The Neuroprotective Activity of Group-II Metabotropic Glutamate Receptors Requires New Protein Synthesis and Involves a Glial-Neuronal Signaling

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Volume 17, Number 6, Issue of March 15, 1997 pp. 1891-1897
Copyright ©1997 Society for Neuroscience

The Neuroprotective Activity of Group-II Metabotropic Glutamate Receptors Requires New Protein Synthesis and Involves a Glial-Neuronal Signaling

Valeria Bruno¹, Francesc X. Sureda¹, Marianna Storto¹, Giacomo Casabona¹, Alessandra Caruso², Thomas Knopfel³, Rainer Kuhn⁴, and Ferdinando Nicoletti¹^,³
¹ I. N. M. Neuromed, Pozzilli, Italy, ² Institute of Biochemistry, School of Medicine, and ³ Institute of Pharmacology, School of Pharmacy, University of Catania, 95125 Catania Italy, and ⁴ CNS Department, Ciba Research Laboratories, Basel, Switzerland

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

The group-II metabotropic glutamate (mGlu) receptor agonists (2S,1 $'$ R,2 $'$ R,3 $'$ R)-2-(2,3-dicarboxycyclopropyl)glycine (DCG-IV),S-4-carboxy-3-hydroxyphenylglycine (4C3HPG), and (2S,1 $'$ S,2 $'$ S)-2-(carboxycyclopropyl)glycine(L-CCG-I) protected mouse cortical neurons grown in mixed culturesagainst excitotoxic degeneration induced by a 10 min pulse withNMDA. Protection was observed not only when agonists were addedin combination with NMDA but also when they were transiently appliedto cultures 6-20 hr before the NMDA pulse. In both cases, neuroprotectionwas reduced by the group-II mGlu receptor antagonist (2S,1 $'$ S,2 $'$ S,3 $'$ R)-2-(2 $'$ -carboxy-3 $'$ -phenylcyclopropyl)glycine(PCCG-IV), as well as by the protein synthesis inhibitor cycloheximide(CHX). Both neurons and astrocytes in mixed cultures were immunostainedwith an antibody that recognized mGlu2 and mGlu3 receptors inrecombinant cells. To determine whether astrocytes played anyrole in the neuroprotection mediated by group-II mGlu receptors,we exposed pure cultures of cortical astrocytes to DCG-IV, 4C3HPG,or L-CCG-I for 10 min. The astrocyte medium collected 2-20 hrafter the exposure to any of these drugs was highly neuroprotectivewhen transferred to mixed cultures treated with NMDA. This protectiveactivity was reduced when CHX was applied to astrocyte culturesimmediately after the transient exposure to group-II mGlu receptoragonists. We conclude that neuroprotection mediated by group-IImGlu receptors in cultured cortical cells requires new proteinsynthesis and involves an interaction between neurons and astrocytes.
Key words: cortical cultures; metabotropic glutamate receptors; excitotoxicity; astrocytes; neuroprotection; new protein synthesis

INTRODUCTION

Metabotropic glutamate (mGlu) receptors form a family of eight subtypes, which have tentatively been classified into threegroups (for review, see Pin and Duvoisin, 1995). Group-I mGlureceptors include mGlu1 and -5, which are coupled to polyphosphoinositidehydrolysis when expressed in recombinant cells. Group-II (mGlu2and -3) and group-III (mGlu4, -6, -7, and -8) mGlu receptor subtypesare negatively linked to adenylyl cyclase, although at least mGlu2is also negatively coupled to voltage-sensitive Ca²⁺ channels (Ikeda et al., 1995). mGlu2, -4, and -7 have been foundto be preferentially localized in presynaptic terminals (Shigemotoet al., 1995, 1996), and their activation inhibits glutamate release(for review, see Pin and Duvoisin, 1995). mGlu3 receptors arealso expressed by astrocytes (Tanabe et al., 1993; Petralia etal., 1996), and their functional role is unknown.

