Mapping the Binding Site of the Neuroprotectant Ifenprodil on NMDA Receptors

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The Journal of Neuroscience, July 15, 2002, 22(14):5955-5965

Mapping the Binding Site of the Neuroprotectant Ifenprodil on NMDA Receptors
Florent Perin-Dureau, Julie Rachline, Jacques Neyton, and Pierre Paoletti
Laboratoire de Neurobiologie, Centre National de la Recherche Scientifique, Unité Mixte de Recherche 8544, Ecole Normale Supérieure, 75005 Paris, France

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
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DISCUSSION
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Ifenprodil is a noncompetitive antagonist of NMDA receptors highly selective for the NMDA receptor 2B (NR2B) subunit. It iswidely used as a pharmacological tool to discriminate subpopulationsof NMDA receptors, and derivatives are currently being developedas candidate neuroprotectants. Despite numerous studies on themechanism of action of ifenprodil on NMDA receptors, the structuraldeterminants responsible for the subunit selectivity have notbeen identified. By combining functional studies on recombinantNMDA receptors and biochemical studies on isolated domains, wenow show that ifenprodil binds to the N-terminal leucine/isoleucine/valine-bindingprotein (LIVBP)-like domain of NR2B. In this domain, several residues,both hydrophilic and hydrophobic, were found to control ifenprodilinhibition. Their location in a modeled three-dimensional structuresuggests that ifenprodil binds in the cleft of the LIVBP-likedomain of NR2B by a mechanism (Venus-flytrap) resembling thatof the binding of Zn on the LIVBP-like domain of NR2A. These resultsreinforce the proposal that the LIVBP-like domains of NMDA receptors,and possibly of other ionotropic glutamate receptors, bind modulatoryligands. Moreover, they identify the LIVBP-like domain of theNR2B subunit as a promising therapeutic target and provide a frameworkfor designing structurally novel NR2B-selectiveantagonists.

Key words: glutamate receptors; NMDA; ifenprodil; phenylethanolamine; LIVBP; neuroprotection

  INTRODUCTION

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INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Ionotropic glutamate receptors (iGluRs) are made of subunits sharing a common membrane topology: a large N-terminal extracellularregion, three transmembrane segments (TM1, TM3, and TM4), a Ploop region (initially called TM2) that forms the pore selectivityfilter, and a cytoplasmic C-terminal region (Dingledine et al.,1999). The agonist binding domain, made of ~150 amino acids precedingTM1 together with the extracellular loop between TM3 and TM4,is distantly related to the bacterial periplasmic-binding protein(PBP) glutamine binding protein (GlnBP) (Stern-Bach et al., 1994).It has been crystallized in the case of the AMPA subunit GluR2and the prokaryotic glutamate receptor subunit GluR0, showinga bilobed structure with the agonist bound in a central cleft(Armstrong et al., 1998; Mayer et al., 2001).

Eukaryotic iGluR subunits possess an additional extracellular N-terminal domain made of the first ~380 amino acids that isweakly related to leucine/isoleucine/valine-binding protein (LIVBP),another PBP (O'Hara et al., 1993). In AMPA and kainate receptors,this domain participates in subunit oligomerization (Kuusinenet al., 1999; Leuschner and Hoch, 1999; Ayalon and Stern-Bach,2001). In NMDA receptors (NRs; heteromers made of NR1 and NR2A-NR2Dsubunits), we have proposed recently that the LIVBP-like domainsof the NR2 subunits also have a bilobed structure, and we haveshown that in NR2A, this domain forms a high-affinity Zn bindingsite (Paoletti et al., 2000) (also see Choi and Lipton, 1999;Fayyazuddin et al., 2000; Low et al., 2000).

Ifenprodil is representative of a class of NMDA receptor antagonists (phenylethanolamines) with high selectivity for NR2B-containingreceptors (Williams, 1993; Chenard and Menniti, 1999). Severalphenylethanolamines are neuroprotective both in vitro and in invivo models of a variety of neurological disorders and lack manyof the side effects associated with non-subunit-selective NMDAreceptor antagonists (references in Kew and Kemp, 1998); theyalso produce antinociceptive effects (Chizh et al., 2001). Ifenprodilacts as a noncompetitive, partial, and voltage-independent antagonist(Carter et al., 1988; Legendre and Westbrook, 1991; Williams,1993). Its potency strongly depends on the extracellular pH andis only weakly affected by the insertion of the NR1 exon 5 (Pahkand Williams, 1997; Mott et al., 1998). Finally, ifenprodil displaysuse dependence such that binding of glutamate increases bindingof ifenprodil and vice versa (Kew et al., 1996; Zheng et al.,2001). On the basis of binding experiments on chimeric NR2 subunits,Gallagher et al. (1996) have proposed that determinants of ifenprodilinhibition locate to the N terminus of NR2B. However, using amutagenesis approach, Masuko et al. (1999) concluded in favorof a binding site located in the N terminus of NR1. Thus, despitethe detailed functional characterization of the mechanism of ifenprodilinhibition, the precise location of the ifenprodil binding sitehas remained for the most partelusive.

All the functional properties of the ifenprodil inhibition of NR2B-containing receptors listed above also apply to the high-affinityZn inhibition of NR2A-containing receptors (Westbrook and Mayer,1987; Christine and Choi, 1990; Paoletti et al., 1997; Trayneliset al., 1998; Choi and Lipton, 1999; Low et al., 2000; Zheng etal., 2001). This striking similarity between both antagonismssuggests that Zn and ifenprodil share a common mechanism of modulationat the structural level. We now show that, similarly to the Znbinding site on the NR2A LIVBP-like domain, the LIVBP-like domainof NR2B forms in its central cleft a high-affinity binding siteforifenprodil.

  MATERIALS AND METHODS

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Molecular biology. The expression plasmids, mutagenesis strategy, RNA synthesis, and NR2A/NR2B chimera constructions havebeen described previously by Paoletti et al. (1997, 2000). Eachmutation was verified by sequencing across the mutated region(~400-600 bp; Genome Express, Montreuil, France). For each mutationstrongly affecting ifenprodil inhibition, two independent cloneswere isolated, sequenced, and functionally characterized (exceptfor NR2B-K234A, for which only one clone has been isolated). Pointmutations in isolated LIVBP-like domains were made by using mismatchPCR (QuikChange; Stratagene Europe, Amsterdam, The Netherlands)and verified by sequencing the entiredomain.

