Glycine Site Antagonists and Partial Agonists Inhibit N-Methyl-D-aspartate Receptor-Mediated [3H]Arachidonic Acid Release in Cerebellar Granule Cells

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Vol. 285, Issue 2, 527-532, May 1998

Glycine Site Antagonists and Partial Agonists Inhibit N-Methyl-D-aspartate Receptor-Mediated [³H]Arachidonic Acid Release in Cerebellar Granule Cells¹

E. Viu² , A. Zapata³ , J. L. Capdevila, L. H. Fossom, P. Skolnick and R. Trullas

Unitat de Neurobiologia, Department of Bioanalítica Mèdica, Institut d'Investigacions Biomèdiques de Barcelona, Consejo Superior de Investigaciones Científicas, Barcelona, Spain (E.V., A.Z., J.L.C., R.T.), and Laboratory of Neuroscience, National Institute for Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, Maryland (L.H.F., P.S.)

	Abstract

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Activation of N-methyl-D-aspartate (NMDA) receptors is known to produce arachidonic acid release, which has been implicatedin excitotoxicity. Antagonists and partial agonists at the glycinesite of the NMDA receptor, despite exhibiting functional differencesin electrophysiological studies, inhibit glutamate-induced neurotoxicityand ischemia-induced neurodegeneration. The objective of thisstudy was to investigate the effects of both glycine site antagonistsand partial agonists on NMDA receptor-mediated [³H]arachidonic acid (AA) release evoked by glutamate, NMDA or acompetitive inhibitor of the glutamate/aspartate uptake carrier.The [³H]AA release evoked by a maximally effective concentration ofglutamate (100 µM) was blocked by the glycine site antagonists7-chlorokynurenic acid (7-CKYN) and 5,7- dichlorokynurenic acid(5,7-DCKYN) and by a low intrinsic efficacy glycine partial agonist(+)-1-hydroxy-3-aminopyrrolid-2-one [(+)-HA-966]. 1-Aminocyclopropanecarboxylicacid (ACPC), a high intrinsic efficacy glycine partial agonist,did not modify [³H]AA release evoked by 100 µM glutamate. However, ACPC blocked(in a glycine reversible manner) the [³H]AA release induced by NMDA (100 µM) with an IC₅₀ of 131 ± 2µM. Furthermore, L-trans-pyrrolidine-2,4-dicarboxylate (PDC),a competitive inhibitor of the glutamate transporter, also released[³H]AA (E_max and EC₅₀ of 127 ± 4% and 30 ± 1 µM, respectively).ACPC, 7-CKYN and (±)-2-amino-7-phosphonoheptanoic acid (AP-7),a competitive NMDA receptor antagonist, inhibited [³H]AA release evoked by PDC. These results demonstrate that bothglycine site antagonists and partial agonists can inhibit NMDAreceptor-mediated [³H]AA release in cerebellar granule cells, an action consistentwith the neuroprotective effects of these compounds.

	Introduction

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Activation of diverse neurotransmitter receptors as well as cell depolarization by elevation of extracellular K⁺ concentration can induce membrane phospholipid degradation andincrease AA release in a variety of neuronal preparations (Lazarewiczet al., 1992; Volterra et al., 1994; Farooqui and Horrocks, 1991).Although AA release may be effected through diverse mechanisms,several studies indicate that the AA release evoked by excitatoryamino acids in primary neuronal cell cultures is largely dependenton activation of NMDA receptor (Lazarewicz et al., 1992). Thus,NMDA has been shown to induce AA release in primary cultures ofstriatum (Dumuis et al., 1988), hippocampus (Sanfeliu et al.,1990) and cerebellar granule cells (Lazarewicz et al., 1988; Lazarewiczet al., 1990). These effects can be blocked by both competitive(e.g., 2-amino-5-phosphonopentanoic acid, AP-5) and noncompetitive(e.g., Mg⁺⁺) NMDA receptor antagonists (Lazarewicz et al., 1988; Sanfeliuet al., 1990). Moreover, phospholipase A₂ is the primary effectorenzyme responsible for NMDA receptor-evoked release of AA in neuronalcultures (Dumuis et al., 1988; Sanfeliu et al., 1990; Lazarewiczet al., 1990), and the coupling of NMDA receptors to phospholipaseA₂ has been shown to be directly linked to extracellular Ca⁺⁺ entry through NMDA receptor-coupled cation channels (Lazarewiczet al., 1990).