Pharmacological activation of group-II or -III mGlu receptors protects neurons against excitotoxic degeneration (Bruno etal., 1994, 1995; Buisson and Choi, 1994, 1995; Altemus et al.,1995; Maiese et al., 1995; Orlando et al., 1995; Turetsky et al.,1995; Buisson et al., 1996). Because activation of group-II and-III mGlu receptors is expected to attenuate neuronal degenerationwithout hampering the efficiency of fast excitatory synaptic transmission,these receptors become potential targets for the experimentaltherapy of acute and chronic neurodegenerative disorders (forreview, see Nicoletti et al., 1996). It has been suggested thatgroup-I or -III mGlu receptor agonists protect cultured neuronsagainst NMDA toxicity by inhibiting the release of glutamate (Brunoet al., 1995) that occurs after the NMDA pulse and contributesto the maturation of the excitotoxic damage (Monyer et al., 1992;for review, see Choi, 1992). The existence of an additional mechanism,however, is suggested by the protective activity of the group-IImGlu receptor agonist (2S,1 $'$ R,2 $'$ R,3 $'$ R)-2-(2,3-dicarboxycyclopropyl)glycine(DCG-IV), under conditions in which there is no excitotoxic componentin the neurodegenerative process (Nicoletti et al., 1996). Wenow report that the neuroprotective activity of group-II mGlureceptor agonists in mixed cultures of cortical cells requiresnew protein synthesis and involves the interaction between neuronsand astrocytes.

MATERIALS AND METHODS
Mixed cortical culture. Mixed cortical cell cultures containing both neurons and astrocytes were prepared from fetal miceat 14-16 d of gestation, as described previously (Rose et al.,1992). Briefly, dissociated cortical cells were plated in 15 mmmultiwell vessels (Falcon Primaria, Lincoln Park, NJ) on a layerof confluent astrocytes (7-14 d in vitro), using a plating mediumof MEM-Eagle's salts (supplied glutamine-free) supplemented with5% heat-inactivated horse serum, 5% fetal bovine serum, glutamine(2 mM), and glucose (final concentration 21 mM). Cultures werekept at 37°C in a humidified 5% CO₂ atmosphere. After 3-5 d invitro, non-neuronal cell division was halted by 1-3 d exposureto 10 µM cytosine arabinoside, and cultures were shifted to amaintenance medium identical to plating medium but lacking fetalserum. Subsequent partial medium replacement was carried out twicea week. Only mature cultures (13-14 d in vitro) were used forthe experiments.

Glial cell culture. Glial cell cultures were prepared as described previously (Rose et al., 1992) from postnatal mice (1-3d after birth). Dissociated cortical cells were grown in 15 mmmultiwell vessels (Falcon Primaria) using a plating medium ofMEM-Eagle's salts supplemented with 10% heat-inactivated horseserum, 10% fetal bovine serum, glutamine (2 mM), and glucose (finalconcentration 21 mM). Cultures were kept at 37°C in a humidifiedCO₂ atmosphere until they reached confluence (7-14 d in vitro).Confluent cultures were then used for the experiments or as asupport for mixed cultures.

Exposure to excitatory amino acids. Brief exposure to NMDA (10 min), in the presence or absence of mGlu receptor agonistsand/or antagonists or protein synthesis inhibitors, was carriedout in mixed or pure cortical cultures at room temperature ina HEPES-buffered salt solution containing (in mM): 120 NaCl, 5.4KCl, 0.8 MgCl₂, 1.8 CaCl₂, 20 HEPES, 15 glucose. After 10 minthe drugs were washed out, and cultures were incubated at 37°Cfor the following 24 hr in medium stock (MS) (MEM-Eagle's supplementedwith 15.8 mM NaHCO₃ and glucose <25 mM). In some experiments,mixed cortical cultures were exposed for 10 min to mGlu receptoragonists, 6 hr before the NMDA pulse. In another set of experiments,a glial-conditioned medium (GCM) was added to the cultures immediatelyafter the NMDA pulse and was kept for the following 24 hr of incubation.GCM was prepared as follows: glial cortical cultures were exposedfor 10 min to mGlu receptor agonists, and then the drugs werewashed out and cultures were kept in MS at 37°C for the following20 hr. After this incubation, the medium was collected and usedimmediately for the experiments.