Electrophysiology and data analysis. Xenopus laevis oocytes were prepared, kept, injected with cRNAs, voltage-clamped, andsuperfused as described by Paoletti et al. (1995, 1997). Oocyteswere injected with 30-40 nl of a mixture of NR1 and NR2 cRNAs(ratio, 1:2) at a final concentration of 100 ng/µl and recordedin the following 1-4 d. The control solution superfusing the oocytescontained (in mM): 100 NaCl, 5 HEPES, 0.3 BaCl₂, and 10 Tricine(used to chelate traces amount of contaminating Zn; Paoletti etal., 1997). The pH was adjusted to 7.3 with KOH. Both L-glutamateand glycine were prepared as 250 µl aliquots (in bidistilled water)at 100 mM and stored at $-$ 20°C. NMDA currents were induced by applicationof the agonist solution containing a saturating concentrationof both L-glutamate and glycine (100 µM each). Ifenprodil (a giftfrom B. Scatton, Sanofi-Synthélabo, Bagneux, France) was preparedas 50 µl aliquots (in bidistilled water) at 10 mM and stored at $-$ 20°C. Ifenprodil (0.03-30 µM) was extemporaneously diluted inagonist solution, protected from light, and used within 4 hr.All experiments were performed at room temperature (18-24°C) withoocytes that exhibited agonist-induced currents within the 150-1500nA range at $-$ 60 mV (except for NR2B-I150A, for which currentswere never >200nA).

The kinetics of ifenprodil inhibition are particularly slow (see Fig. 2A; for 1 µM ifenprodil, they are much slower than theestimated rate of complete exchange of the solution in our recordingchamber, ~2 sec; Paoletti et al., 1997) and therefore could beestimated directly from the current relaxations at the onset andoffset of ifenprodil applications. The kinetic parameters shownin Figure 1B were estimated with the fitting procedure of Clampfit6.0.5 (Axon Instruments, Foster City, CA). Off relaxations couldbe well fitted with a single exponential (yielding $tau$ _off), whereason relaxations had to be fitted with either two exponentials orone exponential and a sloping baseline; however, during the first30 sec of ifenprodil application (leading to 90-95% of the totalinhibition at equilibrium), on relaxations could be satisfactorilyfitted with a single exponential (yielding $tau$ _on).

Because of the slow on rate of ifenprodil inhibition, ifenprodil solutions had to be applied for 30 sec (30 µM), 60 sec (3-10µM), 60-90 sec (0.3-1 µM), or 120 sec (30-100 nM) to reach equilibrium.Regarding the very slow dissociation rate constant of ifenprodil,recovery to control agonist-induced current was usually not attempted(except in those experiments aimed at evaluating $tau$ _off). Thus,the typical protocol used in this study was control agonist solutionapplied for 40 sec (to verify the stability of the control current),immediately followed by two increasing ifenprodil concentrationssuccessively applied (90-150 sectotal).

Experimental points were fitted with the following Hill equation: (100 × I_ifen/I_control) = 100 $-$ a/((1 + (IC₅₀/[ifen])n_H),where 100 × I_ifen/I_control is the mean relative current (percentage),[ifen] is the ifenprodil concentration, n_H is the Hill coefficient,IC₅₀ is the concentration of ifenprodil producing 50% of the maximalinhibition, and a is the maximal inhibition at the saturatingifenprodil concentration. IC₅₀, a and n_H were set as free parameters.For NR1/NR2B mutated receptors (see Fig. 6), ifenprodil concentration-responsecurves at $-$ 60 mV were fitted without any attempt to correct forthe ifenprodil voltage-dependent block (correction would havebeen ~10% at 10 µM ifenprodil and negligible for lower ifenprodilconcentrations). For mutants displaying mean relative currents>60% even at the highest ifenprodil concentration tested (10 µM),no Hill fit was attempted, but rather, experimental points weregraphically linked by a constrained sigmoidal curve, and IC₅₀was arbitrarily reported to be >10 µM.

To study the voltage-dependent block in NR2A wild-type (wt)- and NR2B (LIVBP NR2A)-containing receptors at high (10 and 30µM) ifenprodil concentrations, 2 sec $-$ 70/+50 mV voltage rampswere used (capacitive and leakage currents were recorded beforeagonist application and subtracted from the agonist-inducedcurrents).

Error bars represent the SD of the mean relativecurrents.

Production of isolated LIVBP-like domains in Escherichia coli and proteolysis experiments. LIVBP-like domains of the NR2Aand of the NR2B subunits were produced as thrombin-cleavable glutathioneS-transferase (GST) fusion proteins in E. coli. LIVBP-like domainsof the rat NR2A (Glu²⁸-Val³⁷⁵) and of the mouse NR2B ( $epsilon$ 2; Ser²⁸-Val³⁷⁶) were subcloned in the pGEX-2T vector (Amersham Biosciences,Buckinghamshire, UK). After transformation, BL21(DE3) cells weregrown in 1 liter of Luria-Bertani medium supplemented with ampicillin(100 µg/ml) at 37°C until OD₆₀₀ reached 0.7-0.8. Protein productionwas induced by 1 mM isopropyl- $beta$ -D-thiogalactopyranoside (RocheBiochemicals, Meylan, France) for 2.5 hr at 37°C. The followingsteps, adapted from those of Chen and Gouaux (1997), were performedeither on ice or at 4°C. Cells were harvested and resuspendedin buffer 1 (in mM: 200 NaCl, 20 Tris, and 1 EDTA, pH 7.5). Thecells were sonicated for 2 min. Inclusion bodies were collectedby centrifugation (15,000 rpm, 20 min), resuspended in buffer1 (20 ml), and purified by a first incubation (30 min) in thepresence of DNase1 (1 mg), deoxycholic acid (120 mg), and lysozyme(100 mg), followed by a second incubation (30 min) with 0.5% TritonX-100. Purified inclusion bodies were then solubilized overnightin buffer 2 (6 M GuHCl, 50 mM Tris, and 10 mM DTT, pH 8.0). Proteins(~1 mg/ml) were refolded by 16 hr of dialysis against a 20-foldhigher volume of buffer 3 (in mM: 500 NaCl, 50 Tris, and 1 DTT,pH 8.0), using a membrane tube with a molecular mass cutoff of15,000 Da (Fisher, Illkirch, France). Buffer 3 was changed after8 hr of incubation. Refolded proteins were separated from theprecipitate by centrifugation (1 hr, 40 000 rpm) and purifiedusing glutathione-Sepharose beads (Amersham Biosciences). LIVBP-likedomains of NR2A and NR2B were cleaved from the GST by a 2 hr digestionwith human thrombin (Roche Biochemicals), which was stopped byaddition of 2 mM PMSF. Protein concentration was measured at OD₂₈₀using extinction coefficients of 57,160 and 52,180 M¹cm¹ for NR2A and NR2B, respectively. With 1 liter of bacterial culture,we usually obtain ~10 mg of purified solubleprotein.