The NMDA receptor is a ligand-gated ion channel that contains discrete but interdependent regulatory domains (reviewed inMcbain and Mayer, 1994). NMDA receptors possess a transmitterrecognition site for acidic amino acids such as L-glutamate; acation channel with a unique voltage-dependent regulation by Mg⁺⁺, a polyamine site, and a coagonist site for glycine. The bindingof glycine to its recognition site on the NMDA receptor is strychnineinsensitive, and occupation of this site by an agonist appearsessential for channel activation (Kleckner and Dingledine, 1988;Curras and Pallotta, 1996).

There is evidence suggesting that glycine is present continuously within the extracellular space at levels that are at ornear saturation (Mcbain and Mayer, 1994). Both the physiologicalrole of glycine in the operation of NMDA receptors in vivo andthe pharmacological activity of antagonists and partial agonists(Foster et al., 1992; Baron et al., 1992; Grimwood et al., 1995;Grimwood et al., 1993; Marvizon et al., 1989) at this site remaincontroversial (Kehne et al., 1995; Lanthorn, 1994). We have hypothesizedthat if occupation of the glycine site by agonists is essentialfor the operation of the NMDA receptor complex, then partial agonistsat this glycine site, in the presence of the extracellular glycineconcentrations found in situ, may function as NMDA antagonists(Skolnick et al., 1989; Trullas et al., 1989).

In the present experiments, we have further explored this hypothesis by examining the effects of both high and low intrinsicefficacy glycine partial agonists and glycine site antagonistson NMDA receptor-mediated AA release in primary granule cell cultures.Furthermore, delayed neuronal cell death in ischemic brain injuryhas been associated with high levels of extracellular glutamateproduced by reverse operation of the high-affinity glutamate/aspartateuptake carrier (GLU/ASP). Thus, we also investigated the abilityof these glycine site ligands to prevent the effects of a competitiveinhibitor of the GLU/ASP carrier PDC on [³H]AA release. We now report that glycine partial agonists andantagonists reduce glutamate-, NMDA- and PDC-evoked AA release.These results provide evidence that in the presence of glycine,both glycine partial agonists and antagonists can function asNMDA receptor antagonists.

	Experimental Procedures

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Cerebellar granule cell cultures. Primary cultures of granule cells were prepared from cerebella of 7-day-old Wistar rat pups essentially as described (Fossomet al., 1995b). Procedures involving animals and their care wereconducted in conformity with institutional guidelines that arein compliance with national (DL no. 116, GU supplement 40, February18, 1992) and international (EEC Council Directive 86/609,OJ L358,1,12 December 1987; NIH Guide for the Care and Use of LaboratoryAnimals, NIH publication no. 85-23, 1985) laws and policies. Dissociatedcells were plated in 24-well plastic plates (2 cm²) previously coated with poly-L-lysine hydrobromide (10 µg/ml,MW > 300,000, Sigma), and the density was adjusted to give $approx$ 4× 10⁵ cells/cm². Cells were cultured in Eagle's basal medium with the followingadditions of 10% heat-inactivated fetal calf serum, 2 mM L-glutamine,0.1 mg/ml gentamicin, and 25 mM KCl. The replication of non-neuronalcells was prevented by adding cytosine arabinoside (10 µM) 18to 24 hr after plating. The cultures were incubated at 37°C in5% CO₂ in air saturated with water vapor. The cells were usedfor experiments after 8 to 11 days in culture.

