(R,S)-4-Phosphonophenylglycine, a Potent and Selective Group III Metabotropic Glutamate Receptor Agonist, Is Anticonvulsive and Neuroprotective In Vivo

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Gasparini, F.
	Articles by Flor, P. J.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Gasparini, F.
	Articles by Flor, P. J.

Vol. 289, Issue 3, 1678-1687, June 1999

(R,S)-4-Phosphonophenylglycine, a Potent and Selective Group III Metabotropic Glutamate Receptor Agonist, Is Anticonvulsive and Neuroprotective In Vivo

F. Gasparini, V. Bruno, G. Battaglia, S. Lukic, T. Leonhardt, W. Inderbitzin, D. Laurie, B. Sommer, M. A. Varney, S. D. Hess, E. C. Johnson, R. Kuhn, S. Urwyler, D. Sauer, C. Portet, M. Schmutz, F. Nicoletti and P. J. Flor

Novartis Pharma AG, Nervous System Research, Basel, Switzerland (F.G., S.L., T.L., W.I., D.L., B.S., R.K., S.U., D.S., C.P., M.S., P.J.F.); Istituto Mediterraneo di Neuroscienze "Neuromed," Pozzilli, Italy (V.B., G.B., F.N.); SIBIA Neurosciences Incorporated, La Jolla, California (M.A.V., S.D.H., E.C.J.); and University of Catania, Catania, Italy (F.N.)

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

Group III metabotropic glutamate receptors (mGluRs) are thought to modulate neurotoxicity of excitatory amino acids, via mechanismsof presynaptic inhibition, such as regulation of neurotransmitterrelease. Here, we describe (R,S)-4-phosphonophenylglycine (PPG)as a novel, potent, and selective agonist for group III mGluRs.In recombinant cell lines expressing the human receptors hmGluR4a,hmGluR6, hmGluR7b, or hmGluR8a, EC₅₀ values for (R,S)-PPG of 5.2± 0.7 µM, 4.7 ± 0.9 µM, 185 ± 42 µM, and 0.2 ± 0.1 µM, respectively,were measured. The compound showed EC₅₀ and IC₅₀ values of $>=$ 200µM at group I and II hmGluRs and was inactive at cloned humanN-methyl-D-aspartate, $alpha$ -amino-3-hydroxy-5-methyl-isoxazole-4-propionate,and kainate receptors (>300 µM). On the other hand, it showedmicromolar affinity for a Ca²⁺/Cl-dependent L-glutamate binding site in rat brain, similar to otherphosphono-substituted amino acids like L-2-amino-4-phosphonobutyrate.In cultured cortical neurons, (R,S)-PPG provided protection againsta toxic pulse of N-methyl-D-aspartate (EC₅₀ = 12 µM), which wasreversed by the group III mGluR antagonist (R,S)- $alpha$ -methylserine-O-phosphatebut not by the group II antagonist (2S)- $alpha$ -ethylglutamate. Moreover,(R,S)-PPG protected against N-methyl-D-aspartate- and quinolinicacid-induced striatal lesions in rats and was anticonvulsive inthe maximal electroshock model in mice. In contrast to the groupIII mGluR agonists L-2-amino-4-phosphonobutyrate and L-serine-O-phosphate,(R,S)-PPG showed no proconvulsive effects (2200 nmol i.c.v.).These data provide novel in vivo evidence for group III mGluRsas attractive targets for neuroprotective and anticonvulsive therapy.Also, (R,S)-PPG represents an attractive tool to analyze the rolesof group III mGluRs in nervous system physiology andpathology.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

The neurotoxicity of excitatory amino acids such as L-glutamate and some of its analogs, e.g., kainate and N-methyl-D-asparticacid (NMDA), is well established in the central nervous system(Lipton and Rosenberg, 1994). Analogs of L-glutamate, which havebeen investigated in neural systems, share with their parent compoundthe $alpha$ -amino acid moiety and a distal, negatively ionizable group(Watkins et al., 1990). These structural features are consideredessential for L-glutamate to interact with each member of itslarge family of ionotropic and metabotropic neurotransmitter receptors(Hollmann and Heinemann, 1994).

In an effort to discover new agents interfering with the glutamatergic system, a large panel of phosphono-substituted $alpha$ -aminoacid derivatives has been generated. D-2-amino-5-phosphonopentanoicacid (D-AP5), D-(E)-2-amino-4-methyl-5-phosphono-3-pentenoic acid(CGP 40116; Fig. 1), D-(E)-4-(3-phosphonoprop-2-enyl)piperazine-2-carboxylicacid (D-CPPene), and 2-amino-3-(2'-chloro-5-phosphonomethyl-biphenyl-3-yl)-propionicacid) (SDZ 220-581), for instance, are potent, selective, andcompetitive antagonists for NMDA receptors, which constitute onepharmacological group within the class of ionotropic glutamatereceptors (iGluRs). Those and many related compounds served astools to elucidate the role of NMDA receptors in brain disorders,such as neurodegenerative processes following ischemia and epilepticseizures (Sauer et al., 1992; Urwyler et al., 1996a). On the otherhand, many phosphono-substituted $alpha$ -amino acids, like L-2-amino-4-phosphonobutyrate(L-AP4), L-serine-O-phosphate (L-SOP), and 4-phosphono-phenylglycine[(R,S)-PPG; Bigge et al., 1989], were found to be inactive asNMDA receptor ligands.

View larger version (15K):
[in this window]
[in a new window]

Fig. 1. Chemical structures of phosphono-amino acid derivatives. (R,S)-PPG, D-(E)-2-amino-4-methyl-5-phosphono-3-pentenoic acid (CGP 40116), and two reference agonists for group III mGluRs, L-AP4 and L-SOP, are depicted. The carbon atom backbone of each structure is numbered in italics. All four compounds contain the amino acid function and a distal phosphonic acid. CGP 40116, a classical competitive NMDA receptor antagonist, and (R,S)-PPG have a considerably larger distance between the two acidic groups than the glutamic acid analogs L-AP4 and L-SOP.

L-AP4 and L-SOP, however, are potent and selective agonists at a group of metabotropic glutamate receptors (mGluRs). EightmGluR subtypes are currently known, which are numbered accordingto the order of their molecular discovery, and are subdividedinto three distinct groups (Tanabe et al., 1992; Conn and Pin,1997). Group I mGluRs (mGluR1 and mGluR5) are positively coupledto the phosphoinositide/Ca²⁺ cascade. Group II (mGluR2 and mGluR3) and group III (mGluR4,mGluR6, mGluR7, and mGluR8) receptors are both negatively coupledto adenylate cyclase in heterologous expression assays. The threegroups can be discriminated pharmacologically with the use ofselective agonists. 3,5-Dihydroxyphenylglycine selectively activatesgroup I mGluRs, whereas 2R,4R-aminopyrrolidine-2,4-dicarboxylateand LY-354740 are examples for group II selective agonists (Connand Pin, 1997; Monn et al., 1997). L-AP4, L-SOP, and close analogsare the only selective agonists known for group III mGluRs, withlow micromolar potency (EC₅₀ values, 0.1-7 µM) at mGluR4, mGluR6,and mGluR8; mGluR7 can only be activated at concentrations higherthan 100 µM (Okamoto et al., 1994; Johansen et al., 1995; Connand Pin, 1997; Flor et al., 1997). Group III (and group II) mGluRsare thought to mediate presynaptic depression of glutamatergicsynaptic potentials in several brain areas, most likely via inhibitionof voltage-gated calcium entry and regulation of glutamate release(Trombley and Westbrook, 1992; Conn and Pin, 1997). Moreover,selective activation of group III mGluRs results in neuroprotectionin vitro; agonists like L-AP4 and L-SOP promote survival of ratcerebellar granule cells and protect cultured cortical and cerebellarneurons against toxic insults, such as prolonged $beta$ -amyloid peptideexposure, transient iGluR activation, or mechanical damage (Grahamand Burgoyne, 1994; Copani et al., 1995; Bruno et al., 1996; Fadenet al., 1997). In contrast to the findings with NMDA receptorantagonists, in vivo neuroprotection with group III mGluR agonistshas not yet been reported to ourknowledge.