Trypsin proteolysis experiments were performed using a protein solution at 0.2 or 0.5 mg/ml (NR2A or NR2B LIVBP-like domain),and the trypsin concentration was adjusted to have a final protease/proteinratio of 1:500. Reactions were performed at room temperature.Preincubations with ifenprodil or Zn were done for 5 min beforeadding trypsin. Proteolysis was stopped at varied times by mixingaliquots of the reaction solution to the SDS-containing 2× samplebuffer. Samples were analyzed on 12% SDS-PAGE gels (Bio-Rad, Hercules,CA) and stained with SyPro Orange (Molecular Probes, Leiden, TheNetherlands), and SyPro Orange fluorescence was revealed usinga fluorophosphoimager (FLA-3000; Fujifilm, St-Quentin-en-Yvelines,France) at $lambda$ = 475nm.

Alignments and three-dimensional modeling. The alignments of Figure 4 were primarily adapted from the alignments presentedby Paoletti et al. (2000). E. coli LIVBP [GenBank accession number,230609; Protein Data Bank (PDB) coordinates, 2LIV; Sack etal., 1989], rat metabotropic GluR1 (mGluR1; GenBank accessionnumber, P23385; PDB coordinates, 1EWT; Kunishima et al.,2000), and human atrial natriuretic peptide clearance receptortype C (ANP-C; GenBank accession number, P17342; PDB coordinates,1JDN; He et al., 2001) were aligned by structure superimpositiondeduced from visual inspection of the secondary structure elements.For NR1, conserved patterns of clusters of hydrophobic residuesbetween the LIVBP-like domain of NR1 and LIVBP were identifiedusing hydrophobic cluster analysis (Callebaut et al., 1997). Thisconservation, which indicates a conserved fold, was used to constrainthe alignment of the LIVBP-like domain of NR1 with LIVBP (Paolettiet al., 2000). The 3D structure of the NR2B LIVBP-like domainwas modeled by homology to the structure of the unliganded formof LIVBP (PDB coordinates, 2LIV; Sack et al., 1989) on thebasis of the sequence alignment shown in Figure 4. The model wasproduced by Modeler 4 (Sali and Blundell, 1993).

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INTRODUCTION
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The LIVBP-like domain of the NR2B subunit confers high sensitivity to ifenprodil

To test our prediction that the target of ifenprodil is the LIVBP-like domain of NR2B, we first assessed the ifenprodil sensitivityof chimeric NMDA receptors in which the LIVBP-like domains wereswapped from one NR2 subunit to the other. Chimeric NR2 subunitsNR2A-(LIVBP NR2B) and the complementary subunit NR2B-(LIVBP NR2A)were obtained by substituting the entire LIVBP-like domain (i.e.,the first ~390 amino acids; Paoletti et al., 2000; Fig. 1A) ofNR2A (a subunit with poor ifenprodil sensitivity; Williams, 1993)by that of NR2B. NMDA receptors were expressed in Xenopus oocytes,and NMDA currents were induced by saturating concentrations ofL-glutamate (100 µM) and glycine (100 µM). As shown in Figure1A, replacing the LIVBP-like domain of NR2A by that of NR2B transfersthe NR2B-specific high-sensitivity ifenprodil inhibition fromNR2B to the chimera. In contrast, the converse chimera shows verylittle ifenprodil sensitivity. Indeed, 1 µM ifenprodil stronglyinhibited NR2B- and NR2A-(LIVBP NR2B)-containing receptors [meanresidual relative currents, 16 ± 2% (n = 12) and 23 ± 4% (n =5), respectively], whereas the same concentration had little effecton either NR2A- or NR2B-(LIVBP NR2A)-containing receptors [meanresidual relative currents, of 94 ± 1% (n = 4) and 97 ± 1% (n= 5), respectively].

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Figure 1. The LIVBP-like domain of NR2B controls the high-affinity ifenprodil inhibition of NMDA receptors. A, Swapping the LIVBP-like domain between NR2B and NR2A subunits transfers the NR2B-specific high-affinity ifenprodil (ifen) inhibition from NR2B to NR2A. Each trace shows the inhibition of the current response to agonists (agos; glutamate and glycine, 100 µM each) by 1 µM ifenprodil in Xenopus oocytes coexpressing either NR2B wt, NR2A wt, or chimeric NR2B/NR2A subunits with the NR1 wt subunit. Note that the slow kinetics of ifenprodil inhibition of NR1/NR2B wt (most particularly the recovery rate) are also observed in NR1/NR2A-(LIVBP NR2B) receptors. The recordings were made at $-$ 60 mV. The bars above the current traces indicate the duration of agonists and ifenprodil applications. A schematic diagram of the NR2 construct is shown on top of each trace: LIVBP, LIVBP-like domain; S1 S2, agonist-binding GlnBP-like domain; 1, 3, 4, transmembrane segments; 2, reentrant pore loop. B, NR1/NR2B wt and NR1/NR2A-(LIVBP NR2B) receptors display similar kinetic parameters of ifenprodil inhibition. The time constants of onset ( $tau$ _on) and offset ( $tau$ _off) of the inhibition of agonist-induced currents by 1 µM ifenprodil were estimated by single-exponential fits to traces such as those shown in A (see Materials and Methods for the fitting procedures). The mean $tau$ _on and $tau$ _off values are as follows: NR2B wt, 7.1 ± 1 sec (n = 13) and 59 ± 7 (n = 7), respectively; NR2A-(LIVBP NR2B), 10.6 ± 0.6 sec (n = 5) and 73 ± 7 sec (n = 3), respectively.