[³H]AA release. Cultured neurons were incubated for 24 hr with 0.1 µCi/well of [³H]AA (specific activity, 221 Ci/mmol). During this period, cellsincorporated >80% of the radioactivity. All procedures were performedat 37°C. Labeled cells were washed twice with 0.5-ml aliquotsof Locke-HEPES buffer (154 mM NaCl, 5.6 mM KCl, 3.6 mM NaHCO₃,1.3 mM CaCl₂, 5.6 mM glucose and 10 mM HEPES, pH 7.35) and oncewith .5 ml of Locke-HEPES buffer with 0.2% fatty acid free bovineserum albumin (LH-BSA). Cells were preincubated for 10 min with0.5 ml of LH-BSA or with LH-BSA containing a competitive NMDAantagonist or glycine site ligands where appropriate. After preincubation,the medium was replaced with 0.5 ml of the same preincubationmedium containing L-glutamate, NMDA or PDC as specified. Aftera 15-min incubation, the medium was collected and centrifuged(12,000 × g) to remove possible contamination by occasionallypresent detached cells. The radioactivity released from the cellswas measured by liquid scintillation counting in disintegrationsper min [dpm; dpm = counts per min (cpm)/% efficiency) × 100].In agreement with previous results (Oomagari et al., 1991), analysisby HPLC of the medium collected after stimulation of cells with100 µM glutamate indicated that >90% of the lipid soluble radioactivityreleased from the cells was in the form of free AA (results notshown). After collecting the medium, cells were lysed in 0.5 mMNaOH and the radioactivity incorporated in membranes was measured.Total radioactivity was the sum of the [³H] released plus the [³H] incorporated into membranes. The amount of [³H]AA released was represented either as percentage of the controlvalues or as a percentage of the total radioactivity incorporatedinto the cultured cells minus the basal release in the absenceof agonists; % net [³H] release = {[([³H]released in the presence of drug × 100/total [³H] incorporated in the presence of drug)/([³H]released in the absence of drug × 100/total [³H] incorporated in the absence of drug)]× 100} $-$ 100.

Materials. Heat-inactivated fetal calf serum, culture media and gentamicin were purchased from GIBCO BRL (Cergy Pontoise, France). Othercell culture reagents were from Sigma (Madrid, Spain). [³H]AA was obtained from NEN (Brussels, Belgium). NMDA, 7-CKYN,5,7-DCKYN, (+)-HA-966 and (±)-AP-7 were from Research Biochemicals(Natick, MA). ACPC and PDC were from Tocris-Cookson (Bristol,UK), and glutamate and glycine were from Fluka Chemie AG (Buchs,Switzerland).

Statistical analysis. Data from inhibition curves were fitted to a four-parameter logistic equation using nonlinear regression analyses with Prismcomputer program (GraphPAD, San Diego, CA). Statistical significanceof differences among curve parameters was evaluated using independentt tests.

	Results

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Effects of glutamate and NMDA on [³H]AA release in cerebellar granule cells. Treatment of cerebellar granule cells with glutamate or NMDA (under Mg⁺⁺-free conditions) produced a concentration-dependent increaseof [³H]AA release in the absence of added glycine (fig. 1). Removalof extracellular Ca⁺⁺ completely blocked the effects of both glutamate (fig. 1) andNMDA (results not shown). In the presence of 1.3 mM Ca⁺⁺, glutamate enhanced [³H]AA release with an EC₅₀ of 13 ± 1 µM and E_max of 473 ± 6% (n= 12). NMDA exhibited a significantly lower potency (EC₅₀ = 62± 1 µM) and a lower maximal effect (E_max = 285 ± 24%, n = 7) thanglutamate in this measure (P < .05, Student's t test). Neitherthe EC₅₀ nor maximal effect of glutamate and NMDA were significantlyaltered in the presence of 10 µM glycine (EC₅₀ = 14 ± 1 µM and59 ± 3 µM; E_max = 432 ± 18% and 290 ± 3% for glutamate, n = 4,and NMDA, n = 4, respectively) (fig. 1). Removal of extracellularCa⁺⁺ or the incubation with NMDA or glutamate during a 15-min perioddid not have any significant effect on cell viability becausethe total radioactivity incorporated into the cells and the basalrelease were not significantly altered by these treatments.