Both, proconvulsive and anticonvulsive effects of group III mGluR agonists have been observed, depending not only on the animalmodel used but also on timing and dosage of the drug treatment(e.g., Graham and Burgoyne, 1994; Abdul-Ghani et al., 1997; Ghauriet al., 1996; Tang et al., 1997).

Here, we report in vitro and in vivo neuroprotective actions of (R,S)-PPG, a compound with structural similarity to competitiveNMDA receptor antagonists and group III mGluR agonists (Fig. 1).(R,S)-PPG was also tested for anticonvulsive properties in themaximal electroshock-induced convulsion model in mice, in comparisonwith L-AP4 and L-SOP. In an effort to characterize activity andselectivity of (R,S)-PPG at the molecular level, the compoundwas tested for interaction with all eight mGluR subtypes, witha representative selection of recombinant human iGluRs and witha Ca²⁺/Cl-dependent L-glutamate binding site of rat brain. Group III mGluRsas attractive drug targets for the treatment of neurological disorders,such as epilepsy and Huntington's disease, will bediscussed.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Chemical Synthesis of (R,S)-PPG. (R,S)-PPG was synthetized in four steps starting from 4-hydroxybenzaldehyde using a different synthetic pathway than the onedescribed (Bigge et al., 1989). The starting material was firstesterified with trifluoromethanesulfonicanhydride. The trifluoromethanesulfonateester was then converted to the corresponding phosphonate esterusing a palladium-catalyzed coupling. Conversion of the aldehydeto the amino nitrile and subsequent hydrolysis performed in concentratedHCl gave (R,S)-PPG with an overall yield of about 30%. Furtherdetails of the synthesis will be publishedelsewhere.

Cloning of hmGluR8a cDNA. The sequence encoding the human metabotropic glutamate receptor subtype 8a (hmGluR8a) was constructed from clones obtainedby library screening in combination with polymerase chain reaction(PCR).

Library Screening. Five × 10⁵ plaques each of two human cDNA libraries from whole adult brain (in $lambda$ gt10; Clontech, Palo Alto, CA) and adult hippocampus(in $lambda$ ZAPII; Stratagene, Heidelberg, Germany) were screened with5' and 3' probes from the rat mGluR4 sequence (Tanabe et al.,1992) as described previously (Laurie et al., 1997). After a secondround of screening, individual cDNA inserts were rescued intoBluescript SK( $-$ ) phagemids (Stratagene) by in vitro ( $lambda$ gt10) orin vivo ( $lambda$ ZAPII) excision. cDNA inserts were characterized byrestriction enzyme mapping and DNA sequencing (ABI systems, Langen,Germany). Two nonoverlapping clones were identified as homologousto portions of the mouse mGluR8 sequence (Duvoisin et al., 1995):HMGBr7 (homologous to bases 576-799 of mouse mGluR8) and HMGHi7(homologous to bases 2059-2830 of mousemGluR8).

PCR. The 5' end of the hmGluR8 coding sequence was amplified from human retinal cDNA. Thermocycling conditions were: 94°C for 1min, 45°C for 1 min, 72°C for 1 min, 10 cycles, then 94°C for30 s, 55°C for 30 s, 72°C for 1 min, 38 cycles, using "Expand-HighFidelity" polymerase (Boehringer Mannheim, Mannheim, Germany).PCR oligos were 5'-GTCGCTGACTGCAATACCACCTGCGGAGAAAATG-3' [senseoligo from mouse mGluR8 sequence (Duvoisin et al., 1995); translationinitiation codon underlined] and 5'-CAACTATCTGAGCCAATCCAG-3'.The resultant 900-bp amplicon, "PCR5p8," was subcloned into thePCR cloning vector pCRII (Invitrogen, San Diego,CA).

The missing sequence between clones HMGBr7 and HMGHi7 was obtained by PCR from human retinal cDNA, and the resultant 1570-bpamplicon was also subcloned into the vector pCRII. Thermocyclingconditions were 94°C for 1 min, 60°C for 1 min, 72°C for 2 min,38 cycles, using Expand-High Fidelity polymerase (Boehringer Mannheim).PCR oligos were 5'-GACTCCTACCAAGCCCAAGCCATG-3' and 5'-CGCTGCTCTCCATAGTCAATGATG-3'.This intervening sequence, "PCRint8", was digested into threefragments with BamHI and the largest (1214-bp) fragment, "3'PCRint8"ligated to HMGHi7 by a common BamHI site, forming 3'PCRint8-HMGHi7.A parallel digest of PCRint8 with MunI released the 420-bp fragment"5'PCRint8".

The full-length hmGluR8a sequence was constructed by ligating 3'PCRint8-HMGHi7 to 5'PCRint8 via a common MunI site, ligatingthe product to PCR5p8 via an NcoI site and finally ligating thewhole sequence into the expression vector pCIneo (Clontech) usingXbaI and SalI sites. The coding region of the assembled hmGluR8aclone (hmGluR8a.pCIneo) was sequenced on both strands. In comparisonwith the very recently published hmGluR8a sequence (Wu et al.,1998

), we find only one amino acid difference: Asp-768 to Ile,which is encoded by the library-derived cloneHMGHi7.

Stable Expression of hmGluR8a in HEK293 Cells. The construct hmGluR8a.pCIneo was linearized by digestion with Asp-700. One microgram of the linearized DNA was used to transfect10⁷ HEK293 cells. Selection for stable integration was made by additionof 0.8 mg/ml G418 (Life Technologies, Basel, Switzerland) to themedium (minimal essential medium with 2 mM L-glutamine supplementedwith 10% dialyzed fetal calf serum; Life Technologies), and 30G418-resistant clonal cell lines were isolated as described previously(Laurie et al., 1995). Further selection was performed by measuringthe glutamate (0.1 mM)-induced depression of forskolin (10 µM)-elevatedcAMP accumulation in cells grown in collagen-coated wells. Responsesranged from no depression to about 85% depression. Using thisapproach, two cell lines, HEK-hmGluR8a-2 and HEK-hmGluR8a-20,were identified as giving consistently good responses for up toat least 20 passages ofsubculturing.

Stable Mammalian Cell Lines for Cloned mGluR1 to mGluR7 and Ionotropic Glutamate Receptors. Generation, culture, and pharmacological characterization of stable cell lines for hmGluR1b, -2, -4a, -5a, -6, -7b, rat mGluR3,hNMDAR1A/2A, hNMDAR1A/2B, hGluR3i, and hGluR6 have been describedrecently (Knöpfel et al., 1995; Laurie et al., 1995, 1997; Daggettet al., 1996; Varney et al., 1996, 1998; Flor et al., 1997 andreferences therein; Lin et al., 1997).

In Vitro Pharmacological Assays for Cloned Glutamate Receptors. Measurements of cyclic AMP accumulation (Flor et al., 1997), inositol monophosphate formation (Knöpfel et al., 1995), andcytoplasmic calcium elevation (Flor et al., 1996) were performedas describedpreviously.