One striking feature of the high-affinity ifenprodil antagonism of NMDA receptors is the slowness of both the onset of blockadeon drug application and the offset after drug removal. The fullrecovery of inhibition by ifenprodil of wt NR1/NR2B receptorsrequires >5 min (Williams, 1993; Kew et al., 1996; Fig. 1A, topleft). Similar slow kinetics were observed with the NR2A-(LIVBPNR2B)-containing receptor using protocols with long applicationsof both agonists and ifenprodil (Fig. 1A,B).

We also obtained ifenprodil concentration-response curves at equilibrium (Fig. 2A). For wt NR1/NR2B receptors, as alreadyshown on recombinant (Williams, 1993; Mott et al., 1998; Masukoet al., 1999) and native (Kew et al., 1996) NMDA receptors, ifenprodilinhibition was partial (maximal inhibition of ~96% at saturatingifenprodil concentrations), had an IC₅₀ in the hundreds of nanomolarrange (156 nM), and had an n_H value very close to 1 (0.99). Similarvalues were obtained with the NR1/NR2A-(LIVBP NR2B) receptors:maximal inhibition of 94%, IC₅₀ of 215 nM, and n_H of 1.0. NR1/NR2Aand NR1/NR2B-(LIVBP NR2A) receptors were only slightly inhibitedby ifenprodil. At the highest concentration of ifenprodil tested(30 µM), the mean residual current was 48 ± 6% (n = 8) for NR2Awt receptors and 67 ± 3% (n = 7) for NR2B-(LIVBP NR2A), thus correspondingto a decrease of at least 200-fold in ifenprodil sensitivity.

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Figure 2. Parameters of ifenprodil inhibition of the chimeric and wild-type NMDA receptors. A, Concentration-response curves at equilibrium and at $-$ 60 mV. Data points were fitted with Hill equations (see Materials and Methods). Each point is the mean value of 3-15 oocytes. The estimated values of IC₅₀, n_H, and maximal inhibition are, respectively, 155 nM, 0.98, and 96% for NR2B wt and 215 nM, 1.00, and 94% for NR2A-(LIVBP NR2B). For NR2A wt and NR2B-(LIVBP NR2A), the estimated IC₅₀ values are 28 and 75 µM, respectively. B, The low-affinity ifenprodil inhibition of NR2A- and NR2B-(LIVBP NR2A)-containing receptors is voltage-dependent. Leak-subtracted agonist-induced NMDA currents were recorded in the absence (cont) and presence of 30 µM ifenprodil (ifen) during 2 sec voltage ramps from $-$ 70 to +50 mV. Insets, Mean relative currents (percentage) measured at $-$ 60 and +40 mV.

Williams (1993) showed that the high- and low-affinity ifenprodil inhibitions differ markedly in their voltage dependency.The high-affinity NR2B-specific ifenprodil inhibition is voltage-independent,whereas the inhibitory effects of high concentrations of ifenprodilat NR2A-containing receptors are mostly voltage-dependent. Thisdifference suggests that ifenprodil binds on two distinct sites,one extracellular (accounting for the high-affinity inhibition)and the other within the pore (accounting for the low-affinityinhibition). The low-affinity ifenprodil pore blockade of wt NR2A-containingreceptors is illustrated in Figure 2B1, which compares agonist-inducedcurrents obtained during voltage ramps ( $-$ 70/+50 mV) before andafter application of a high ifenprodil concentration (30 µM).The current is very weakly inhibited by ifenprodil at +40 mV comparedwith $-$ 60 mV (see inset). As shown in Figure 2B2, a qualitativelysimilar voltage-dependent ifenprodil block is observed with NR2B-(LIVBPNR2A)-containing receptors. [Note that in wt NR2B-containing receptors,high ifenprodil concentrations ( $>=$ 30 µM) also produce an outwardrectification of the residual currents (data not shown).] Therefore,as for wt NR2A-containing receptors, the blocking effect of ifenprodilat NR2B-(LIVBP NR2A)-containing receptors most probably involvesthe binding of ifenprodil to the pore site rather than to the"extracellular" site. In consequence, the apparent 200-fold shiftin ifenprodil sensitivity deduced from the concentration-responsecurves constructed at negative potentials underestimates the selectivityof the ifenprodil binding for the extracellular site associatedwith the LIVBP-like domain of NR2B versus that ofNR2A.

Ifenprodil protects the isolated LIVBP-like domain of NR2B against digestion by trypsin

The experiments presented above using chimeric NMDA receptors suggest that the LIVBP-like domain of NR2B contains moleculardeterminants that are required for ifenprodil to produce its high-affinityinhibitory effects. Two hypotheses could account for an involvementof the NR2B LIVBP-like domain in the ifenprodil modulation: (1)the LIVBP-like domain of NR2B contains (at least part of) theifenprodil binding site; and (2) the LIVBP-like domain of NR2Bdoes not bind ifenprodil but is required for the transductionmechanism that links binding of ifenprodil to receptor inhibition.We sought to discriminate between the two hypotheses by testingwhether ifenprodil could bind to the isolated LIVBP-like domainof NR2B using a proteolysis protection assay. The rationale underlyingsuch experiments is that ligand binding, by stabilizing the proteinin its folded conformation, may decrease the accessibility ofproteolytic sites (Hubbard, 1998).

