Neuroprotection Mediated by Glial Cell Line-Derived Neurotrophic Factor: Involvement of a Reduction of NMDA-Induced Calcium Influx by the Mitogen-Activated Protein Kinase Pathway

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The Journal of Neuroscience, May 1, 2001, 21(9):3024-3033

Neuroprotection Mediated by Glial Cell Line-Derived Neurotrophic Factor: Involvement of a Reduction of NMDA-Induced Calcium Influx by the Mitogen-Activated Protein Kinase Pathway
Olivier Nicole, Carine Ali, Fabian Docagne, Laurent Plawinski, Eric T. MacKenzie, Denis Vivien, and Alain Buisson
Université de Caen, Unité Mixte de Recherche, Centre National de la Recherche Scientifique 6551, 14074 Caen Cedex, France

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The glial cell line-derived neurotrophic factor (GDNF) is first characterized for its trophic activity on dopaminergic neurons.Recent data suggested that GDNF could modulate the neuronal deathinduced by ischemia. The purpose of this study was to characterizethe influence of GDNF on cultured cortical neurons subjected totwo paradigms of injury (necrosis and apoptosis) that have beenidentified during cerebral ischemia and to determine the molecularmechanisms involved. First, we demonstrated that both neuronsand astrocytes express the mRNA and the protein for GDNF and itsreceptor complex (GFR $alpha$ -1 and c-Ret). Next, we showed that theapplication of recombinant human GDNF to cortical neurons andastrocytes induces the activation of the MAP kinase (MAPK) pathway,as visualized by an increase in the phosphorylated forms of extracellularsignal-regulated kinases (ERKs). Thereafter, we demonstrated thatGDNF fails to prevent apoptotic neuronal death but selectivelyattenuates slowly triggered NMDA-induced excitotoxic neuronaldeath via a direct effect on cortical neurons. To further characterizethe neuroprotective mechanisms of GDNF against NMDA-mediated neuronaldeath, we showed that a pretreatment with GDNF reduces NMDA-inducedcalcium influx. This effect likely results from a reduction ofNMDA receptor activity rather than an enhanced buffering or extrusioncapacity for calcium. Finally, we also demonstrated that an ERKsactivation pathway is necessary for GDNF-mediated reduction ofthe NMDA-induced calcium response. Together, these results describea novel mechanism by which the activation of MAPK induced by GDNFmodulates NMDA receptor activity, a mechanism that could be responsiblefor the neuroprotective effect of GDNF in acute braininjury.

Key words: GDNF; excitotoxicity; apoptosis; NMDA receptor; Fura-2; MAPK

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ischemia-induced neuronal injury is thought to result from an excessive release of excitatory amino acids and the subsequentactivation of their postsynaptic receptors. This excitotoxic pathwaymay also contribute to brain and spinal cord cell loss after variousacute insults. The first step in the excitotoxic cascade is mediatedby the activation of ion channel-linked glutamate receptors, especiallyNMDA receptors, probably because of their high calcium (Ca²⁺) permeability (Choi, 1995). The subsequent activation of cytoplasmicCa²⁺-dependent enzymes has been proposed to mediate the final excitotoxicity.More recently, various clues have emerged to suggest that bothglobal and focal ischemia may have an apoptotic component (Linniket al., 1993; MacManus et al., 1993).

Because of their capacity to promote neuronal survival during embryogenesis, the use of growth factors has been proposed tolimit the consequences of cerebral ischemia. Among these cytokines,a structurally related family has gained prominence because ofits high level of expression in biopsies of patients with acutebrain injury or neurodegenerative diseases, i.e. the transforminggrowth factor- $beta$ s (TGF- $beta$ s) (Pratt and McPherson, 1997). Althoughthe beneficial effects of TGF- $beta$ have been well studied (Buissonet al., 1998), questions have arisen about the role of a distantmember of the TGF- $beta$ family, the GDNF, during braininjury.