L-[³H]Glutamate-Binding Assay for mGluR3. HEK293 cells stably transfected with the cDNA encoding rat mGluR3 were cultured and harvested as described previously (Laurieet al., 1995). Membranes from these cells were washed by fivecycles of centrifugation (10 min at 50,000g, 4°C) and resuspensionin assay buffer before being frozen and stored at $-$ 80°C untiltheir use in the binding experiments. After thawing, membraneswere washed five times by centrifugation and resuspension in ice-coldassay buffer as above. The L-[³H]glutamate-binding assay was performed in 0.6 ml of 50 mM Tris-HClbuffer (pH 7.5 at 0°C) containing an aliquot of the membrane suspension(about 50 µg of protein), 5 nM L-[³H]glutamate (NEN, Regensdorf, Switzerland), 2.5 mM CaCl₂, andthe test compounds at the appropriate concentrations. Nonspecificbinding was determined by including 0.5 mM unlabeled L-glutamate.The samples were incubated at 0°C for 4 h before bound and freeradioligand were separated by centrifugation at 4°C for 20 minat approximately 10,000g. The supernatant was decanted, and thepellets were quickly and superficially rinsed with ice-cold assaybuffer and then added to scintillation fluid containing tissuesolubilizer (Solvable; NEN). After solubilization at 50°C overnight,the radioactivity was measured by liquid scintillation counting.Competition curves were analyzed, and IC₅₀ values were determinedby nonlinear curve fitting using the program GraphPad Prism (GraphPadSoftware, Inc., San Diego,CA).

Ca²⁺/Cl-Dependent L-[³H]Glutamate Binding to Rat Brain Membranes. This assay was essentially performed as described previously (Urwyler et al., 1996b). In brief, the assay mixture (in a finalvolume of 1.1 ml) contained 50 mM Tris-HCl (pH 7.4), 2.5 mM CaCl₂,extensively washed rat hippocampal membranes (freshly preparedon the day of the experiment) corresponding to approximately 3mg of original tissue (wet weight), 5 nM L-[³H]glutamate, and the test compounds at the desired concentrations.Nonspecific binding was defined with 0.2 mM DL-AP7. The sampleswere incubated for 25 min at 37°C before bound and free radioligandwere separated by centrifugation at 12,000g for 4 min. The pelletswere quickly and superficially rinsed with 100 µl of ice-coldincubation buffer and then added to scintillation fluid containingtissue solubilizer (Solvable; NEN). After solubilization at 50°Covernight, the radioactivity was measured by liquid scintillationcounting.

Preparation of Cultured Cortical Cells and Examination of NMDA Toxicity. Mixed cultures of cortical cells were prepared from fetal mice (14-16 days of gestation), as described (Bruno et al., 1996),and used 13 to 14 days after plating. Cultures were exposed to100 µM NMDA for 10 min at room temperature in a HEPES-bufferedsalt solution. After extensive washing, cultures were incubatedfor 18 to 24 h at 37°C in minimal essential medium-Eagle's buffer(Life Technologies) supplemented with 25 mM NaHCO₃ and 21 mM glucose.Neuronal toxicity was examined by phase-contrast microscopy andquantitated after staining with trypan blue. Stained neuroneswere counted from three random fields per well. Lactate dehydrogenaserelease into the medium was also measured as described previously(Bruno et al., 1996).

Examination of Neuronal Toxicity after Intrastriatal Infusion with NMDA and Quinolinic Acid. Male Sprague-Dawley rats (250-300 g) were anesthetized with pentobarbital (50 mg/kg, i.p.) and infused with NMDA (100 nmol/0.5µl/2 min) or NMDA + group III mGluR agonists (balanced to neutralpH) in the left caudate nucleus, at +2.0 mm AP, 2.6 mm L, and5 mm V, according to the Pellegrino and Cushman atlas. The injectionwas repeated at a second site (1 mm posterior to the first site)to increase the extent of striatal toxicity. Seven days later,animals were sacrificed, and neuronal damage was assessed by eitherhistological analysis or measurements of striatal glutamate decarboxylase(GAD) activity. For histological analysis, the brains were rapidlyfrozen in isopentane at $-$ 40°C and then stored at 0°C. Twenty-micrometercryostat sections were Nissl-stained and examined in light microscopy.For measurements of GAD activity, the corpus striatum was dissectedbilaterally and homogenized in 5 mM imidazol buffer containing0.2% Triton X-100 and 10 mM dithiothreitol. An aliquot of thehomogenate was incubated in 400 µl of 10 mM phosphate buffer (pH7.0) containing 10 mM 2-mercaptoethanol, 0.02 mM pyridoxalphosphate,and 1 µCi of L-[³H]glutamate (Amersham Intl., Buckinghamshire, UK; specific activity46 Ci/mmol) for 1 h at 37°C; the reaction was stopped with 15µl of ice-cold 11.8 N HClO₄. After centrifugation in a microfugeat maximal speed, 10 µl of the supernatant were diluted with 0.01N HCl and derivatized with O-phtalaldehyde and mercaptoethanolfor 1 min at room temperature before injection into HPLC. TheHPLC apparatus consisted of a programmable solvent module 126(Beckman Instruments, Inc., Fullerton, CA), an analytical C₁₈reversed-phase column kept at 30°C (Ultrasphere ODS 5 µm spherical,80 Å pore, 2 mm × 15 cm; Beckman Instruments Inc.), and an RF-551spectrofluorimetric detector (Shimadzu Corp., Tokyo, Japan). Excitationand emission were set at 360 and 450 nm, respectively. The mobilephase consisted of 50 mM sodium phosphate, 10% methanol, pH 7.2(A), and 50 mM sodium phosphate, 70% methanol, pH 7.2 (B). After8 min of isocratic conditions with 98% (A) and 2% (B), (B) wasincreased up to 40% within 30 min and then to 98% within 1 minand then maintained at 98% for 11 min before returning to theinitial conditions. The radioactivity coeluting with $gamma$ -aminobutyricacid (GABA) was collected and counted by scintillation spectrometry.Protein concentrations in the original samples were determinedby using a commercially available kit (Bio-Rad, Richmond,CA).

Intrastriatal injection of quinolinic acid and evaluation of excitotoxic neurodegeneration by magnetic resonance imaging wasperformed as previously described (Sauer et al., 1992

Maximal Electroshock Test (MES). Experiments were conducted on 19- to 25-g male mice [Tif:MAGf (SpF)] at 21-22°C. Generalized tonic-clonic convulsions of thehind extremities were induced by passing alternating electricalcurrents of 50 Hz and 18 mA through corneal electrodes (for reference,see Kupferberg and Schmutz, 1997). L-AP4, L-SOP, and (R,S)-PPGwere dissolved in 0.9% saline, the pH corrected to 7.0 and administeredi.c.v., i.p., or i.v. with pretreatment times of 15 or 30 min.Five to 10 animals per dose were used; ED₅₀ values were calculatedon the basis of at least five doses, and each experiment was doneat least twice. The number of animals protected from tonic hindlimb extension seizure and the duration of hind limb tonus weredetermined in each dosegroup.

Statistics. Significant differences were estimated using the two-tailed Dunnett's t test by comparing test-drug groups with the controlgroup. Values of 2P < 0.05 were considered as statisticallysignificant.

Materials. Molecular biology reagents and enzymes were purchased from Amersham, Bio-Rad, Boehringer Mannheim, Invitrogen, New EnglandBiolabs, and Stratagene. Tissue culture reagents were from LifeTechnologies and Sigma. Forskolin, 3-isobutyl-1-methylxanthine,and L-SOP were obtained from Sigma. All other reference agonistsand antagonists were purchased from Tocris (Anawa Trading SA,Zürich, Switzerland). CGP 40116 was synthesized within NovartisPharma AG by Dr. Roland Heckendorn. All other chemicals were ofreagent grade and were obtained from Fluka (Buchs, Switzerland),Merck (Darmstadt, Germany), Serva (Heidelberg, Germany), orSigma.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Profiling of (R,S)-PPG against All Eight Cloned mGluR Subtypes. As shown in Fig. 2, (R,S)-PPG most potently inhibited forskolin-stimulated cAMP accumulation in recombinant cells stably expressinghmGluR8a, producing 70 to 80% inhibition at a maximally effectiveconcentration of 100 µM and an EC₅₀ value of 0.2 ± 0.1 µM (mean± S.E.M.). Concentration-response curves for agonist activityat the other known group III mGluR subtypes were measured, andEC₅₀ values of 5.2 ± 0.7 µM, 4.7 ± 0.9 µM, and 185 ± 42 µM (means± S.E.M.) were found for hmGluR4a, hmGluR6, and hmGluR7b, respectively(Fig. 2; Table 1). In contrast, (R,S)-PPG showed no significantinhibition of forskolin-stimulated cAMP accumulation in untransfectedCHO-K1 and HEK293 cells when tested at 300 µM and 100 µM, respectively(not shown). Different extents of maximal inhibition of cAMP formationby (R,S)-PPG were observed in the four cell lines expressing recombinantgroup III mGluRs, ranging from 45 to 80% inhibition. The Hillcoefficients for the interaction of (R,S)-PPG with the four groupIII mGluRs were between 1.5 and 2.5 (Table 1).