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Fig. 1. Concentration-dependent release of [³H]AA by glutamate and NMDA in cerebellar granule cells. Granule cells were pre-incubated with [³H]AA for 24 hr and treated for 15 min with varying concentrations of glutamate or NMDA in BSA-containing, Mg⁺⁺ free medium, in the presence or absence of 10 µM Gly or 1.3 mM Ca⁺⁺. Results are expressed as percent mean ± S.E.M. of the total incorporated radioactivity after subtracting the basal release in the absence of agonists. Basal [³H]AA release was 368 ± 25 dpm, total [³H]AA incorporated was 37,073 ± 2,347 dpm. $bullet$ , GLU, n = 12; $black-triangle$ , GLU + 10 µM GLY, n = 4; $open circle$ , GLU no Ca⁺⁺, n = 2; $square$ , NMDA, n = 7; $black-square$ , NMDA + 10 µM GLY, n = 4.

Effects of glycine site ligands on [³H]AA release evoked by glutamate. 7-CKYN, 5,7-DCKYN and (+)-HA-966 inhibited glutamate (100 µM) induced [³H]AA release in a concentration dependent manner. Nonlinear regressionanalyses of inhibition curves showed that the glycinergic antagonists7-CKYN and 5,7-DCKYN did not significantly differ in their potenciesto inhibit [³H]AA release evoked by 100 µM glutamate. The IC₅₀ values for 7-CKYNand 5,7-DCKYN were 9 ± 1 µM (n = 4) and 10 ± 2 µM (n = 3), respectively.In contrast, the low efficacy, partial agonist (+)-HA-966 inhibited100 µM glutamate induced [³H]AA release with an IC₅₀ of 263 ± 2 µM (n = 4), a much lowerpotency than observed for glycine antagonists (P < .05, Student'st test) (fig. 2).

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Fig. 2. Concentration-dependent inhibition by glycine site ligands of 100 µM glutamate induced [³H]AA release from cerebellar granule cells. Granule cells were pre-incubated with [³H]AA for 24 hr. Varying concentrations of 7-CKYN, 5,7-DCKYN and (+)-HA-966 were added 10 min before addition of 100 µM glutamate in BSA-containing, Mg⁺⁺ free medium. Experiments were performed in the presence 10 µM Gly. Results are expressed as percent mean ± S.E.M. of the total incorporated radioactivity after subtracting the basal release in the absence of drugs. Release evoked by 100 µM glutamate was 1920 ± 192 dpm. $black-triangle$ , 5,7-DCKYN, n = 3; $black-square$ , (+)-HA-966, n = 4; $triangle$ , 7-CKYN, n = 4.

Effects of ACPC on [³H]AA release evoked by glutamate and NMDA. ACPC, a partial agonist at the glycine site with an intrinsic activity higher than (+)-HA-966 in electrophysiological andneurochemical studies (Watson and Lanthorn, 1990; Marvizon etal., 1989; Priestley and Kemp, 1994), did not alter the [³H]AA release induced by 100 µM glutamate (results not shown).However, ACPC inhibited [³H]AA release evoked by 20 µM glutamate (in the presence of 10µM added glycine) to an I_max of 60 ± 4% with an IC₅₀ of 506 ±18 µM (fig. 3A). ACPC also produced a complete, concentrationdependent, inhibition of the [³H]AA release evoked by 100 µM NMDA (in the presence of 10 µM addedglycine) with an IC₅₀ of 131 ± 2, n = 7 (fig. 3B). The inhibitoryeffect of ACPC was reversed by increasing the concentration ofglycine from 10 µM to 1 mM (fig. 3B, inset).