Assessment of neuronal injury. Neuronal injury was estimated in all experiments by examination of cultures with phase-contrastmicroscopy at 100-400×, 1 d after the insult, when the processof cell death was largely complete. Neuronal damage was quantitativelyassessed in all experiments by estimation of dead neurons by trypan-bluestaining. Stained neurons were counted from three random fieldsper well. Neuronal injury was also assessed by measuring the activityof lactate dehydrogenase (LDH) released from damaged or destroyedcells into the extracellular medium 1 d after the addition ofthe excitotoxins. Because results obtained with cell count ormeasurement of LDH activity were similar, only the former methodwas used in most of the experiments.

Characterization of mGlu2/3 antibodies, immunocytochemistry, and Western blot analysis. Mixed cortical cultures at 13-14 din vitro were stained for mGlu2/3 receptors using immunopurifiedpolyclonal antibodies raised against a synthetic peptide correspondingto the following C-terminal amino acid sequence of rat mGlu2 receptor(one-code letter): VPTVCNGREVVDSTTSSL (for a detailed descriptionof the preparation of the antibody, see Koulen et al., 1996).The specificity of the antibody was assessed in HEK 293 cellstransfected with mGlu2 or -3 subtype. In brief, HEK 293 cellswere transfected with 4 µg of plasmid DNA/dish by calcium phosphateprecipitation (Chen and Okayama, 1987). Forty-eight hours later,cells were lysed, separated on 8% SDS-PAGE, transferred to nitrocellulosemembranes, and incubated with primary and secondary antibodies.The primary antibody was diluted 1:1000 in NETG buffer, and thesecondary antibody (peroxidase-coupled goat anti-rabbit; Bio-Rad,Richmond, CA) was diluted 1:1500. Specific bands were detectedusing the enhanced chemiluminescence (ECL) Western blotting analysissystem (Amersham, Milano, Italy).

For immunostaining, mixed cortical cells were washed twice with PBS, fixed for 30 min in 2% paraformaldehyde, washed threetimes with PBS, and then permeabilized with 0.1% Triton X-100in PBS for 10 min. Cells were then washed, blocked with serum,and incubated with the primary antibody (1:2000) for 2 hr at roomtemperature. After the cells were washed three times, the secondaryantibody was added for 1 hr. After the reaction with avidin-biotin-horseradishperoxidase (Vectastain, ABC-Elite kit, Vector Labs, Burlingame,CA), staining was developed by exposure to 0.05% diaminobenzidine/0.01%H₂O₂ (2-10 min). Western blot analysis in protein extracts frompure cultures of mouse cortical astrocytes was performed as describedby Casabona et al. (1996), using dilutions of the primary antibodyup to 1:250. Protein extracts from (1) rat cerebral cortex, (2)mouse cerebral cortex, and (3) pure cultures of rat cortical astrocytes,prepared as described previously (Condorelli et al., 1989), wereused as controls. Immunoreactive bands were detected by ECL (seeabove).

Materials. NMDA, L-2-amino-4-phosphonobutanoate (L-AP4), S-4-carboxy-3-hydroxyphenylglycine (4C3HPG), (2S,1 $'$ S,2 $'$ S)-2-(carboxycyclo-propyl)glycine(L-CCG-I), and 3,5-dihydroxyphenylglycine (DHPG) were purchasedfrom Tocris Cookson (Bristol, UK).Cycloheximide (CHX) was obtainedfrom Sigma (St. Louis, MO). DCG-IV was a kind gift of ProfessorH. Shinozaki (Tokyo Metropolitan Institute for Medical Sciences,Japan) and (2S,1 $'$ S,2 $'$ S,3 $'$ R)-2-(2 $'$ carboxy-3 $'$ -phenylcyclopropyl)glycine(PCCG-IV) was kindly provided by Professor R. Pelliccari (Instituteof Pharmacology and Chemistry, University of Perugia, Italy).