View larger version (20K):
[in this window]
[in a new window]

Fig. 2. Agonist activity of (R,S)-PPG at group III hmGluRs. Concentration-response curves for inhibition of forskolin (10 µM)-stimulated cAMP accumulation by (R,S)-PPG at CHO cells expressing hmGluR4a, hmGluR6, and hmGluR7b as well as HEK cells expressing hmGluR8a. Each data point represents mean value ± S.E.M. from at least three independent experiments (n $>=$ 6). Sigmoidal curves were fit using the GraphPad Prism program (GraphPad Software, Inc., San Diego, CA).

View this table:
[in this window]
[in a new window]

TABLE 1
Activity of (R,S)-PPG on metabotropic and ionotropic glutamate receptors expressed in recombinant mammalian cells
Concentration-response curve fitting and statistical analysis were done using the GraphPad Prism program (GraphPad Software, Inc.). EC₅₀ values are given ± S.E.M. (n $>=$ 3); n_H, Hill coefficient.

To address specificity of (R,S)-PPG, the compound was tested for agonist and antagonist activity at all known group I, II,and III mGluR subtypes. In recombinant cells expressing hmGluR1bor hmGluR5a, quisqualate produced 5- to 15-fold stimulation ofphosphoinositide hydrolysis at concentrations of 20 µM and 0.3µM, which are approximate EC₈₀ concentrations for these two clonallines. (R,S)-PPG, tested at 500 µM, neither stimulated phosphoinositidehydrolysis on its own nor reversed the quisqualate effects ineither hmGluR1b- or hmGluR5a-expressing cells (Fig. 3A). Moreover,at concentrations of 10 µM and 100 µM, (R,S)-PPG was also foundinactive at hmGluR1b and hmGluR5a (data not shown).

View larger version (35K):
[in this window]
[in a new window]

Fig. 3. Activity of (R,S)-PPG at group I, II, and III hmGluRs. A, inositol monophosphate formation of CHO cells expressing hmGluR1b and Ltk cells expressing hmGluR5a. Exposure to buffer was taken as control and set to 1.0; for submaximal and maximal stimulation of hmGluR1b, 20 µM quisqualate and 1000 µM quisqualate were used, respectively; 0.3 µM quisqualate gave submaximal stimulation of hmGluR5a, and 10 µM quisqualate showed the maximal effect. To test for agonist activity at group I mGluRs, (R,S)-PPG was applied at 500 µM to CHO-hmGluR1b and Ltk-hmGluR5a cells. Antagonist activity of 500 µM (R,S)-PPG at hmGluR1b and hmGluR5a was determined by coapplication of the submaximal concentrations of quisqualate (around EC₈₀). Mean values ± S.E.M. from at least two independent experiments are shown (n $>=$ 4). B, inhibition of forskolin-stimulated cAMP accumulation in CHO cells expressing either hmGluR2 or hmGluR4a. Forskolin (10 µM) stimulated cAMP formation about 40-fold (taken as control). All values are given as fraction of control. The effect of forskolin is inhibited by 30 µM (1S,3R)-ACPD in hmGluR2-expressing cells and by 1 µM L-AP4 in hmGluR4a-expressing cells. These submaximal agonist concentrations represent approximately EC₈₀. To test for agonist activity, (R,S)-PPG was applied to forskolin-stimulated CHO-hmGluR2 and CHO-hmGluR4a cells. Antagonist activity of (R,S)-PPG at hmGluR2 and hmGluR4a was determined by coapplication of submaximal concentrations of (1S,3R)-ACPD and L-AP4, respectively. Columns represent mean values ± S.E.M. of at least two independent experiments (n $>=$ 5). Asterisks indicate statistically significant antagonism or agonist activity of (R,S)-PPG (2P < .01; Dunnett's t test). C, inhibition of forskolin (10 µM)-stimulated cAMP accumulation in CHO cells expressing hmGluR7b and HEK cells expressing hmGluR8a. Forskolin-stimulated cAMP formation was taken as control. To obtain submaximal depression of the forskolin-stimulated cAMP accumulation, 500 µM L-AP4 and 1 µM L-AP4 were used for hmGluR7b and hmGluR8a, respectively (this represents about EC₈₀). (R,S)-PPG was tested for agonist activity as well as antagonist activity of submaximal L-AP4. Asterisks indicate statistically significant agonist activity of (R,S)-PPG (2P < .01; Dunnett's t test, n $>=$ 4).

In Chinese hamster ovary (CHO) cells stably expressing hmGluR2, 1-aminocyclopentane-1S,3R-dicarboxylic acid [(1S,3R)-ACPD],at 30 µM, depressed forskolin-stimulated cAMP accumulation byapproximately 65%, which represents about 80% of the maximal response(Fig. 3B). Five hundred micromolar (R,S)-PPG showed no significantdepression of cAMP when applied alone but showed 52% reversalof cAMP depression when coapplied with 30 µM (1S,3R)-ACPD (Fig.3B), indicating antagonist activity at hmGluR2. At 300 µM, theantagonist activity of (R,S)-PPG was reduced to 45%; at 100 µM,no significant antagonist activity of (R,S)-PPG at hmGluR2 wasobserved (2P > .05, Dunnett's t test, n = 8). At recombinant ratmGluR3 expressed in human embryonic kidney (HEK) cells, (R,S)-PPGas well as L-AP4 had only very weak affinity in an L-[³H]glutamate binding assay. (R,S)-PPG, L-AP4, and L-glutamate showedaround 50% inhibition of L-[³H]glutamate binding at 200 µM, 300 µM, and 200 nM, respectively(data notshown).

As shown in Fig. 3, B and C, and Table 1, inhibition of forskolin-stimulated cAMP formation in recombinant cells expressinghmGluR4a, hmGluR6, hmGluR7b, or hmGluR8a by (R,S)-PPG was at leastas efficacious as with L-AP4, applied at EC₈₀. Coapplication ofL-AP4 and (R,S)-PPG (300 or 1000 µM) did not reverse the L-AP4response.

Characterization of (R,S)-PPG at Ionotropic Glutamate Receptors. (R,S)-PPG was originally designed and characterized for NMDA-receptor binding (Bigge et al., 1989). However, the compoundwas found to be inactive up to 100 µM in the [³H]-3-(2-carboxypiperazin-4-yl)-propyl-1-phosphoric acid receptorbinding assay on rat cortical brain membranes, indicating that(R,S)-PPG does not bind to the L-glutamate site of native ratNMDA receptors. Here, we extend the characterization by employingstable cell lines transfected with the hNMDAR1A/2B subunit combination(Varney et al., 1996) to address functional agonist and antagonistactivity of (R,S)-PPG at cloned human NMDA receptors. In thiscell line, L-glutamate (applied at 1 µM) induced a rise in intracellularcalcium concentration. (R,S)-PPG neither induced a calcium risewhen applied at 300 µM nor antagonized the L-glutamate-inducedcalcium signal (Fig. 4). In contrast, the competitive NMDA-receptorantagonist CGP 40116 concentration-dependently prevented the L-glutamate-evokedrise in intracellular calcium (Fig. 4). Similar lack of activityof 300 µM (R,S)-PPG was observed in calcium assays for clonedhNMDAR1A/2A (data not shown, Table 1).