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Fig. 3. A, Concentration-dependent inhibition by ACPC of 20 µM glutamate-induced [³H]AA release from cerebellar granule cells. Granule cells were preincubated with [³H]AA for 24 hr. Varying concentrations of ACPC were added 10 min before addition of 20 µM glutamate in BSA-containing, Mg⁺⁺ free medium. Experiments were performed in the presence 10 µM Gly. Results are expressed as percent mean ± S.E.M. of the total incorporated radioactivity after subtracting the basal release in the absence of drug. Release evoked by 20 µM glutamate was 1445 ± 163 dpm. The I_max and IC₅₀ of ACPC were 60 ± 4% and 506 ± 18 µM, respectively. Values represent mean ± S.E.M., n = 4. B, Concentration-dependent inhibition by ACPC of 100 µM NMDA-induced [³H]AA release from cerebellar granule cells. Granule cells were preincubated with [³H]AA for 24 hr. Experiments were performed in the presence 10 µM Gly. Varying concentrations of ACPC were added 10 min before addition of 100 µM NMDA in BSA-containing, Mg⁺⁺ free medium. Results are expressed as percent mean ± S.E.M. of the total incorporated radioactivity after subtracting the basal release in the absence of drug. Release evoked by 100 µM NMDA was 1243 ± 289 dpm. The IC₅₀ of ACPC was 131 ± 2 µM. $black-square$ , ACPC (n = 7). Inset, addition of 1 mM glycine reverses the effect of 100 µM ACPC on NMDA (100 µM)-induced [³H]AA release from cerebellar granule cells. *Significantly different from control and GLY 1 mM groups (P < .05, Student's t test).

Effects of glycine site ligands on [³H]AA release evoked by PDC. PDC, a competitive inhibitor of the glutamate transporter, produced a concentration dependent release of [³H]AA in cerebellar granule cells with E_max and EC₅₀ of 127 ± 4%and 30 ± 1 µM, respectively (fig. 4A). The effect of PDC was reversedby 100 µM AP-7, a competitive NMDA-receptor antagonist. In addition,ACPC (1 mM), and 7-CKYN (50 µM) inhibited [³H]AA release evoked by PDC (fig. 4B).

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Fig. 4. A, Concentration-dependent release of [³H]AA by PDC in cerebellar granule cells. Cells were preincubated with [³H]AA for 24 hr and treated for 15 min with varying concentrations of PDC in BSA-containing, Mg⁺⁺ free medium. Results are expressed as percent mean ± S.E.M. of the total incorporated radioactivity after subtracting the basal release in the absence of drugs. Basal [³H]AA release was 205 ± 61 dpm. $black-square$ , PDC, n = 4. B, Inhibition by 7-CKYN, ACPC and AP-7 of [³H]AA release induced by 100 µM PDC in cerebellar granule cells. *Significantly different from PDC group (P < .05, Student's t test).

	Discussion

Top Abstract Introduction Procedures Results Discussion References

Consistent with previous findings (Lazarewicz et al., 1988, 1990, 1992), glutamate and NMDA produced a concentration-dependentrelease of previously accumulated [³H]AA in cerebellar granule cells. This effect was dependent onextracellular Ca⁺⁺. Glutamate was $approx$ 4-fold more potent and 2-fold more efficaciousthan NMDA (fig. 1). The magnitude of these effects was similarto that observed in previous studies using cerebellar granulecells (Rodriguez et al., 1993; Lazarewicz et al., 1988, 1990).The 4-fold lower potency of NMDA in this measure is also consistentwith previous studies demonstrating that glutamate is $approx$ 10-foldmore potent than NMDA as an inhibitor of radioligand binding towild-type glutamate receptors in rodent forebrain (Monahan andMichel, 1987; Olverman et al., 1988).