The GDNF transcript has been detected in all major brain regions (Schaar et al., 1993). Based on an expression strategy toidentify high affinity binding proteins, the GDNF receptor $alpha$ -1(GFR $alpha$ -1) has been cloned (Jing et al., 1996; Treanor et al., 1996).It is a protein anchored to the cell surface by a glycosyl-phosphatidylinositol (GPI) devoid of an associated kinase activity. The signalingcomponent of the GDNF receptor has been identified as the tyrosinekinase receptor encoded by the proto-oncogene c-Ret (Durbec etal., 1996; Trupp et al., 1996). After binding to its specificreceptor complex, GDNF activates several downstream intracellularpathways, including mitogen-activated protein kinase (MAPK) (Worbyet al., 1996) and PI-3 kinase (Soler et al., 1999), resultingin long-term changes in gene expression (Messer et al., 1999).

GDNF was first characterized as a potent neurotrophic factor for dopaminergic and motor neurons (Lin et al., 1993; Hendersonet al., 1994). To date, several studies have revealed a neuroprotectiveinfluence of GDNF against various toxic challenges (Krieglsteinet al., 1995). Recently, it has been suggested that GDNF couldalso modulate neuronal death induced by acute brain injury (Wanget al., 1997). In this study, these authors demonstrated that,after middle cerebral artery occlusion (MCAo) in rodents, theapplication of GDNF reduces the infarcted volume. Although theneuroprotective activity of GDNF against ischemia-induced neuronaldeath is now well established (Abe et al., 1997; Kitagawa et al.,1998), little is known about the mechanisms that underpin thisneuroprotection. The purpose of the present study was to determinethe influence of GDNF on apoptosis and necrosis, two differentparadigms of neuronal death that have been identified during cerebralischemia, and to explore the molecular mechanisms by which GDNFexerts itseffect.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

PCR-reverse transcriptase system kits, Wizard Plus Minipreps DNA Purification System, and U0126 were purchased from Promega(Charbonnières, France). DMEM, poly-D-lysine, laminin, cytosine $beta$ -D-arabinofuranoside (Ara-C), staurosporine (Stp), ExtrAvidin,and cycloheximide were obtained from Sigma (L'Isle D'Abeau, France).Horse serum and fetal bovine serum were from Life Technologies(Cergy Pontoise, France). Recombinant human GDNF (rhGDNF) wasobtained from R&D Systems (Oxon, UK), and antibodies raised againstGDNF, GFR $alpha$ -1, c-Ret, extracellular signal-regulated kinase 1 (ERK1),phospho-ERKs (p-ERKs), p-c-Jun N-terminal protein kinase (p-JNK),and p-38 were purchased from Santa Cruz (Heidelberg, Germany).NMDA, AMPA, kainate, and (+)5-methyl-10,11-dihydro-5H-dibenzo(a,d)cyclohepten-5,10-iminemaleate (MK-801) were from Tocris (Bristol,UK).

Mixed cortical cultures
Mixed cortical cultures containing both neurons and astrocytes were prepared from fetal OF1 mice at 14-16 d gestation, asdescribed by Rose et al. (1993). Briefly, dissociated corticalcells were plated in 24 wells on a layer of confluent astrocytes,using a medium stock (MS; MEM with 25 mM glucose) supplementedwith 5% horse serum, 5% fetal bovine serum, and 2 mM glutamine.After 7 d in vitro (DIV), non-neuronal cell division was haltedby a 1-3 d exposure to 10 µM Ara-C. Subsequent partial mediumreplacement was performed twice a week, and after 12 DIV, cultureswere shifted to a maintenance medium identical to plating mediumbut lacking serum. Cultures were used after 14DIV.

Glial cultures
Glial cell cultures were prepared from postnatal mice (1-3 d after birth), as described previously (Rose et al., 1993). Dissociatedcortical cells were grown in multiwell vessels using a platingmedium of MS supplemented with 10% horse serum, 10% fetal bovineserum, and 2 mM glutamine. Cultures were kept at 37°C in a humidified5% CO₂-containing atmosphere until they reached confluency (7-14DIV). Confluent cultures were used then as a support for mixedcultures.