Isolated LIVBP-like domains of NR2A and NR2B were produced in E. coli as thrombin-cleavable GST fusion proteins (see Materialsand Methods). On SDS-PAGE gels, both domains run as a major bandof the expected molecular mass (~40 kDa) (Fig. 3). Minor bandsof lower molecular mass, mostly seen at ~30 kDa in the case ofNR2B, partly result from thrombin overdigestion (see below). Weperformed trypsin digestion of the isolated NR2B LIVBP-like domainin the presence and absence of 10 µM ifenprodil (a saturatingconcentration for the high-affinity inhibition) (Fig. 2A), usinga trypsin/protein ratio of 1:500. In the absence of ifenprodil,digestion of the NR2B LIVBP-like domain occurs quickly, as shownby the complete disappearance of the 40 kDa band after 5 min.In contrast, in the presence of ifenprodil, the rate of digestionis greatly slowed, with a substantial amount of undigested proteinstill present after 5 min (Fig. 3A). Similar results were obtainedin nine different experiments with ifenprodil concentrations of10 µM (n = 6), 30 µM (n = 2), and 100 µM (n = 1). Thus, the presenceof ifenprodil markedly slows the trypsin digestion of the LIVBP-likedomain of NR2B.

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Figure 3. Ifenprodil protects the isolated LIVBP-like domain of NR2B but not that of NR2A against hydrolysis by trypsin. Isolated LIVBP-like domains of NR2A and NR2B were produced in E. coli and subjected to trypsinization with or without ifenprodil or Zn for various amounts of time (up to 10 min). Fifty micrograms of the purified LIVBP-like domains were mixed with 0.1 µg of trypsin. The samples were analyzed on 12% SDS-PAGE gels. Lane 0 corresponds to the protein solution just before trypsin addition. A, Ifenprodil (10 µM) protects the NR2B LIVBP-like domain (main band at ~40 kDa) against trypsin digestion. B, Ifenprodil (10 µM) also protects a C-terminal truncated NR2B LIVBP-like domain (main band at ~30 kDa) against trypsin digestion. C, Ifenprodil (100 µM) does not protect the NR2A LIVBP-like domain (main band at ~40 kDa) against trypsin digestion. D, Zn (10 µM) protects the NR2A LIVBP-like domain against trypsin digestion.

Interestingly, we consistently observed an ifenprodil-induced protection of the minor band migrating at 30 kDa (Fig. 3A).We have obtained experimental evidence that this band is not abacterial contaminant but most probably represents a thrombin-truncatedproduct of the LIVBP-like domain (thrombin is used to cleave offthe GST). Indeed, we have expressed, refolded, and purified ashortened version of the NR2B LIVBP-like domain [in which Val²⁹³, the residue after a putative thrombin cleavage site (Arg²⁹²), has been replaced by a stop codon] and have obtained a highlypurified band, migrating at the expected molecular mass (~30 kDa)and very efficiently protected against proteolysis by ifenprodil(10 µM; n = 3) (Fig. 3B).

To eliminate the possibility that ifenprodil inhibits trypsin, we repeated the experiments on the isolated LIVBP-like domainof NR2A. As shown in Figure 3C, the rate of trypsin digestionof the NR2A domain is not affected by 100 µM ifenprodil, indicatingthat ifenprodil does not inhibit trypsin. Similar results wereobtained eight times [10 µM (n = 4) or 100 µM (n = 4) ifenprodil].In contrast, Zn (10 µM), a known ligand of the NR2A LIVBP-likedomain (Paoletti et al., 2000), is very efficient at protectingthe isolated domain of NR2A against trypsin digestion (n = 3)(Fig. 3D).

In conclusion, ifenprodil specifically protects the isolated LIVBP-like domain of NR2B against proteolysis. This implies thatthe NR2B LIVBP-like domain contains the ifenprodil bindingsite.

Identification of residues of the LIVBP-like domain of NR2B controlling the high-affinity ifenprodil inhibition

We searched for residues of the LIVBP-like domain of NR2B putatively involved in ifenprodil binding using site-directed mutagenesis.We had shown in our previous work on high-affinity Zn inhibitionthat the residues known (or proposed) to contact the ligand invarious LIVBP-like domains cluster in a few discrete homologousregions scattered throughout the sequence (Paoletti et al., 2000)(Fig. 4, shaded boxes). In LIVBP and LIVBP-like domains of known3D structure, these regions are mostly made of loops between secondarystructure elements (usually one $beta$ -strand followed by one $alpha$ -helix)and line a central cleft separating two globular subdomains (Quiochoand Ledvina, 1996; Kunishima et al., 2000). We used the sequencealignments between the bacterial protein LIVBP and the LIVBP-likedomains of the NR2 subunit that we had proposed previously (basedon the conservation of patterns of hydrophobic clusters; Paolettiet al., 2000) to delineate putative ligand-binding regions inthe LIVBP-like domain of NR2B (Fig. 4). We then performed pointmutagenesis targeted to these regions and assessed ifenprodilsensitivity of the NR2B mutated receptors. Given that ifenprodilbinding to NMDA receptors may involve a variety of interactions(electrostatic, hydrophobic, and hydrogen bonds; see Discussion),we did not restrict our mutagenesis to specific residues chosenfor their chemical properties but rather mutated into alanineeach residue of the studied regions (alanine scan).

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Figure 4. Ligand-contacting regions in proteins containing LIVBP-like domains. Amino acid sequence alignment of the LIVBP-like domains of the NMDA receptor subunits NR2A, NR2B, and NR1 and the LIVBP-like domains of known structures from LIVBP (Sack et al., 1989), mGluR1 (Kunishima et al., 2000), and ANP-C (He et al., 2001). For LIVBP (E. coli), mGluR1, and ANP-C, the alignments were obtained from structure superimposition; for NR2A and NR2B, the alignments were adapted from those of Paoletti et al. (2000); for NR1, the alignment was based on the conserved pattern of a cluster of hydrophobic residues within LIVBP-like domains (see Materials and Methods). The $beta$ strands (arrows) and $alpha$ helices (open bars) identified in LIVBP, mGluR1, and ANP-C crystal structures are indicated on top of the alignment. The insertions found in mGluR1 with respect to LIVBP are indicated by I1 (14 residues), I2 (31 residues), I3 (47 residues), and I4 (13 residues) and in ANP-C by I1 (21 residues). Shaded boxes indicate regions (mostly loops) known to contact the ligand molecules in LIVBP-like domains (adapted from Paoletti et al., 2000). Residues of NR2A controlling high-affinity Zn inhibition (see Paoletti et al., 2000) and residues of NR2B identified as controlling ifenprodil inhibition (present study) are highlighted. Residues of NR1 mutated by Masuko et al. (1999) and affecting ifenprodil inhibition are indicated by triangles. Residues of mGluR1 and ANP-C participating in dimerization of the LIVBP-like domains (Kunishima et al., 2000; He et al., 2001) are indicated by closed circles.