The observation that NMDA is only 50% as efficacious as glutamate in stimulating [³H]AA release is consistent with previous studies (Dumuis et al.,1988; Lazarewicz et al., 1990) and substantiates radioligand bindingstudies demonstrating that NMDA is less efficacious than glutamate(Foster and Wong, 1987; Loo et al., 1987). The ability of glycineantagonists to block glutamate-stimulated [³H]AA release (fig. 2), at concentrations that are inactive atnon-NMDA receptors, indicates that in cerebellar granule neurons,this effect of glutamate is mediated solely via activation ofNMDA receptors. In contrast, both NMDA and AMPA/kainate receptorsare involved in the glutamate evoked release of [³H]AA in cortical and striatal cell cultures (Dumuis et al., 1988;Stella et al., 1995).

The failure of exogenous glycine to augment glutamate- and NMDA-stimulated AA release (fig. 1) indicates that the concentrationof glycine in the medium is sufficient to permit the action ofglutamate and NMDA. In the presence of saturating concentrationsof glycine, the glycine site antagonists 7-CKYN and 5,7-DCKYN,as well as a low intrinsic efficacy glycine partial agonist, (+)-HA-966,all inhibited [³H]AA release evoked by 100 µM glutamate. These results providefurther evidence that activation of the glycine site is necessaryfor the operation of NMDA receptors (Kleckner and Dingledine,1988; Lerma et al., 1990; Curras and Pallotta, 1996), demonstratingthat this principle also applies to NMDA-evoked arachidonic acidrelease. The potencies of 7-CKYN (IC₅₀ = 9 µM) and (+)-HA-966(IC₅₀ = 263 µM) to inhibit glutamate (100 µM)-evoked [³H]AA release are similar to values previously reported for thesecompounds to act as NMDA antagonists in brain slices (Foster andKemp, 1989; Kemp et al., 1988) and in preventing hypoxia-inducedneurodegeneration in rat cortical cell cultures (Priestley etal., 1990). Moreover, the potency of 5,7-DCKYN (IC₅₀ = 10 µM)to inhibit glutamate-evoked [³H]AA release is similar to the value reported (IC₅₀ = 4 ± 1 µM)for inhibition of NMDA-stimulated cGMP accumulation in cerebellarslices (Baron et al., 1990). Nonetheless, both the absolute valuesand rank order potencies of these glycine site compounds differfrom data obtained in radioligand binding and electrophysiologicalstudies. For example, in forebrain membranes, 5,7-DCKYN exhibitshigher affinity (K_i 80 nM) for the glycine site than 7-CKYN (K_i360 nM) (Baron et al., 1992). The higher potencies of these compoundsin radioligand binding assays can be explained by incubation conditions(e.g., temperature, ionic milieu, elimination of endogenous glycine,and a homogeneous tissue preparation) intended to optimize ligandaffinities that cannot be duplicated using intact cell or tissuepreparations. The differences in rank order potency among glycinesite ligands may be attributed, at least in part, to preparationdependent variations in NMDA receptor subunit composition. Thus,studies in recombinant receptors indicate that subunit compositionis the primary determinant of ligand affinity for a wide varietyof structurally diverse compounds (Laurie and Seeburg, 1994; Waffordet al., 1993). Consistent with this interpretation, the potenciesof a series of glycine site ligands to inhibit [³H]glycine binding can vary by >20-fold between hippocampus andcerebellum (Yoneda and Ogita, 1991).