Near pure neuronal cell cultures
These cultures containing <5% astrocytes were prepared as detailed previously (Rose et al., 1993). Dissociated cortical cellsin MS supplemented with 5% fetal bovine, 5% horse serum, and 2mM glutamine were plated in multiwell vessels that had been coatedpreviously with poly-D-lysine and laminin. After 3 DIV, non-neuronalcell division was halted by an exposure to 10 µM Ara-C. Therewas no further exchange of the media. After 12 DIV, cultures didnot need the presence of serum to survive. They were shifted toa maintenance medium identical to plating medium but lacking serum.Cultures were used after 7 DIV for serum deprivation (SD) andafter 13-14 DIV for excitotoxicinjury.

Reverse transcription and PCR
Total RNAs were isolated from mouse cerebral cortices and murine cell cultures through the use of either the RNAxel kit (Eurobio,Les Ulis, France) or the Rneasy Kit (Qiagen, Courtaboeuf, France).One microgram of total RNAs was reverse transcribed into cDNAusing poly-dT oligonucleotides. Then, an aliquot of the cDNA librarieswas amplified using sense and antisense primers for GDNF (640bp, 45 cycles), GFR $alpha$ -1 (351 bp, 38 cycles), and c-Ret (615 bp,40 cycles). The number of PCR cycles was chosen, correspondingto 50% of the saturating curve of each PCR product. The followingconstructs were used: GDNF sense oligonucleotide, ATG AAG TTATGG GAT GTC GT, and antisense oligonucleotide, CAG GGT CAG ATACAT CCA CA; GFR $alpha$ -1 sense oligonucleotide, CAT GTT CCT AGC CACTCT GT, and antisense oligonucleotide, TCCAGT AGG TCA TTT CCCTG; c-Ret sense oligonucleotide, TGT ATG TAG ACC AGC CAG CT, andantisense oligonucleotide, ACT ATG CAC AAA GCC TCC AG. Amplifiedproducts were separated by 1.5% agarose gel electrophoresis andvisualized by ethidium bromidestaining.

SDS-PAGE and Western blot
The cerebral cortex of adult mouse and the murine-cultured cortical neurons (DIV 14) and astrocytes (confluent cultures) werelysed in Tris-NaCl-Triton buffer and centrifuged for 5 min (2500rpm) to obtain whole-cell extracts. Then, an SDS-PAGE (polyacrylamidepercentage, 20% for GDNF and 12% for GFR $alpha$ -1 and c-Ret) was performedbefore immobilization onto a polyvinylidene difluoride membrane.Blots were exposed for 1 hr at room temperature to the primaryantibody (anti-Ret, 1:100; anti-GFR $alpha$ -1, 1:100; anti-GDNF, 1:100)in a blocking reagent [Tris-buffered saline (TBS): Tris 10 mMand NaCl 200 mM, pH 7.4] containing 0.1% Tween 20, 5% dry milk.The membranes were washed and incubated for 1 hr with the appropriatesecondary biotin-conjugated antibody (1:1000) and then for 1 hrwith ExtrAvidin (1:2000) before revelation using a chemiluminescencekit (NEN, Paris,France).

Immunocytochemistry
Murine cortical cultures (DIV 14) were fixed in 4% paraformaldehyde in PBS, pH 7.4, for 30 min. After two rinsings in PBS,the preparations were incubated overnight with the primary antibodyraised against either GDNF or GDNF receptors (GDNF, GFR $alpha$ -1, andc-Ret, 1:100 in PBS, plus 1% BSA and 0.1% Tween). Cells were thenwashed and incubated for 1 hr with the appropriate secondary biotin-conjugatedantibody. Antibody-antigen complexes were amplified with avidin(Vectastain ABC Kit; Vector Laboratories, Burlingame, CA) andrevealed by H₂O₂-peroxidasereaction.

Analysis of p-ERKs
Murine-cultured cortical neurons (DIV 14) and astrocytes (confluent cultures) were lysed in a buffer containing 1 mM sodiumorthovanadate and phosphatase inhibitors mixture (Sigma, L'IsleD'Abeau, France). After homogenization, the protein concentrationwas measured by Bradford's method, using BSA as the standard.Equivalent amounts of protein for each sample were resolved in15% SDS-PAGE that was blotted electrophoretically to polyvinylidenedifluoride membranes. Blots were incubated with the p-ERK antibody(1:200), followed by incubation with the appropriate secondarybiotin-conjugated antibody (1:1000) and then with ExtrAvidin (1:2000)before revelation using a chemiluminescence kit (NEN, Paris, France).The blots were then incubated in stripping buffer (62 mM TrisHCl, pH 6.8, 2% SDS, and 100 mM $beta$ -mercaptoethanol) for 30 minat 50°C, followed by incubation with TBS containing 0.1% Tween20, 5% dry milk. The blots were then incubated with an ERK1 polyclonalantibody (1:200) that binds to ERK1 andERK2.