Mutants were screened by measuring the inhibition of agonist-induced current at two concentrations of ifenprodil: 300 nM,a concentration approximately twice the IC₅₀, and 3 µM, a nearlysaturating concentration for NR1/NR2B wt receptors. We arbitrarilyconsidered as "significant" (or "critical") those mutants thathad a current of >70% of the control at 300 nM ifenprodil (vs37% for wt NR2B receptors; Table 1). Of the 41 mutations tested(all of which gave functional receptors), we detected 13 mutationsresulting in a significant decrease in ifenprodil sensitivity(Table 1). Typical current traces are shown in Figure 5 for threedifferent mutated receptors and wt NR1/NR2B receptors. NR2B-V42Aexemplify mutant receptors with an ifenprodil inhibition clearlydecreased at 300 nM but still potent at 3 µM, whereas NR2B-D101Aand NR2B-F176A exemplify mutants with the strongest effects. Suchmutants receptor are almost insensitive to 300 nM ifenprodil andonly weakly affected by 3 µM ifenprodil.


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Table 1. Screening of point mutations in the LIVBP-like domain of NR2B for effects on ifenprodil sensitivity

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Figure 5. Identification in the LIVBP-like domain of NR2B critical residues controlling high-affinity ifenprodil inhibition. A comparison of the current traces obtained from oocytes coexpressing NR1 with either wt or mutated NR2B subunits is shown. Ifenprodil was applied at two increasing concentrations (300 nM and 3 µM) during an application of agonists. The bars above the current traces indicate the duration of agonists (agos) and ifenprodil (ifen) applications. The holding potential was $-$ 60 mV. These current traces are typical of NR2B mutants having an intermediate (V42A) or strong (D101A, F176A) effect on ifenprodil sensitivity.

Concentration-response curves of ifenprodil antagonism were constructed for each critical mutant (Fig. 6). Ifenprodil concentrationswere maintained at <10 µM to minimize the contribution of thelow-affinity voltage-dependent block (Fig. 2B). Critical mutantscan be subdivided into two groups according to the degree of reductionof ifenprodil sensitivity. One group includes the mutants V42A,T103A, D104A, E106A, T233A, K234A, E236A, L261A, and G264A, forwhich IC₅₀ values for ifenprodil are in the low micromolar range(4- to 25-fold higher than wt NR2B-containing receptors; Table2). The second group includes D101A, I150A, F176A, and F182A,the four mutants having the most pronounced effects on ifenprodilsensitivity. For these mutants, IC₅₀ values were estimated tobe >10 µM (>60-fold higher than for wt NR2B receptors; Table 2).In fact, substituting Asp¹⁰¹, Ile¹⁵⁰, Phe¹⁷⁶, and Phe¹⁸² into Ala is almost as effective in shifting the apparent ifenprodilsensitivity as replacing the entire LIVBP-like domain of NR2Bby that of NR2A. In that latter receptors, we have shown thatthe ifenprodil inhibition results mostly from ifenprodil bindinginto the pore (Fig. 2B2). A similar mechanism may account forpart of the residual ifenprodil inhibition observed with receptorsmutated at "critical" positions. Thus, with these mutants, thedecrease in affinity of the NR2B LIVBP-like domain for ifenprodilcould be significantly higher than the apparent 60-fold deducedfrom the concentration-response curves.

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Figure 6. Ifenprodil concentration-response curves of receptors mutated at critical residues. Each graph corresponds to a region in the LIVBP-like domain of NR2B in which one or more critical residues controlling ifenprodil inhibition were identified. The dotted curves are the fits of the ifenprodil concentration-response curves of the NR1/NR2B wt receptors (left dotted curve) and the chimeric NR1/NR2B-(LIVBP NR2A) receptors (right dotted curve) obtained in Figure 2B. The estimated values of IC₅₀ of the different mutated receptors are listed in Table 2. Estimated values of Hill coefficients (0.92-1.10) and maximal inhibitions (88-100%) are in the same range as those obtained with NR2B wt receptors (Fig. 2A). Each data point is the mean value obtained from 3 to 22 oocytes. The recordings were made at $-$ 60 mV.


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Table 2. Parameters of the ifenprodil inhibition of NMDA receptors mutated at critical NR2B residues

Mutations at critical positions suppress ifenprodil-induced protection of the isolated NR2B LIVBP-like domains against trypsin proteolysis

The results obtained above suggest that the critical residues identified in the NR2B LIVBP-like domain are closely associatedwith the ifenprodil binding site. We obtained an additional andindependent evidence showing that these residues are requiredfor high-affinity ifenprodil binding using the biochemical assayon isolated LIVBP-like domains. As illustrated in Figure 7, mutatingthe isolated LIVBP-like domain at the critical position Asp¹⁰¹ (Fig. 7A; n = 4) or Phe¹⁷⁶ (Fig. 7B; n = 4) abolishes the ifenprodil-induced protectionagainst proteolysis (compare with Fig. 3A).