The ability of (+)-HA-966, a partial agonist at the glycine site, to inhibit glutamate evoked [³H]AA release with an efficacy similar to the observed with competitiveglycine antagonists is in agreement with previous studies showingthat HA-966 and 7-CKYN display equivalent neuroprotective effectsagainst glutamate induced neurotoxicity in vitro (Boje et al.,1993). The similar inhibition obtained with a partial agonistand an antagonist can be explained by the very low intrinsic activityof HA-966 obtained in most preparations (Priestley and Kemp, 1994;Henderson et al., 1990). However, ACPC, a partial agonist witha higher intrinsic activity than HA-966 (Watson and Lanthorn,1990; Priestley and Kemp, 1994), did not alter the [³H]AA release evoked by a maximally effective concentration ofglutamate (100 µM) but inhibited [³H]AA release induced by 20 µM glutamate by a maximum of 60% (fig.3A). Moreover, ACPC completely blocked (in a glycine reversiblemanner) the [³H]AA release induced by 100 µM NMDA (fig. 3B).

Electrophysiological studies indicate that ACPC is a partial agonist with a very high intrinsic activity (80-95%) (Watsonand Lanthorn, 1990; Priestley and Kemp, 1994). However ACPC isneuroprotective in vivo (Long and Skolnick, 1994; Fossom et al.,1995b) and also mimics several other pharmacological actions,such as anticonflict (Trullas et al., 1989; Przegalinski et al.,1996), antidepressant (Trullas and Skolnick, 1990), and blockadeof opiate tolerance (Kolesnikov et al., 1994) of NMDA antagonists.The apparent divergence between the NMDA receptor antagonist profileof ACPC in vivo and the high efficacy that this compound showsin electrophysiological experiments has led to the suggestionthat the effects of ACPC in vivo cannot be attributed to an actionof this compound at the NMDA receptor (Kemp and Leeson, 1993;Wood, 1995). However, the inhibition by ACPC, in a glycine reversiblemanner, of NMDA evoked [³H]AA release observed in the present study in cerebellar granulecells provides strong evidence to suggest that ACPC reduces NMDAreceptor function at the glycine site. Moreover, consistent witha high intrinsic efficacy partial agonist action, ACPC partiallyinhibited glutamate evoked [³H]AA release (fig. 3A). As the concentration of glutamate (orNMDA) increases, the ability of exogenous glycine to augment theactions of glutamate (or NMDA), such as generation of cGMP orneurotoxicity, is lost in cerebellar granule cell cultures (Bojeet al., 1993; Fossom et al., 1995b). Both electrophysiologicaland neurochemical evidence indicates that this augmentation byglycine may in part be attributed to a "left shift" in the concentrationeffect curve of glutamate (or NMDA) (Johnson and Ascher, 1987;Monaghan et al., 1988; Hood et al., 1990). At low to moderateconcentrations of NMDA or glutamate, ACPC would result in a smallerincrease in the affinity of glutamate relative to that observedwith glycine, resulting in an apparent "functional NMDA antagonist"action. However, at higher glutamate (or NMDA) concentrations,this dampening effect would be negligible. This hypothesis isconsistent with the ability of ACPC to produce a concentrationdependent but partial reduction in granule cell neurotoxicityat glutamate concentrations (<25 µM) that induce low to moderatedamage (Boje et al., 1993; Fossom et al., 1995a), while lackingthis neuroprotective action against a maximally effective glutamateinsult. Similarly, ACPC reduced cGMP formation in these culturesat low to moderate but not high concentrations of NMDA (Fossomet al., 1995b; Fossom et al., 1995a).