Excitotoxicity
Slowly triggered excitotoxicity was induced at 37°C by 24 hr exposure to 12.5 µM NMDA, 10 µM AMPA, or 50 µM kainate in MSsupplemented with 10 µM glycine (Choi, 1992). MK-801 (10 µM) wasalways added concurrently with AMPA or kainate to block secondaryNMDA receptor activation. rhGDNF was coapplied with the excitotoxinand left in the bathing media for 24 hr. Neuronal death was estimatedby examination of the cultures under phase-contrast microscopyand quantified by the measurement of lactate dehydrogenase (LDH)release from damaged cells into the bathing medium 1 d after theonset of excitotoxin exposure (Koh and Choi, 1987). The LDH levelcorresponding to complete neuronal death (without glial death)was determined in sister cultures exposed to 200 µM NMDA. BackgroundLDH levels were determined in sister cultures subjected to shamwash and subtracted from experimental values to yield the signalspecific for experimentally inducedinjury.

Apoptosis
Serum deprivation. SD was initiated by transferring pure neuronal cultures (DIV 7), which require serum to survive for 24hr, into growth medium (MS) lacking serum (Martin et al., 1988)in the presence or absence of rhGDNF. The control consisted ofsham wash with serum-containing medium. Secondary NMDA receptoractivation was blocked by addition of MK-801 to the bathing medium.Neuronal cell death was assessed by phase-contrast cell countingafter staining with 0.4% trypan bluedye.
Staurosporine-induced apoptosis. Stp exposure was performed at 37°C for 24 hr by transferring mixed cortical cell cultures(DIV 13-14) in MS supplemented with glycine (10 µM), containing200 nM Stp (Koh et al., 1995) with or without rhGDNF. To confirmthe neuronal death as apoptotic, the protein synthesis inhibitorcycloheximide (1 µg/ml) was administered with Stp in an additionalset of cultured cells. MK-801 (10 µM) was always added concurrentlywith Stp to block secondary NMDA receptor activation. Neuronalcell death was assessed by the measurement of LDHrelease.
Analysis of DNA fragmentation in agarose gel. Cortical cells were lysed at 4°C for 30 min in a buffer containing 0.2% SDS,200 µg/ml proteinase K, 50 µg/ml RNase A. After treatment, DNAwas extracted with Wizard Plus Minipreps DNA Purification System.DNA samples were loaded onto a 1.4% agarose gel and run at 90V for 1hr.
Intracellular free Ca²⁺ measurement. Cell cultures were loaded with fura-2 (30 min, room temperature) in 5 µM fura-2 AM plus0.1% pluronic F-127 (Molecular Probes, Leiden, the Netherlands)and incubated for an additional 30 min in an HEPES-buffered salinesolution. Experiments were performed at room temperature, on thestage of a Nikon Eclipse inverted microscope equipped with a 75W xenon lamp and a Nikon 40×, 1.3 numerical aperture (NA) epifluorescenceoil immersion objective. Fura-2 (excitation of 340 and 380 nm;emission of 510 nm) ratio images were acquired with a CCD camera(Princeton Instruments, Trenton, NJ) and digitized (256 × 512pixels) using Metafluor software (Universal Imaging Corporation,Chester, PA). Fluorescence ratios (340/380 nm) were convertedto intracellular Ca²⁺ concentrations using the following formula: [Ca²⁺]_i = K_d[(R $-$ R_min)/(R_max $-$ R)] F₀/F_s, where R is the ratio forobserved 340/380 fluorescence ratio, R_min is the ratio for a Ca²⁺-free solution, R_max is the ratio for a saturated Ca²⁺ solution, K_d = 135 nM (the dissociation constant for fura-2),F₀ is the intensity of a Ca²⁺-free solution at 380 nm, and F_s is the intensity of a saturatedCa²⁺ solution at 380 nm. We analyzed 20 neurons per coverslip fromthree different dissections containing both neurons andastrocytes.
Statistical analysis. Results are expressed as mean ± SEM. When n = 12 is indicated, this value corresponds to 12 differentwell pools derived from three different dissections. Statisticalanalysis consisted of one-way ANOVA, followed by Bonferroni-Dunn'stest. For the fura-2 experiments, statistical analysis consistedof multiple ways ANOVA followed by Bonferroni-Dunn'stest.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cultured cortical astrocytes and neurons both display GDNF and GDNF receptors