View larger version (27K):
[in this window]
[in a new window]

Fig. 4. Lack of activity at NMDA-type ionotropic glutamate receptors by (R,S)-PPG. Elevation of cytoplasmic calcium ion concentrations, [Ca²⁺]_i, in Ltk cells expressing cloned human NMDA receptors (subunit combination 1A/2B). A, increase in the fluorescent response ratio F₃₄₀/F₃₈₀ corresponds to an elevation in [Ca²⁺]_i. Three single calcium measurements are shown: application of 1 µM L-glutamate (L-Glu) alone, coapplication of L-Glu (1 µM) and (R,S)-PPG (300 µM), and 300 µM (R,S)-PPG alone. The duration of the applications is indicated with a column. B, each column represents calcium signals (mean values ± S.E.M.) of at least six measurements of two independent experiments. The response of 1 µM L-Glu was taken as control and set to 100%. Asterisks indicate statistically significant antagonist activity (2P < .01; Dunnett's t test).

Moreover, stable cell lines expressing human AMPA(GluR3) or kainate(GluR6) receptors were utilized in the same assay (Daggettet al., 1996

; Varney et al., 1998

). Application of L-glutamateresulted in robust increases of cytoplasmic calcium, whereas (R,S)-PPG(300 µM) did neither evoke calcium signals on its own nor antagonizeL-glutamate in either of the two cell lines (data not shown; Table1).

Ca²⁺/Cl-Dependent L-[³H]Glutamate Binding to Rat Brain Membranes. L-AP4, L-SOP, and (R,S)-PPG displaced L-[³H]glutamate binding at rat hippocampal membranes, measured in the presence of CaCl₂,with IC₅₀ values of 0.5 µM, 3.1 µM, and 1.9 µM, respectively (Table2). Thus, L-AP4 was the most potent among the three compounds,having a 4-fold higher affinity than (R,S)-PPG, which was aboutequipotent with L-SOP.

View this table:
[in this window]
[in a new window]

TABLE 2
Activity of group III mGluR agonists at a Ca²⁺/CI-dependent L-glutamate binding site of rat brain
The affinities of L-AP4, L-SOP, and (R,S)-PPG as displacers of L-[³H]glutamate binding to rat hippocampal membranes were measured in the presence of calcium chloride as described (Urwyler et al., 1997b

). The results shown are means ± S.E.M. from three independent experiments, each performed in triplicate; n_H, Hill coefficient.

Neuroprotective Activity of (R,S)-PPG in Neuronal Culture. In primary cultures of cortical neurons cocultured with glia, (R,S)-PPG was highly neuroprotective when applied during theNMDA-induced excitotoxic pulse (10 min). The action of (R,S)-PPGwas concentration-dependent, with an apparent EC₅₀ value of 12µM (Fig. 5A). Maximally effective concentrations of (R,S)-PPGrescued slightly more than 50% of the neuronal population fromexcitotoxic degeneration (Fig. 5). (R,S)- $alpha$ -Methylserine-O-phosphate(MSOP), a preferential antagonist of group III mGluRs (Thomaset al., 1996), prevented the neuroprotective activity of (R,S)-PPG.In contrast, the selective group II mGluR antagonist (2S)- $alpha$ -ethylglutamicacid (EGlu) (Jane et al., 1996; Thomas et al., 1996) did not affectthe action of (R,S)-PPG (Fig. 5B). Neither (R,S)-PPG nor MSOPor EGlu had any effect on neuronal viability when applied to thecultures in the absence of NMDA (not shown).

View larger version (22K):
[in this window]
[in a new window]

Fig. 5. Protection of cultured cortical neurons against NMDA-induced excitotoxic degeneration by (R,S)-PPG. A, concentration-protection relationship of (R,S)-PPG against NMDA (100 µM)-induced degeneration in mixed cortical cultures assessed by extracellular lactate dehydrogenase activity (measured as mOD/min). The value measured with 100 µM NMDA was taken as 100%. To determine EC₅₀ and Hill coefficient (nH), a sigmoidal curve was fit using the GraphPad Prism program (GraphPad Software, Inc.). B, neuronal degeneration in mixed cortical cultures was induced by 100 µM NMDA (resulting in approximately 85% of maximal NMDA toxicity) and assessed by extracellular lactate dehydrogenase activity (measured as mOD/min, set to 100%). Statistically significant neuroprotection by (R,S)-PPG is indicated by asterisks (2P < .01; Dunnett's t test, n $>=$ 4, at least two independent experiments). (R,S)-PPG neuroprotection can be antagonized by MSOP but not by EGlu.

Protection by (R,S)-PPG against NMDA- and Quinolinic Acid-Induced Striatal Lesions. Intrastriatal infusion of various ionotropic glutamate receptor agonists results in neurochemical and neuropathological changesresembling Huntington's disease (DiFiglia, 1990). First, we haveused infusion of 100 nmol of NMDA which induces an extended areaof necrosis characterized by neuronal loss, reactive gliosis,edema, and neuronal pyknosis (Fig. 6A). Neuronal damage was visibleacross the extension of the caudate nucleus, up to 3 mm posteriorto the injection site. Coinfusion of 250 nmol of (R,S)-PPG withNMDA resulted in efficacious neuroprotection against excitotoxicneuronal damage; particularly in the more lateral parts of thecaudate nucleus, drastically reduced neuronal loss and pyknosisas well as less edema formation were seen (Fig. 6B). To quantitatethe protective effect of (R,S)-PPG, we have measured striatalGAD activity as a biochemical marker of viable GABAergic neurones(Fig. 7), which has been widely used as post-mortem assessmentof lesion size (e.g., Urwyler et al., 1996a). NMDA infusion ledto a 45 to 50% decrease in GAD activity as compared with the respectivecontralateral side. No reduction in GAD activity was observedin animals coinfused with NMDA plus (R,S)-PPG. The protectiveactivity of (R,S)-PPG against NMDA toxicity was mimicked by L-AP4(50 or 250 nmol, Fig. 7).

View larger version (126K):
[in this window]
[in a new window]

Fig. 6. (R,S)-PPG protects against NMDA-induced striatal lesions in vivo. Nissl staining of 20-µm cryostat sections from rat caudate nucleus lateral to the site of NMDA (100 nmol) injection (A); note the large area of extensive necrotic damage at the left side of the micrograph (white arrowheads) and widespread neuronal pyknosis; black arrowheads point at two pyknotic neurones. When (R,S)-PPG (250 nmol) is coinjected with NMDA (B), necrotic damage and neuronal pyknosis is drastically reduced; open arrowheads indicate two healthy neurons. Also, note the higher neuronal density in B compared with A.

View larger version (26K):
[in this window]
[in a new window]

Fig. 7. Quantitation of in vivo neuroprotection by (R,S)-PPG. Degeneration of GABAergic neurones in rat corpus striatum was induced by NMDA (100 nmol) injection and assessed by measuring the GAD activity. GAD activity of rat corpus striatum contralateral to the site of NMDA injection was taken as control and set to 100%. Each column represents mean values ± S.E.M. Statistically significant neuroprotection by (R,S)-PPG and L-AP4 is indicated by asterisks (2P < .01, Dunnett's t test; the number of tested animals in each group is indicated within the columns; for each group, at least two independent experiments were performed).

Furthermore, we tested (R,S)-PPG for protection against intrastriatal infusion of quinolinic acid (200 nmol), which producedlarger lesions than NMDA. Lesion size was quantitated by magneticresonance imaging as described (Sauer et al., 1992

). Comparedwith the control group receiving 200 nmol of quinolinic acid (11animals treated), coinfusion of (R,S)-PPG (250 nmol) showed significantprotection (2P < .005, Dunnett's t test) with a reduction of thelesion size by 58.4% ± 13% (mean ± S.E.M., n = 13animals).