RESULTS
In primary cultures of mouse cortical cells, a 10 min pulse with 100 µM NMDA induced necrotic death of ~70% of the neuronalpopulation, without damaging the underlying monolayer of astrocytes.As expected, the selective group-II mGlu receptor agonists DCG-IVand 4C3HPG, as well as the preferential group-II mGluR agonistL-CCG-I, substantially reduced neuronal toxicity when appliedin combination with NMDA. This neuroprotection was prevented bythe putative group-II mGlu receptor antagonist PCCG-IV (Thomsenet al., 1996) (Table 1). To unravel the possible role of a geneticprogram in the neuroprotective activity of group-II mGlu receptoragonists, we used the protein synthesis inhibitor CHX. CHX inhibited³H-glycine incorporation into proteins in a concentration-dependentfashion, with an apparent IC₅₀ value of 100 ng/ml. CHX was usedroutinely at a concentration of 500 ng/ml. When applied immediatelyafter the NMDA pulse, CHX was inactive per se, but it attenuatedthe neuroprotective activity of DCG-IV (Fig. 1). This suggestedthat neuroprotection was mediated by new protein synthesis, whichwas induced during the 10 min exposure to DCG-IV. To examine thispoint further, we transiently applied DCG-IV, 4C3HPG, or L-CCG-I6-20 hr before a toxic pulse with NMDA. All of these group-IImGlu receptor agonists attenuated NMDA toxicity to the same extentas they were co-added with NMDA (exemplified in Fig. 2). Thisneuroprotective activity was prevented by CHX (when present duringthe 6-20 hr interval) as well as by PCCG-IV, which was active,however, when present during but not after the transient exposureto DCG-IV or 4C3HPG (Fig. 2). A 10 min preincubation with thegroup-III mGlu receptor agonist L-AP4 or the group-I mGlu receptoragonist DHPG did not substantially protect against NMDA toxicity(Fig. 2), although L-AP4 was neuroprotective when applied in combinationwith NMDA (Table 1).

Table 1. Neuroprotective activity of mGlu receptor agonists against NMDA toxicity in mixed cultures of cortical cells

Count of dead cells
LDH release

Control NMDA (100 µM) Control NMDA (100 µM)

Basal 36 ± 6 415 ± 15 21 ± 6 245 ± 9

DCG-IV, 1 µM 29 ± 8 163 ± 6^* 31 ± 5 100 ± 6^*

4C3HPG, 50 µM 42 ± 12 205 ± 7^* 19 ± 7 120 ± 5^*

PCCG-IV, 20 µM 28 ± 4 385 ± 22 17 ± 9 261 ± 10

DCG-IV + PCCG-IV 31 ± 6 395 ± 10 24 ± 11 240 ± 8

4C3HPG + PCCG-IV 31 ± 5 380 ± 7 17 ± 5 210 ± 8

L-CCG-I, 10 µM 40 ± 6 197 ± 8^* 15 ± 7 115 ± 7^*

L-AP4, 10 µM 26 ± 4 223 ± 5^* 17 ± 8 137 ± 6^*

mGlu receptor agonists and/or PCCG-IV were applied in combination with NMDA. Values are means ± SEM of 6-15 determinations. ^* p < 0.01 (one-way ANOVA + Fisher protected least significant difference), when compared with NMDA alone. Dead cells were countedas cells stained with trypan blue in three random fields/well(200 cells counted per field). LDH release is expressed as mOD/min.LDH, lactate dehydrogenase.