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Figure 7. Lack of ifenprodil-induced protection against trypsin digestion of NR2B LIVBP-like domains mutated at critical positions. Point mutations (D101A and F176A) were introduced in the plasmid pGEX-2T-LIVBP NR2B and the mutated domains produced in E. coli. Protection by ifenprodil (10 µM) against trypsin digestion was tested using the protocol described in Figure 3. A, Mutation D101A. B, Mutation F176A.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

By combining a functional and biochemical approach on wild-type and mutated NMDA receptors, we show in the present work thatthe high-affinity binding site of ifenprodil is situated in theN-terminal LIVBP-like domain of the NR2B subunit. This domain,isolated from the rest of the receptor, is sufficient to forman ifenprodil binding site, and we have identified a number ofresidues in this domain that are closely associated with ifenprodilbinding.

An alanine mutagenesis scan in the NR2B LIVBP-like domain targeted to regions known to contain ligand-contacting residuesin other proteins with the LIVBP-like domain allowed the identificationof 13 residues (Table 1) likely to participate in the formationof the high-affinity ifenprodil binding site. These critical residuesare highly diverse in their chemical nature. As shown in Table2, their side chain can be either charged (Asp¹⁰¹, Asp¹⁰⁴, Glu¹⁰⁶, Lys²³⁴, and Glu²³⁶) or uncharged but polar (Thr¹⁰³ and Thr²³³), aliphatic (Val⁴², Ile¹⁵⁰, Leu²⁶¹, and Gly²⁶⁴), or aromatic (Phe¹⁷⁶ and Phe¹⁸²). Such a diversity is expected given the complex chemical natureof ifenprodil and the variety of interactions it may have withits receptor site. In a study investigating the structure-activityrelationships of a series of bis(phenylalkyl)amines (includingifenprodil) assayed for their potency as NR2B-selective antagonists,Tamiz et al. (1998) proposed that the binding site for NR2B-selective,ifenprodil-like antagonists is made of (at least) three majorsubsites or "pockets" (Chenard and Menniti, 1999): one hydrophobic,accommodating the phenyl ring; one interacting electrostaticallywith the central basic nitrogen atom; and one being both hydrophobicand a hydrogen bond acceptor and accommodating the phenol group.The optimum intramolecular distances between these subsites havebeen evaluated to ~8Å from the nitrogen atom to the phenolic hydroxylicgroup and ~10Å from the nitrogen binding site to the hydrophobicpocket interacting with the phenylring.

To evaluate whether the spatial distribution of the critical residues could match the proposed pharmacophore model, we constructeda 3D model of the NR2B LIVBP-like domain. The 3D structure ofthe LIVBP-like domain of NR2B was modeled by homology to the knownstructure of the unliganded form of LIVBP (Sack et al., 1989)on the basis of the sequence alignment shown in Figure 4 (seeMaterials and Methods). The modeled structure of the LIVBP-likedomain of NR2B consists of two globular lobes, each lobe beingmade of alternation of $beta$ strands and $alpha$ helices, interconnectedby a hinge made of three short linkers delineating a deep centralcleft (Fig. 8A). The critical residues all belong to regions liningthe central cleft, and most of them have their side chain projectingfrom both lobes into the cleft. This suggests that, as in thecase of Zn binding to the LIVBP-like domain of NR2A (Paolettiet al., 2000), ifenprodil binds in the cleft of the LIVBP-likedomain of NR2B and could promote its closure (Venus-flytrap mechanism).Thus, on ifenprodil binding, the critical residues may group accordingto the pharmacophore model presented above, with a central highlypolar and negatively charged cluster (made of residues from $beta$ 3/ $alpha$ 3and $beta$ 8/ $alpha$ 8 loops and interacting with the positively charged protonatednitrogen) surrounded by two hydrophobic clusters, one comprisingthe two aromatic Phe¹⁷⁶ and Phe¹⁸² together with Ile¹⁵⁰ (and interacting with the phenyl ring) and the other, less welldefined, made of Val⁴², Gly²⁶⁴, and Leu²⁶¹ (Fig. 8A). The estimated width of the modeled cleft (~25Å) issufficiently large to accommodate one molecule of ifenprodil.

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Figure 8. LIVBP-like domain of NR2 subunits as binding domains for extracellular modulators of NMDA receptor activity. A, 3D model of the LIVBP-like domain of NR2B and the putative ifenprodil binding site. This model was produced by homology modeling using the sequence alignment shown in Figure 4 and the Protein Data Bank coordinates of LIVBP (2LIV), the unliganded form of LIVBP (Sack et al., 1989). The residues identified as critical for high-affinity ifenprodil inhibition (numbered 1-13 for clarity) are displayed in the space fill representation and according to the following color code: Corey-Pauling-Koltun (CPK) for polar and charged residues (lobe I: Asp¹⁰¹₍₂₎, Thr¹⁰³₍₃₎, Asp¹⁰⁴₍₄₎, Glu¹⁰⁶₍₅₎; lobe II: Thr²³³₍₉₎, Lys²³⁴₍₁₀₎, Glu²³⁶₍₁₁₎), green for aliphatic residues (lobe I: Val⁴²₍₁₎; lobe II: Leu²⁶¹₍₁₂₎, Gly²⁶⁴₍₁₃₎; hinge: Ile¹⁵⁰₍₆₎), and yellow for aromatic residues (lobe II: Phe¹⁷⁶₍₇₎, Phe¹⁸²₍₈₎). On the right of the model is a space fill representation of the ifenprodil molecule (CPK color code). B, Functional organization of the extracellular regions of the NR2 subunits. See Discussion for more details.

In this putative ifenprodil binding site, some residues could contact ifenprodil through ligand-protein backbone interactions.This could be true for Gly²⁶⁴ and Leu²⁶¹, which in our model has its side chain buried in lobe 2. Somecritical residues may not contact ifenprodil directly but ratheract "downstream" of ifenprodil binding. This could be the casefor Ile¹⁵⁰, a residue localized in the hinge (linker $beta$ 5/ $alpha$ 5) between thetwo lobes. The mutation of this residue produces receptors withvery small currents (50-150 nA at $-$ 60 mV) and with a marked desensitization(data not shown). Thus, Ile¹⁵⁰ could participate in the mechanism of flytrap closure of thedomain rather than directly contact the ligand. Finally, one cannotexclude that there are other additional critical residues forifenprodilinhibition.