Pathological conditions of hypoglycemia or ischemic brain injury are associated with both AA and excitatory amino acid release(Lazarewicz et al., 1992). It has been suggested that under conditionsof energy deprivation, like anoxia or ischemia, there is an excessiveincrease of extracellular excitatory amino acids produced by reverseoperation of the high-affinity glutamate/aspartate (GLU/ASP) uptakecarrier (Szatkowski and Attwell, 1994). In the present study,we mimicked the reversal of this carrier by treating cells withPDC, a competitive substrate of the high affinity GLU/ASP transporter(Bridges et al., 1991; Griffiths et al., 1994) that does not showNMDA receptor agonist activity at concentrations in the low micromolarrange (Balcar et al., 1995). In the present studies, PDC increased[³H]AA release in a concentration-dependent manner and this increasewas NMDA receptor mediated since it was blocked by AP-7. In agreementwith the results obtained with glycine antagonists and partialagonists on glutamate and NMDA mediated [³H]AA release, both 7-CKYN and ACPC inhibited the [³H]AA release evoked by a maximally effective concentration ofPDC. These results suggest that glycine site antagonists and partialagonists may reduce the effects of excessive excitatory aminoacid release induced by alterations of the GLU/ASP uptake systemand are consistent with previous studies showing that glycineantagonists and partial agonists reduce neuronal damage afterischaemia in animal models (Wood et al., 1993; Von Lubitz et al.,1992; Pellegrini-Giampietro et al., 1994; Fossom et al., 1995b).

AA release and its metabolism has been hypothesized to play a significant role in the cell damage produced by the excitotoxiccascade (Bigge and Boxer, 1994; Volterra et al., 1994; Katsukiand Okuda, 1995; Bazan et al., 1995). AA oxidation produces freeradicals that may contribute to neuronal damage via inflammatoryreactions or may act as dowstream mediators of excitotoxicty andfurther enhance glutamate release (Bigge and Boxer, 1994). Theability of glycine partial agonists and antagonists to attenuateNMDA receptor mediated AA release and protect against cell damageinduced by a variety of excitotoxic treatments (Boje et al., 1993;Von Lubitz et al., 1992; Patel et al., 1990; Long and Skolnick,1994; Foster et al., 1990; Priestley et al., 1990; Fossom et al.,1995b; Zapata et al., 1996) is consistent with this hypothesis.

In summary, the present results show that both glycine antagonists and partial agonists can inhibit glutamate and NMDA stimulated[³H]AA release. These findings are consistent with both in vivoand in vitro studies demonstrating the neuroprotective propertiesof these compounds. Furthermore, these results provide evidencethat in the presence of saturating concentrations of glycine,both glycine partial agonists and antagonists may function asNMDA receptor antagonists.

	Footnotes

Accepted for publication January 26, 1998.

Received for publication October 9, 1997.

¹ This work was supported by a grant from Dirección General de Investigación Científica y Técnica, Ministry of Educationof Spain, DGICYT, PB94-0017 to R.T.

² E.V. was supported by a predoctoral fellowship from Direcció General D'Universitats/CIRIT. Generalitat de Catalunya.

³ A.Z. is a Severo Ochoa Fellow from Ferrer International Foundation.

Send reprint requests to: Ramon Trullas, Ph.D., Unitat de Neurobiologia, IIBB/C.S.I.C., Jordi Girona 18-26, 08034 Barcelona, Spain. E-mail: rtonbi{at}cid.csic.es

	Abbreviations

AA, arachidonic acid; ACPC, 1-aminocyclopropanecarboxylic acid; (±)-AP-5, 2-amino-5-phosphonopentanoic acid; (±)-AP-7, 2-amino-7-phosphonoheptanoic acid; ASP, aspartate; BSA, bovine serum albumin; 7-CKYN, 7-chlorokynurenic acid; 5, 7-DCKYN, 5,7-dichlorokynurenic acid; GLU, glutamate; GLY, glycine; (+)-HA-966, 1-hydroxy-3-aminopyrrolid-2-one; HPLC, high-pressure liquid chromatography; LH-BSA, Locke-HEPES buffer with fatty acid-free bovine serum albumin; MK-801, 5-methyl-10,11-dihydro-5H-dibenzo(a,d)cyclohept- 5,10-imine hydrogen, dizocilpine maleate; NMDA, N-methyl-D-aspartate; PDC, L-trans-pyrrolidine-2,4-dicarboxylic acid.

	References

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Glycine Site Antagonists and Partial Agonists Inhibit N-Methyl-D-aspartate Receptor-Mediated [3H]Arachidonic Acid Release in Cerebellar Granule Cells1

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