Fig. 1. The protein synthesis inhibitor cycloheximide (CHX) attenuates the neuroprotective activity of DCG-IV in mixed cultures ofcortical cells. Cultures were exposed to a toxic pulse with 100µM NMDA in the absence or presence of DCG-IV. CHX (500 ng/ml)was applied to the cultures immediately after the NMDA pulse.Addition of 100 µM NMDA resulted in the necrotic death of 70 ±8% of the neuronal population (n = 32), without any apparent damageto the underlying monolayer of astrocytes. This value was setat 100%. In untreated cultures, the number of trypan-blue-positivedead neurons was always <3% of the total population. Values indicatethe mean ± SEM and were calculated from four independent experiments(n = 4 individual wells for each experiment). In each experiment,SD was <10% of the mean value.
[View Larger Version of this Image (12K GIF file)]

Fig. 2. Neuroprotective activity of group-II mGlu receptor agonists applied to mixed cultures for 10 min, 6 hr before the toxic pulsewith NMDA. DCG-IV, 1 µM; 4C3HPG, 50 µM; L-CCG-I, 10 µM; L-AP4,10 µM; DHPG, 50 µM; PCCG-IV, 20 µM; CHX, 500 ng/ml. CHX was appliedimmediately after the transient exposure to DCG-IV or 4C3HPG andwas maintained during the 6 hr interval preceding the NMDA pulse.PCCG-IV was applied either in combination with DCG-IV or 4C3HPG(labeled as PCCG) or immediately after the exposure to DCG-IVor 4C3HPG (labeled as PCCGp). In the latter case, PCCG-IV wasmaintained during the 6 hr interval preceding the NMDA pulse (labeledas PCCGp). Values (mean ± SEM) were calculated from three to sixindependent experiments (n = 4 individual wells in each experiment).*p < 0.01 [one-way ANOVA + Fisher protected least significantdifference (PLSD)] when compared with values obtained with DCG-IVor 4C3HPG without addition of CHX or PCCG-IV. Neuroprotectionby DCG-IV or 4C3HPG was also significant when both drugs weretransiently applied 12 or 20 hr before the NMDA pulse (not shown).
[View Larger Version of this Image (16K GIF file)]

Because the mGlu3 receptor is present in astrocytes (Tanabe et al., 1993; Petralia et al., 1996), we wondered whether astrocytescontribute to the neuroprotective activity of group-II mGlu receptoragonists. To examine this question, we incubated pure culturesof mouse cortical astrocytes with DCG-IV, 4C3HPG, or L-CCG-I for10 min and collected the medium at different times after thisincubation. The astrocyte medium collected 2-20 hr after the exposureto group-II mGlu receptor agonists was highly neuroprotectivewhen transferred to sister mixed cultures treated with NMDA (Figs.3, 4). In contrast, the medium collected from untreated astrocytecultures or from cultures treated with L-AP4 or DHPG was inactive(Fig. 4). The conditioned medium removed from astrocytes treatedwith group-II mGluR agonists lost its neuroprotective activityunder the following conditions: (1) when collected immediatelyafter the transient exposure to DCG-IV (Fig. 3) or 4C3HPG (notshown); (2) when CHX was applied after the exposure to DCG-IVor 4C3HPG (Fig. 5); (3) when PCCG-IV was applied during, but notafter, the exposure to DCG-IV or 4C3HPG; and (4) when the mediumwas exposed to 100°C for 20 min before being transferred to mixedcultures. We have therefore hypothesized that group-II agonistsstimulate astrocytes to produce a heat-sensitive factor, whichis released into the medium and rescues neurons against NMDA toxicity.
Fig. 3. Neuroprotective activity of the glial-conditioned medium collected from pure cultures of astrocytes, at different times aftera 10 min exposure to DCG-IV (1 µM). Values were obtained froma representative experiment and calculated from the mean of fourindividual determinations. Values relative to the glial-conditionedmedium collected at 2, 6, or 20 hr after exposure to DCG-IV weresignificantly different as compared with values obtained withcontrol (CTRL) astrocyte medium (i.e., with medium from astrocytestreated with the buffer alone) or with the medium collected fromastrocyte cultures immediately after washing out DCG-IV (labeledas 0) (p < 0.01 by one-way ANOVA + Fisher PLSD test). This experimentwas repeated two times with similar results.
[View Larger Version of this Image (16K GIF file)]

