desensitization kineticsof kainate receptors. In contrast, protons inhibit AMPA receptorsby enhancing desensitization of the receptor (Ihle and Patneau,2000; Lei et al., 2001). Third, mutations of conserved residuesin GluR6 that reduce proton sensitivity of NMDA receptors alsoreduce proton sensitivity of kainate receptors. This finding suggeststhat similar structural elements on both kainate and NMDA receptorsmediate proton inhibition. Finally, as with NMDA receptors (Trayneliset al., 1995), spermine potentiated the current through GluR6receptors by producing an acidic shift in the p_Ka of the protonsensor. This caused the receptor to become less sensitive to protons.Spermine potentiation of GluR6(R) was voltage independent, didnot affect the onset or extent of current desensitization, anddid not affect the agonist potency for the receptor. These resultssuggest that spermine potentiates kainate receptors primarilyby relieving proton inhibition of the receptor. They also provideadditional confirmation of the similarity in the mechanism ofaction of protons on kainate and NMDAreceptors.

Our results suggest that protons inhibit kainate receptors by acting at a site on the receptor that is outside of the channelpore. Presumably, this site consists of an ionizable residue(s)at which protonation stabilizes the protein in a nonconductingstate. It seems likely that this site resides on the extracellularface of the receptor, possibly in the LIVBP-like domain, as hasbeen suggested for the proton sensor on NMDA receptors (Masukoet al., 1999). Indeed, residues that are critical for proton inhibition(E396 and E397) of GluR6 kainate receptors are located betweenthe two lobes of the LIVBP-like domain in GluR6. This is the samelocation at which the analogous residues (E342 and D343) are foundin the NMDA receptor (Masuko et al., 1999). Spermine is thoughtto relieve proton inhibition of NMDA receptors by binding to asite in the LIVBP-like domain of these receptors near the protonsensor (Masuko et al., 1999). The similarity in the action ofspermine on kainate and NMDA receptors is consistent with thepossibility that this polyamine could bind to a similar site inthe LIVBP-like domain of kainate receptors. Thus, the LIVBP-likedomain could act as a common structural element in kainate andNMDA receptors mediating the effects of protons and polyamines.This hypothesis of a modular architecture of ionotropic GluR subunitsis consistent with the suggestions of Paoletti and coworkers (Paolettiet al., 2000; Perin-Dureau et al., 2002). However, it is importantto note that the GluR6 mutations studied here, although criticalfor proton inhibition, may not reflect the true location of theproton sensor. Therefore, although it seems unlikely, we cannotexclude the possibility that protons act on a region on the intracellularface of the kainate receptor or a portion of the plasma membranethat is intimately associated with the receptor. Additional studieswill be necessary to address thesequestions.

Kainate receptors of distinct subunit combinations play different functional roles in the brain (Mulle et al., 2000). Potentiationor block of different kainate receptors by protons suggests thatproton regulation would be an important factor shaping kainateneurotransmission in the CNS. For example, changes in kainatereceptor subunit composition at a synapse during development (Bahnet al., 1994) or after a pathophysiological insult (Mathern etal., 1998) could have marked effects on the proton regulationof kainate neurotransmission at that synapse. Alternately, changesin extracellular pH that occur under physiological conditionsmay have implications for kainate receptor function. Proton levelsin the brain are not stable and fluctuate rapidly in both theacid and alkaline direction during neuronal activity (Chesslerand Kaila, 1992). Because of the selective localization and functionof different kainate receptors, pH changes could have distincteffects on different aspects of kainateneurotransmission.

Whereas pH fluctuates during synaptic transmission, the amplitude of this change is much greater during pathophysiologicalinsults, such as spreading depression, seizures, and ischemia,during which interstitial pH can fall to 6.5 and below for prolongedperiods (Somjen, 1984; von Hanwehr et al., 1986). This large decreasein interstitial pH has been shown to be neuroprotective by inhibitingthe activity of NMDA receptors (Kaku et al., 1993). Our resultssuggest that most kainate receptors would also be inhibited bythese large decreases in pH and that, during certain conditions,such as global ischemia (Sheardown et al., 1990), proton inhibitionof kainate receptors may provide some measure of neuroprotection.In particular, our results suggest that protons would be effectiveat inhibiting steady-state current produced by glutamate spilloveronto extrasynaptic kainate receptors. In contrast, GluR6/KA1 receptorsare potentiated by protons. Both GluR6 and KA1 subunit are highlyexpressed in CA3 pyramidal cells (Bahn et al., 1994). Perhapsoveractivation of these GluR6/KA1 receptors at acidic pH levelscontributes to the selective vulnerability of this cellpopulation.

  FOOTNOTES

Received Aug. 6, 2002; revised Dec. 3, 2002; accepted Dec. 6, 2002.

This work was supported by the Epilepsy Foundation (D.D.M.), National Alliance for Research on Schizophrenia and Depression(D.D.M.), University Research Council of Emory University (D.D.M.),National Institute of Neurological Disorders and Stroke (R.J.D.),and Bristol Myers Squibb (R.J.D.). We thank N. Ciliax and J. Petersfor excellent technicalassistance.

Correspondence should be addressed to Dr. David D. Mott, Department of Pharmacology, Rollins Research Center, Room 5010, 1510Clifton Road, Emory University School of Medicine, Atlanta, GA30322. E-mail: dmott{at}pharm.emory.edu.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

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