Protection by (R,S)-PPG against MES-Induced Convulsions in Mice. MES is commonly used as a basic in vivo test for anticonvulsive compounds (Kupferberg and Schmutz, 1997 and references therein).In this test, with i.c.v. injections of L-AP4 and L-SOP, a pretreatmenttime of 15 min, and doses between 60 and 220 nmol, no anticonvulsiveeffects were seen. When doses were increased to approximately2000 nmol, L-AP4 and L-SOP induced clonic/clonic-tonic seizuresat 5 to 10 min after drug administration in 40 to 60% of the treatedanimals (Table 3). In contrast, (R,S)-PPG up to 2200 nmol didnot show any proconvulsant effect. Moreover, (R,S)-PPG when appliedat 173 nmol (i.c.v.) produced 100% protection against MES withan ED₅₀ value of 78 nmol (Table 3). At doses above 2000 nmol(i.c.v.), all three compounds were lethal in 20 to 60% of theanimals. (R,S)-PPG given i.p. or i.v. was inactive against MES-inducedconvulsions up to 100 mg/kg and 10 mg/kg, respectively.

View this table:
[in this window]
[in a new window]

TABLE 3
Activity of L-AP4, L-SOP, and (R,S)-PPG in the maximal electroshock test (mouse)
n.d., ED₅₀ values were not determined. The results shown are derived from at least two independent experiments, each performed with at least five animals per group.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

In Vitro Pharmacology. Recent cDNA cloning and recombinant expression of the heterogeneous family of G protein-coupled (metabotropic) glutamate receptorshas created a large gap between the molecular knowledge of mGluRsubtypes and the understanding of their role in brain functionand dysfunction. Thus, the discovery of subtype-selective compoundsand their testing in experimental models for nervous system physiologyand pathology has become increasinglyimportant.

In the present study, using 12 different cell lines stably expressing cloned ionotropic and metabotropic glutamate receptorsubtypes, we have characterized the pharmacological profile of(R,S)-PPG. This compound behaved as a potent agonist at hmGluR8a(EC₅₀ = 200 nM), hmGluR6 (EC₅₀ = 4.7 µM), and hmGluR4a (EC₅₀ =5.2 µM), with no appreciable activity (up to 200 µM) at hmGluR1,hmGluR2, rat mGluR3, hmGluR5, and hNMDAR1A/2B, hNMDAR1A/2A, AMPAR(hGluR3),andkainateR(hGluR6).

(R,S)-PPG therefore exhibited approximately 1000-fold selectivity for hmGluR8 and $>=$ 40-fold selectivity for hmGluR4a and hmGluR6versus group I/II mGluRs and all tested iGluRs. (R,S)-PPG activatedhmGluR7b only at high micromolar concentrations (EC₅₀ = 185 µM),which is only slightly more potent than the compound's weak antagonistactivity at hmGluR2 and its activity against glutamate bindingat rat mGluR3 (Table 1). In addition to its potent activity atgroup III mGluRs, (R,S)-PPG, as well as L-AP4 and L-SOP, displayedmicromolar affinity for a Ca²⁺/Cl-dependent L-[³H]glutamate binding site in rat brain (Fagg et al., 1982

; Urwyleret al., 1996b

). The functional role of this binding site was proposedto be that of a glutamate transporter, but alternative explanationsare also possible (see Urwyler et al., 1996b

and references thereinfor detailed discussion). The affinity of (R,S)-PPG at this sitewas found to be 4-fold lower than the affinity of L-AP4. Whetherthis difference is reflected at the level of endogenous glutamateaccumulation, and thus could contribute to explain the discrepancywe have found between L-AP4 and (R,S)-PPG in the MES model inmice (see below), is currently unclear, especially because theexplanation cannot be extended to L-SOP.

In summary, (R,S)-PPG represents a novel group III mGluR agonist, with in vitro pharmacological properties indistinguishablefrom the current agonists L-SOP, L-AP4, and cyclopropyl-AP4 (Johansenet al., 1995

; Okamoto et al., 1994

; Conn and Pin, 1997

; Flor etal., 1997

;). Interestingly, however, (R,S)-PPG differs structurallyfrom all of these compounds but shares close similarity with classicalcompetitive NMDA receptor antagonists like CGP 40116, as the distancebetween the amino acid moiety and the phosphonate group is comparable.Because this distance is substantially smaller in L-AP4 and L-SOP,the potency and selectivity of (R,S)-PPG for group III mGluRsis quite surprising and suggests a particular mode of bindingof (R,S)-PPG, involving the phenyl spacer between the $alpha$ -aminoacid and phosphonic acidmoieties.

$alpha$ -Methylphosphonophenyl glycine, a mixed antagonist of group II and III mGluRs (Bedingfield et al., 1996

), is structurallythe most closely related compound and differs from (R,S)-PPG onlyby a methyl group in the $alpha$ -position. Thus, replacement of thatgroup with the hydrogen of (R,S)-PPG has changed the antagonisticproperties into selective agonist activity. Similar propertieshave been shown for linear L-glutamate analogs and cyclopropylglycinederivatives (Jane et al., 1996

; Thomas et al., 1996

), where theintroduction of a methyl group at the $alpha$ -position changed agonistsintoantagonists.

Neuroprotection and Anticonvulsive Actions Mediated by (R,S)-PPG. Neuroprotective effects of L-AP4 and L-SOP observed in several in vitro paradigms (see Introduction) prompted us to examine(R,S)-PPG, as a structurally different but pharmacologically indistinguishablecompound, in the model of NMDA-induced degeneration of mouse corticalneurons cocultured with glia (Bruno et al., 1996). Here, we found(R,S)-PPG highly neuroprotective, and its action was antagonizedby MSOP, which is a group III mGluR antagonist (Thomas et al.,1996), but not by the group II mGluR antagonist EGlu. These resultstherefore strengthen the suggestion that activation of group IIImGluRs is neuroprotective in vitro (e.g., Copani et al., 1995;Bruno et al., 1996; Faden et al., 1997).

To investigate neuroprotective effects of (R,S)-PPG also in vivo, we analyzed striatal degeneration following local infusionof NMDA and quinolinic acid into the rat caudate nucleus. Theuse of such excitotoxic injury models, to produce neuronal depletion,reactive gliosis, and alterations of neurotransmitter levels,has been highly valuable for examining pathological patterns reminiscentof Huntington's disease (HD). Even if the primary cause of HDis unrelated, excitotoxic injury mediated by iGluR activationmay play a role in progressive neuronal depletion (DiFiglia, 1990

We found (R,S)-PPG protective against NMDA- and quinolinic acid-induced striatal lesions; to our knowledge, this providesthe first in vivo evidence that activation of group III mGluRsis neuroprotective in animalmodels.

Inhibition of glutamate release by presynaptic mGluR4, -7 and/or -8 (Shigemoto et al., 1997

) may represent a common mechanismof neuroprotection in vitro and in vivo. Accordingly, an enhancedrelease of endogenous glutamate has been shown to facilitate theprogression of NMDA toxicity in cortical cultures (Monyer et al.,1992

). Additionally, in vivo striatal toxicity induced by kainateor NMDA receptor agonists such as quinolinic acid and NMDA criticallyinvolves the presence of cortical glutamatergic fibers afferentto the caudate nucleus of striatum (Colwell et al., 1996

and referencestherein). Although little recurrent excitation exists in the striatum,the endogenously released L-glutamate may have a permissive roleon NMDA and quinolinic acid toxicity, perhaps by activating postsynapticgroup I mGluRs or other facilitatoryreceptors.

Upon depletion of the caudate neuronal population during the progression of HD, the resulting "excess" of corticostriatalglutamatergic input may cause further neuronal loss (DiFiglia,1990

), and inhibition of this input via group III mGluRs may provideprotection. In addition to the regulation of presynaptic glutamaterelease, an inhibition of NMDA receptors by postsynaptic groupIII mGluRs via a protein phosphorylation cascade (Martin et al.,1997

) may also be involved in their neuroprotective effects. Thus,activation of group III mGluRs could open several novel strategiesto interfere with the progressive course of neurodegenerativedisorders.