Fig. 4. Neuroprotective activity of the conditioned medium collected from pure cultures of astrocytes 20 hr after a 10 min exposureto the indicated mGlu receptor agonists. CTRL, Control medium(i.e., medium collected from astrocyte cultures treated with thebuffer alone). DCG-IV, 1 µM; 4C3HPG, 50 µM; L-CCG-I, 10 µM; L-AP4,10 µM; DHPG, 50 µM. Values (mean ± SEM) were calculated from threeto five independent experiments (n = 4 individual wells in eachexperiment). *p < 0.01 (one-way ANOVA + Fisher PLSD) when comparedwith CTRL.
[View Larger Version of this Image (16K GIF file)]

Fig. 5. The neuroprotective activity of the glial-conditioned medium collected from pure cultures of astrocytes transiently exposedto DCG-IV (1 µM) or 4C3HPG (50 µM) is attenuated under the followingconditions: (1) when PCCG-IV (PCCG, 20 µM) is present during theexposure to DCG-IV or 4C3HPG; (2) when CHX (500 ng/ml) is appliedto cultured astrocytes immediately after the exposure to DCG-IVor 4C3HPG and maintained afterward; or (3) when the medium ofastrocytes treated with DCG-IV or 4C3HPG is exposed to 100°C for20 min (Heat) just before being transferred to mixed corticalcultures. Values are mean ± SEM and were calculated from threeto five independent experiments (n = 4 individual wells in eachexperiment). *p < 0.01 when compared with the glial-conditionedmedium collected from astrocytes treated with DCG-IV or 4C3HPGalone.
[View Larger Version of this Image (23K GIF file)]

To confirm the presence of group-II mGlu receptors in astrocytes, we performed immunocytochemical studies in mixed culturesusing a polyclonal antibody generated against a C-terminal aminoacid sequence that is highly homologous between mGlu2 and -3 receptors,This antibody specifically labeled protein extracts from HEK 293cells transfected with either mGlu2 or mGlu3 receptor cDNAs (Fig.6A) and stained both neurons and the underlying monolayer of astrocytesin mixed cultures of mouse cortical cells (Fig. 6B). Western blotanalysis, however, did not reveal any immunoreactive band in proteinextracts from pure mouse cortical astrocyte cultures, under conditionsin which the mGlu2/3 receptor antibody labeled extracts from bothrat and mouse cerebral cortex (not shown; for additional details,see legend of Fig. 6). One possible explanation is that the amountof mGlu3 receptor protein expressed by cultured astrocytes isbelow the detection level by Western blot analysis. Accordingly,no immunoreactive band was found in extracts from cultures ofrat cortical astrocytes, where mGlu3 receptor mRNA levels weredetectable by RT-PCR (our unpublished observation).
Fig. 6. A, Immunoblotting with purified mGluR2/3 antibodies on lysates from HEK 293 cells transfected with a plasmid encoding themGlu2 or -3 receptor. Note that the antibody reacts mostly witha high molecular weight band, which may correspond to receptoraggregates (Hayashi et al., 1993). A 100 kDa band correspondingto the deduced molecular weight of mGlu2 and -3 receptors wasdetected only after long-term exposure. Untransfected HEK 293cells (mock) or HEK 293 cells transfected with mGlu1a, -5a, and-4 receptor cDNA (not shown) were not stained by the mGlu2/3 receptorantibody. B, Immunostaining of mixed cultures of cortical cellswith the mGlu2/3 receptor antibody. Note that both neurons andastrocytes are stained by the antibody. 2/3, Specific staining;NS, nonspecific staining. Scale bar, 20 µm. We also performedWestern blot analysis on protein extracts from membranes preparedfrom (1) pure cultures of mouse astrocytes, (2) pure culturesof rat astrocytes, (3) mouse cerebral cortex, and (4) rat cerebralcortex (60 µg of protein loaded for each lane). In extracts frommouse or rat cerebral cortex, the mGlu2/3 receptor antibody labeledexclusively a 100 kDa band and an additional band of higher molecularweight, which may correspond to receptor aggregates (not shown).No immunolabeling was observed in extracts from either mouse orrat cultured astrocytes. This suggests that the antibody thatwe have used is specific for mGlu2/3 but the amount of receptor(s)expressed by cultured astrocytes is possibly too low to be detectedby Western blot analysis.
[View Larger Version of this Image (102K GIF file)]