Despite the lack of direct proof that the critical residues do contact ifenprodil, both our functional and our biochemicalresults support the proposed model of ifenprodil binding withinthe cleft of the LIVBP-like domain of NR2B. In particular, thethree residues Asp¹⁰¹, Phe¹⁷⁶, and Phe¹⁸², the substitutions of which produce the largest effects on ifenprodilsensitivity (Fig. 6, Table 2) and suppress the ifenprodil-inducedprotection of the isolated NR2B LIVBP-like domain against proteolysis(Fig. 7; not tested for Phe¹⁸²), seem to be mandatory for high-affinity ifenprodil binding.The fact that these residues are present on both lobes (Asp¹⁰¹ on lobe 1 and Phe¹⁷⁶ and Phe¹⁸² on lobe 2) is an additional argument in favor of a Venus-flytraptype ofmechanism.

Although our results are fully consistent with the initial observation of Gallagher et al. (1996), that an N-terminal regionof NR2B controls the high-affinity ifenprodil inhibition, theyare in clear discrepancy with that of Masuko et al. (1999), whoproposed that the ifenprodil binding site resides in the LIVBP-likedomain of NR1. These authors based their conclusion on the factthat some mutations in the LIVBP-like domain of NR1 strongly affectifenprodil sensitivity of NR1/NR2B responses. However, the analysisof sequence alignments between NR1 and other LIVBP-like domainsfavors another interpretation. X-ray structures of homodimersof LIVBP-like domains have been obtained recently for two receptors,rat mGluR1 (Kunishima et al., 2000) and ANP-C (He et al., 2001),and in both receptors, the LIVBP-like domain (which forms theagonist-binding domain) dimerizes through a central interfacemade of highly hydrophobic residues (Fig. 4, filled circles).Strikingly, the residues of NR1 identified by Masuko et al. (1999)are also mostly hydrophobic (including three tyrosines and onephenylalanine) and align to positions homologous to those shownto participate in the dimer interface in mGluR1 and ANP-C (Fig.4, triangles). Therefore, even if we do not discount the possibilitythat a large molecule such as ifenprodil might contact residuesfrom both NR1 and NR2B, we propose that the critical residuesidentified on NR1, rather than being directly involved in contactingifenprodil, form an interface between two LIVBP-like domains (eitherNR1/NR1 or NR1/NR2B). As demonstrated for the activation mechanismof mGluR1 (Kunishima et al., 2000), a rotation of this intersubunitdimer interface might be fundamental in transferring to the gatingmachinery the ifenprodil-induced conformational change in theNR2B LIVBP-likedomain.

The present results reinforce our proposal that LIVBP-like domains of NMDA receptors, and possibly of other eukaryotic iGluRs,bind modulatory ligands (Paoletti et al., 2000). Moreover, theresults also strengthen the hypothesis of a modular architectureof iGluR subunits, with an extracellular region made of a tandemof functionally specialized Venus-flytrap domains, one (GlnBP-like)binding the agonist (glutamate for all iGluR subunits except NR1,which binds glycine) and the other (LIVBP-like) binding a modulatoryligand (Zn for NR2A and ifenprodil for NR2B) (Fig. 8B). This latterproposal is particularly well supported by the finding that domainsseparated from the rest of the receptor retain their ligand-bindingproperties (for the GlnBP-like domain; see Kuusinen et al., 1995;present study for the LIVBP-like domains). In NMDA receptors,it has been shown recently that during gating, both domains, theLIVBP- and GlnBP-like, functionally interact to produce one formof receptor desensitization (Krupp et al., 1998; Villarroel etal., 1998; Zheng et al., 2001). This interaction might be a commonmechanistic feature of iGluRs, stressing the need for additionalstudies aimed at identifying the interdomain contacts as wellas their connection to the channelgate.

Finally, our results identify the LIVBP-like domain of the NR2B subunit as a new target for neuroprotective and analgesicagents. This target has a particularly attractive neuropharmacologicalprofile. First, it is selective of a subpopulation of NMDA receptors(those containing NR2B subunits), thus reducing the unacceptableside effects usually associated with broad-spectrum NMDA antagonists.Second, the blockers will be most efficient at high levels ofglutamate (because of the use dependency; Kew et al., 1996) andat low pH (because of the strong pH dependency; Mott et al., 1998),and they will be still potent at depolarized potentials (becauseof the voltage independence; Williams, 1993), all conditions oftenencountered in pathological situations such as stroke, seizures,and pain states. It has been shown on the GlnBP-like domain thatthe efficacy of different agonists is directly related to thedegree of cleft closure that they induce: the more the domaincloses on agonist binding, the more efficient the agonist (Armstrongand Gouaux, 2000). Similarly, if ifenprodil binding were to promotethe closure of the NR2B LIVBP-like domain (which remains to beproved), inhibition of channel activity could be directly relatedto the degree of lobe separation in this domain. One could thenimagine NR2B-selective inhibitors with different potency accordingto the level of domain closure they produce. In that respect,a partial antagonist (inducing an intermediate level of domainclosure) would be an attractive drug, because it would both maintaina persistent level of NMDA receptor activity even at saturatingconcentrations and allow chronic treatment with reduced side effects.Our results provide a structural framework for designing suchnew neuroprotectiveagents.

  FOOTNOTES

Received Feb. 27, 2002; revised May 6, 2002; accepted May 7, 2002.

This work was supported by Assistance Publique des Hôpitaux de Paris (F.P.D.), Ministère de la Recherche (J.R.), and InstitutNational de la Santé et de la Recherche Médicale (P.P.). Weare most grateful to Roderick MacKinnon and members of his laboratorywho helped much in starting the biochemical approach. We thankPhilippe Ascher and Roderick MacKinnon for comments on this manuscript.We also thank Sanofi-Synthélabo for the gift ofifenprodil.

Correspondence should be addressed to Dr. Pierre Paoletti, Laboratoire de Neurobiologie, Ecole Normale Supérieure, 46 rued'Ulm, 75005 Paris, France. E-mail: paoletti{at}biologie.ens.fr.

  REFERENCES

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MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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