The potency at cloned mGluRs relative to the protective activity of (R,S)-PPG in primary culture (EC₅₀ = 12 µM) suggests thatthe neuroprotective action of (R,S)-PPG preferentially involvesmGluR4, mGluR6, and/or mGluR8, which are all expressed by culturedcortical neurons (Faden et al., 1997

). For in vivo neuroprotection,however, mGluR6 is probably irrelevant because of its restrictedexpression in the retinal bipolar cells layer. A more detailedexamination of the relative contribution of individual group IIImGluR subtypes to in vitro and in vivo neuroprotection awaitsthe discovery of more selective agonists and the utilization ofgroup III mGluR subtype-deficientmice.

Modulation of epileptic seizures by group III mGluRs has been frequently reported (e.g., Ghauri et al., 1996

; Abdul-Ghaniet al., 1997

; Tang et al., 1997

). Thus, we were tempted to test(R,S)-PPG, in comparison with L-AP4 and L-SOP, in the MES modelin mice. MES is a basic screening test for anticonvulsive drugs,it is indicative of drug activity primarily against generalizedtonic-clonic and, secondarily, also partial seizures, and it ledto the discovery of several clinically approved antiepileptics,e.g., carbamazepine, oxcarbazepine, and phenytoin (Kupferbergand Schmutz, 1997

and references therein). Surprisingly, our resultsfor (R,S)-PPG obtained with this model revealed important differencesas compared with the prototypic group III mGluR agonists L-AP4and L-SOP. In agreement with previous results (Ghauri et al.,1996

; Tang et al., 1997

), both L-AP4 and L-SOP were proconvulsiveat high doses (around 2000 nmol) and did not protect against MES-inducedseizures at any of the given doses (60-2400 nmol). In contrast,(R,S)-PPG exhibited substantial anticonvulsive activity with anED₅₀ value of 78 nmol, full protection at 173 nmol, and did notexhibit any proconvulsive effect up to 2200 nmol. These discrepanciescould possibly be explained by physicochemical properties and/ordivergent in vivo metabolism of the structurally quite differentgroup III mGluR agonists L-AP4, L-SOP, and (R,S)-PPG. Althoughwe cannot exclude that anticonvulsive properties of (R,S)-PPGare mediated by a mechanism distinct from group III mGluRs, otherreports also support group III mGluRs as mediators of anticonvulsiveand antiepileptogenic effects. Abdul-Ghani et al. (1997)

reportedprotective effects of L-AP4 on development of electrical kindlingand also in fully kindled rats. Furthermore, Tang et al. (1997)

reported for L-SOP an immediate, transient (<10 min) proconvulsiveeffect followed by a prolonged (>1 day) anticonvulsive effectagainst sound-induced seizures with an anticonvulsant ED₅₀ valueof 36 nmol. Moreover, recent experimental evidence from mGluR7-deficientmice that exhibit spontaneous epileptic seizures upon certainolfactory stimuli indicates that at least one group III mGluRis critically involved in maintaining the delicate balance betweenneuronal inhibition and excitation (H. van der Putten, personalcommunication).

In conclusion, (R,S)-PPG represents a novel pharmacological tool to analyze the role of group III mGluRs in nervous systemphysiology and pathology, and our in vivo data support a neuroprotectiveand anticonvulsive role for group III mGluRs and encourage thesearch for systemically active group III mGluR agonists as promisingdrugs for the treatment of neurological disorders, such as Huntington'sdisease andepilepsies.

	Acknowledgments

We thank H. Allgeier for critically reading the manuscript and helpful discussion, R. Heckendorn for providing CGP 40116,H. van der Putten for sharing unpublished data, and P. Schoeffterfor initial cAMP measurements with the HEK-hmGluR8a celllines.

	Footnotes

Accepted for publication January 25, 1999.

Received for publication October 19, 1998.

Send reprint requests to: Dr. Peter J. Flor, K-125.6.08, Nervous System Research, Novartis Pharma AG, CH-4002 Basel, Switzerland. E-mail: peter-josef.flor{at}pharma.novartis.com

	Abbreviations

(1S,3R)-ACPD, 1-aminocyclopentane-1S,3R-dicarboxylic acid; CHO, Chinese hamster ovary; EGlu, (2S)- $alpha$ -ethylglutamic acid; HEK, human embryonic kidney; iGluR, ionotropic glutamate receptor; L-AP4, L-2-amino-4-phosphonobutyrate; mGluR, metabotropic glutamate receptor; MSOP, (R,S)- $alpha$ -methylserine-O-phosphate; PCR, polymerase chain reaction; PPG, 4-phosphonophenylglycine; MES, maximal electroshock test; GAD, glutamate decarboxylase; NMDA, N-methyl-D-aspartic acid; GABA, $gamma$ -aminobutyric acid.