DISCUSSION
mGlu receptors have recently been considered as a putative target for the experimental therapy of neurodegenerative disorders,because their activation affects multiple intracellular eventsthat contribute not only to the induction but also to the progressionof neuronal damage (for review, see Nicoletti et al., 1996). Activationof group-II mGlu receptors protects cultured neurons against degenerationinduced by various insults, including excitotoxins (Bruno et al.,1994, 1995; Buisson and Choi, 1995; Buisson et al., 1996), oxygen-glucosedeprivation (Buisson and Choi, 1995), $beta$ -amyloid peptide (Copaniet al., 1995), and the broad protein kinase inhibitor staurosporine(Koh et al., 1995). In addition, intracerebral infusion of group-IImGlu receptor agonists protects against quinolinic acid-inducedlesions of striatal medium-size spiny neurons (Altemus et al.,1995; Orlando et al., 1995), as well as against hippocampal neuronaldegeneration secondary to kainate-induced seizures (Kwak et al.,1994). The neuroprotective activity of group-II mGlu receptoragonists is generally ascribed to the activation of neuronal mGlu2receptors, which are presynaptically located and inhibit glutamaterelease (for review, see Pin and Duvoisin, 1995). Inhibition ofglutamate release, however, cannot account for the neuroprotectiveactivity of group-II mGlu receptor agonists against apoptosisinduced by oxygen-glucose deprivation (Buisson and Choi, 1994), $beta$ -amyloid peptide (Copani et al., 1995), or staurosporine (Kohet al., 1995), because apoptosis by oxygen-glucose deprivationor $beta$ -amyloid peptide was induced in the presence of ionotropicglutamate receptor antagonists, whereas staurosporine inhibitsboth protein kinase C or Ca²⁺/calmodulin-dependent protein kinase II (Ruegg and Burgess, 1989),which have been implicated in the development of excitotoxic damage(Favaron et al., 1990; Dawson et al., 1995). In addition, DCG-IVprotects cultured neurons even when applied 30 min after a toxicpulse with NMDA, when large amounts of endogenous glutamate havealready accumulated in the extracellular medium (Bruno et al.,1995).

This suggests that activation of group-II mGlu receptors promotes a mechanism of neuronal rescue, which cannot be simply reconductedto the inhibition of glutamate release. Accordingly, we have foundthat neuroprotection mediated by group-II mGlu receptor activationis long lasting (because DCG-IV, 4C3HPG, or L-CCG-I were stillactive when transiently applied hours before the NMDA pulse) andrequires new protein synthesis. In contrast, the group-III mGlureceptor agonist L-AP4 lost its neuroprotective activity whenapplied before the NMDA pulse. Group-II and -III mGlu receptorsshare the same transduction pathway (Tanabe et al., 1992, 1993)but show a different anatomical localization. mGlu7 receptors,for example, are localized in presynaptic membrane specialization,whereas group-II mGlu receptors are found predominantly in preterminalaxons (Shigemoto et al., 1995, 1996). In addition, mGlu3 receptorsare found in glial cells (Tanabe et al., 1993; Petralia et al.,1996), whereas evidence for the presence of group-III mGlu receptorsin astrocytes is lacking. A role for astrocytes in neuroprotectionwas suggested by the evidence that cortical neurons in pure culturesare more sensitive to toxicity induced by acute exposure to glutamate,by 24 hr exposure to NMDA, or by oxygen-glucose deprivation (Duganet al., 1995), and less sensitive to the protective activity ofDCG-IV against kainate-induced degeneration (our unpublished observation)than neurons in mixed cultures. We have hypothesized thereforeeither that astrocytes produce a permissive factor that enablesthe protective activity of neuronal group-II mGlu receptors orthat activation of group-II mGlu receptors in astrocytes promotesa form of glial-neuronal signaling responsible for neuroprotection.To examine this question, we transiently exposed cultures of pureastrocytes to mGlu receptor agonists and then transferred theconditioned medium to sister mixed cultures treated with NMDA.Only the glial-conditioned medium collected from astrocytes treatedwith group-II mGlu receptor agonists exhibited neuroprotectiveactivity, which was prevented by PCCG-IV, a selective group-IImGlu receptor antagonist (Thomsen et al., 1996). PCCG-IV, however,was not effective when applied to cultured astrocytes after theexposure to agonists, suggesting that neuroprotection did notresult from the uptake and successive release of DCG-IV or 4C3HPGinto the conditioned medium. It is possible that astrocytes synthesizeand release a proteic neurotrophic factor, which is denaturatedwhen samples are exposed to 100°C for 20 min. Alternatively, activationof group-II mGlu receptors (presumably mGlu3) in astrocytes mayinduce the synthesis of an enzyme, which in turn catalyzes theformation of a heat-sensitive neurotrophic factor.

The mechanism by which activation of group-II mGlu receptors in astrocytes induces protein synthesis is unknown. In recombinantcells, these receptors are negatively linked to adenylyl cyclase(Tanabe et al., 1992, 1993). Under some circumstances, however,activation of native group-II mGlu receptors paradoxically mayamplify an evoked increase in cAMP formation, perhaps becauseof the presence of particular isoforms of adenylyl cyclase thatare stimulated by the large amounts of the $beta$ $gamma$ -subunits releasedfrom the G_i proteins (Winder and Conn, 1993). Interestingly, thelatter mechanism occurs in astrocytes and is involved in certainforms of glial-neuronal communication (Balazs et al., 1996; Winderet al., 1996). Alternatively, group-II mGlu receptor agonistsmight stimulate the mitogen-activated protein kinase pathway,as they do in neurons (Strasser and Choi, 1996). Either of thesetransduction pathways may induce the expression of genes encodingputative neuroprotective factors that are released from astrocytesand protect the neighbor neurons against excitotoxic death. Arole for cAMP in the glial mechanism responsible for neuroprotectionmay help explain the intriguing finding that dibutyryl-cAMP, amembrane-permeable cAMP analog, is neuroprotective per se andmay obliterate the protective activity of DCG-IV against NMDAtoxicity in mixed cultures of cortical cells (Mattson and Kater,1988; Bruno et al., 1995).

In conclusion, the present results provide evidence for a novel form of glial-neuronal signaling that contributes to the neuroprotectiveactivity of group-II mGlu receptor agonists in mixed culturesof cortical cells. Signaling seems to be mediated by an astrocyte-derivedneurotrophic factor, the production of which requires new proteinsynthesis. This defensive mechanism, however, may not be efficientagainst all types of excitotoxic insults, because activation ofgroup-II mGlu receptors does not protect cortical neurons grownin mixed cultures against AMPA toxicity (Bruno et al., 1995; Buissonand Choi, 1995; Buisson et al., 1996), whereas the effect on kainate-inducedtoxicity is still controversial. It is noteworthy that the presenceof astrocytes exacerbates AMPA neurotoxicity, although it protectscultured neurons against glutamate or NMDA toxicity (Dugan etal., 1995).

FOOTNOTES

Received Aug. 13, 1996; revised Dec. 5, 1996; accepted Dec. 11, 1996.

Correspondence should be addressed to Dr. Ferdinando Nicoletti, Institute of Pharmacology, School of Pharmacy, Universityof Catania, Viale A. Doria 6, 95125 Catania, Italy.

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