	References

Top Abstract Introduction Experimental Procedures Results Discussion References

Abdul-Ghani AS, Attwell PJ, Singh-Kent N, Bradford HF, Croucher MJ and Jane DE (1997) Anti-epileptogenic and anticonvulsant activity of L-2-amino-4-phosphonobutyrate, a presynaptic glutamate receptor agonist. Brain Res 755: 202-212[Medline].
Bedingfield JS, Jane DE, Kemp MC, Toms NJ and Roberts PJ (1996) Novel potent selective phenylglycine antagonists of metabotropic glutamate receptors. Eur J Pharmacol 309: 71-78[Medline].
Bigge CF, Drummond JT, Johnson G, Malone T, Probert AW, Jr, Marcoux FW, Coughenour LL and Brahce LJ (1989) Exploration of phenyl-spaced 2-amino-(5-9)-phosphonoalkanoic acids as competitive N-methyl-D-aspartic acid antagonists. J Med Chem 32: 1580-1590[Medline].
Bruno V, Copani A, Bonanno L, Knöpfel T, Kuhn R, Roberts PJ and Nicoletti F (1996) Activation of group III metabotropic glutamate receptors is neuroprotective in cortical cultures. Eur J Pharmacol 310: 61-66[Medline].
Colwell CS, Altemus KL and Levine MS (1996) Metabotropic glutamate receptor activation selectively limits excitotoxic damage in the intact neostriatum. Brain Res 726: 223-226[Medline].
Conn PJ and Pin JP (1997) Pharmacology and functions of metabotropic glutamate receptors. Annu Rev Pharmacol Toxicol 37: 205-237[Medline].
Copani A, Bruno V, Battaglia G, Leanza G, Pellitteri R, Russo A, Stanzani S and Nicoletti F (1995) Activation of metabotropic glutamate receptors protects cultured neurons against apoptosis induced by beta-amyloid peptide. Mol Pharmacol 47: 890-897[Abstract].
Daggett LP, Jachec C, Lin FF, Deal C, Varney MA, Hess SD, Velicelebi G and Johnson EC (1996) Functional characterization of two isoforms of the human GluR6 receptor and distribution of GluR6 RNA editing sites. Soc Neurosci Abst (236.11).
DiFiglia M (1990) Excitotoxic injury of the neostriatum: A model for Huntington's disease. Trends Neurol Sci 13: 286-289.[Medline]
Duvoisin RM, Zhang C and Ramonell K (1995) A novel metabotropic glutamate receptor expressed in the retina and olfactory bulb. J Neurosci 15: 3075-3083[Abstract].
Faden AI, Ivanova SA, Yakovlev AG and Mukhin AG (1997) Neuroprotective effects of group III mGluR in traumatic neuronal injury. J Neurotrauma 14: 885-895[Medline].
Fagg GE, Foster AC, Mena EE and Cotman CW (1982) Chloride and calcium ions reveal a pharmacologically distinct population of L-glutamate binding sites in synaptic membranes: Correspondence between biochemical and electrophysiological data. J Neurosci 2: 958-965[Medline].
Flor PJ, Gomeza J, Tones MA, Kuhn R, Pin JP and Knöpfel T (1996) The C-terminal domain of the mGluR1 metabotropic glutamate receptor affects sensitivity to agonists. J Neurochem 67: 58-63[Medline].
Flor PJ, Van Der Putten H, Rüegg D, Lukic S, Leonhardt T, Bence M, Sansig G, Knöpfel T and Kuhn R (1997) A novel splice variant of a metabotropic glutamate receptor, human mGluR7b. Neuropharmacology 36: 153-159[Medline].
Ghauri M, Chapman AG and Meldrum BS (1996) Convulsant and anticonvulsant actions of agonists and antagonists of group III mGluRs. Neuroreport 7: 1469-1474[Medline].
Graham ME and Burgoyne RD (1994) Activation of metabotropic glutamate receptors by L-AP4 stimulates survival of rat cerebellar granule cells in culture. Eur J Pharmacol 288: 115-123[Medline].
Hollmann M and Heinemann S (1994) Cloned glutamate receptors. Annu Rev Neurosci 17: 31-108[Medline].
Jane DE, Thomas NK, Tse HW and Watkins JC (1996) Potent antagonists at the L-AP4- and (1S,3S)-ACPD-sensitive presynaptic metabotropic glutamate receptors in the neonatal rat spinal cord. Neuropharmacology 35: 1029-1035[Medline].
Johansen PA, Chase LA, Sinor AD, Koerner JF, Johnson RL and Robinson MB (1995) Type 4a metabotropic glutamate receptor: Identification of new potent agonists and differentiation from the L-(+)-2-amino-4-phosphonobutanoic acid-sensitive receptor in the lateral perforant pathway in rats. Mol Pharmacol 48: 140-149[Abstract].
Knöpfel T, Sakaki J, Flor PJ, Baumann P, Sacaan AI, Velicelebi G, Kuhn R and Allgeier H (1995) Profiling of trans-azetidine-2,4-dicarboxylic acid at the human metabotropic glutamate receptors mGlu1b, -2, -4a and -5a. Eur J Pharmacol 288: 389-392[Medline].
Kupferberg HJ and Schmutz M (1997) Screening of new compounds and the role of the pharmaceutical industry, in Epilepsy: A Comprehensive Textbook (Engel J andPedley TA eds) vol 2, pp 1417-1434, Lippincott-Raven Publishers, Philadelphia.
Laurie DJ, Danzeisen M, Boddeke HW and Sommer B (1995) Ligand binding profile of the rat metabotropic glutamate receptor mGluR3 expressed in a transfected cell line. Naunyn Schmiedeberg's Arch Pharmacol 351: 565-568[Medline].
Laurie DJ, Schoeffter P, Wiederhold KH and Sommer B (1997) Cloning, distribution and functional expression of the human mGlu6 metabotropic glutamate receptor. Neuropharmacology 36: 145-152[Medline].
Lin FF, Varney M, Sacaan AI, Jachec C, Daggett LP, Rao S, Flor P, Kuhn R, Kerner JA, Standaert D, Young AB and Velicelebi G (1997) Cloning and stable expression of the mGluR1b subtype of human metabotropic receptors and pharmacological comparison with the mGluR5a subtype. Neuropharmacology 36: 917-931[Medline].
Lipton SA and Rosenberg PA (1994) Excitatory amino acids as a final common pathway for neurologic disorders. N Engl J Med 330: 613-622[Free Full Text].
Martin G, Nie Z and Siggins GR (1997) Metabotropic glutamate receptors regulate N-methyl-D-aspartate-mediated synaptic transmission in nucleus accumbens. J Neurophysiol 78: 3028-3038[Abstract/Free Full Text].
Monn JA, Valli MJ, Massey SM, Wright RA, Salhoff CR, Johnson BG, Howe T, Alt CA, Rhodes GA, Robey RL, Griffey KR, Tizzano JP, Kallman MJ, Helton DR and Schoepp DD (1997) Design, synthesis, and pharmacological characterization of (+)-2-aminobicyclo[3.1.0]hexane-2,6-dicarboxylic acid (LY354740): A potent, selective, and orally active group 2 metabotropic glutamate receptor agonist possessing anticonvulsant and anxiolytic properties. J Med Chem 40: 528-537[Medline].
Monyer H, Giffard RG, Hartley DM, Dugan LL, Goldberg MP and Choi DW (1992) Oxygen or glucose deprivation-induced neuronal injury in cortical cell cultures is reduced by tetanus toxin. Neuron 8: 967-973[Medline].
Okamoto N, Hori S, Akazawa C, Hayashi Y, Shigemoto R, Mizuno N and Nakanishi S (1994) Molecular characterization of a new metabotropic glutamate receptor mGluR7 coupled to inhibitory cyclic AMP signal transduction. J Biol Chem 269: 1231-1236[Abstract/Free Full Text].
Sauer D, Allegrini PR, Thedinga KH, Massieu L and Fagg GE (1992) Evaluation of quinolinic acid-induced excitotoxic neurodegeneration in rat striatum by quantitative magnetic resonance imaging in vivo. J Neurosci Methods 42: 69-74[Medline].
Shigemoto R, Kinoshita A, Wada E, Nomura S, Ohishi H, Takada M, Flor PJ, Neki A, Abe T, Nakanishi S and Mizuno N (1997) Differential presynaptic localization of metabotropic glutamate receptor subtypes in the rat hippocampus. J Neurosci 17: 7503-7522[Abstract/Free Full Text].
Tanabe Y, Masu M, Ishii T, Shigemoto R and Nakanishi S (1992) A family of metabotropic glutamate receptors. Neuron 8: 169-179[Medline].
Tang E, Yip PK, Chapman AG, Jane DE and Meldrum BS (1997) Prolonged anticonvulsant action of glutamate metabotropic receptor agonists in inferior colliculus of genetically epilepsy-prone rats. Eur J Pharmacol 327: 109-115[Medline].
Thomas NK, Jane DE, Tse HW and Watkins JC (1996) $alpha$ -Methyl derivatives of serine-O-phosphate as novel, selective competitive metabotropic glutamate receptor antagonists. Neuropharmacology 35: 637-642[Medline].
Trombley PQ and Westbrook GL (1992) L-AP4 inhibits calcium currents and synaptic transmission via a G-protein-coupled glutamate receptor. J Neurosci 12: 2043-2050[Abstract].
Urwyler S, Campbell E, Fricker G, Jenner P, Lemaire M, McAllister KH, Neijt HC, Park CK, Perkins M, Rudin M, Sauter A, Smith L, Wiederhold KH and Müller W (1996a) Biphenyl-derivatives of 2-amino-7-phosphono-heptanoic acid, a novel class of potent competitive N-methyl-D-aspartate receptor antagonists-II: Pharmacological characterization in vivo. Neuropharmacology 35: 655-669[Medline].
Urwyler S, Laurie D, Lowe DA, Meier CL and Müller W (1996b) Biphenyl-derivatives of 2-amino-7-phosphonoheptanoic acid, a novel class of potent competitive N-methyl-D-aspartate receptor antagonist-I: Pharmacological characterization in vitro. Neuropharmacology 35: 643-654[Medline].
Varney MA, Jachec C, Deal C, Hess SD, Daggett LP, Skvoretz R, Urcan M, Morrison JH, Moran T, Johnson EC and Velicelebi G (1996) Stable expression and characterization of recombinant human heteromeric N-methyl-D-aspartate receptor subtypes NMDAR1A/2A and NMDAR1A/2B in mammalian cells. J Pharmacol Exp Ther 279: 367-378[Abstract/Free Full Text].
Varney MA, Jachec C, Rao S, Lin FF, Daggett L, Hess S, Velicelebi G and Johnson EC (1998) Pharmacological characterization of the recombinant human AMPA receptor subtype 3 stably expressed in HEK293 cells. J Pharmacol Exp Ther 285: 358-370[Abstract/Free Full Text].
Watkins JC, Krogsgaard Larsen P and Honore T (1990) Structure-activity relationships in the