The expression of GDNF and the GDNF receptor complex in murine cerebral cortex and murine cortical cultures was determinedat the mRNA level. Each set of oligonucleotides used for reversetranscription-PCR studies gave the PCR products of the expectedsize (640 bp for GDNF, 351 bp for GFR $alpha$ -1, 615 bp for c-Ret), asillustrated in Figure 1, A, D, and G. To demonstrate the specificityof the PCR products, digest controls through the use of the internalrestriction sites of the PCR products were performed (data notshown). These studies revealed that mRNAs for GDNF (Fig. 1A),GFR $alpha$ -1 (Fig. 1D), and c-Ret (Fig. 1G) are expressed in murinecerebral cortex, cortical neurons, and astrocytes.

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Figure 1. Comparison of protein expression of GDNF and GDNF receptor complex between murine cerebral cortex and cultured cortical neurons and astrocytes. Total RNAs of murine astrocytic (Ast) and neuronal (Neur) cortical cultures and murine cerebral cortex (Cx) were extracted and reverse transcribed using a poly-dT primer. A, D, G, PCR amplification was performed then using a specific set of primers for GDNF (A), GFR $alpha$ -1 (D), and c-Ret (G). B, E, H, Western blot was performed on a lysate derived from murine cerebral cortex, neurons, or astrocyte cultures showing GDNF (B) and GDNF receptor expression (E, H). C, F, I, Immunocytochemistry analysis of GDNF and GDNF receptor components in cultured astrocytes and neurons. Bright-field photomicrographs of either pure cortical astrocytes or pure cortical neurons in culture, after fixation and peroxidase staining for antibodies raised against GDNF (C), GFR $alpha$ -1 (F), and c-Ret (I).

The expression of GDNF and GDNF receptor complex was characterized further at the protein level by immunoblotting and immunocytochemistry.Immunoblot that is performed from cerebral cortex lysate, culturedneurons, or astrocyte lysates with an anti-GDNF antibody revealsa single band (Fig. 1B) at the expected molecular weight (20 kDa)(Krieglstein et al., 1998). Similarly, immunoblot that is performedwith an anti-GFR $alpha$ -1 antibody reveals the presence of two bandsat the expected molecular weights (58 and 45 kDa) (Fig. 1E), correspondingto the glycosylated and nonglycosylated forms of GFR $alpha$ -1 (Jinget al., 1996). Immunoblot that is performed with an anti-c-Retantibody reveals the presence of a band (Fig. 1H), as previouslydescribed by Van Weering et al. (1998), corresponding to a 170kDa mature form at the plasma membrane. Together, these resultsreveal the expression of GDNF and GDNF receptor proteins in micecerebral cortex, cortical neurons, and cortical astrocyte cultures.In the next experiment, we performed immunocytochemistry studieson pure cultured cortical neurons and astrocytes. We showed thatboth neurons and astrocytes in culture express GDNF and the GDNFreceptor complex (GFR $alpha$ -1 and c-Ret) (Fig. 1C,F,I). When the sameexperiments were performed without adding the primary antibody,we did not observe any nonspecific labeling (data notshown).

Neurons and astrocytes express a functional receptor complex

It has been demonstrated previously in dopaminergic neurons that the GDNF transduction pathway involves MAPK (Worby et al.,1996). However, there is no information available about the transductionpathway in cortical neurons. Here, we performed an immunoblottingstudy with antibodies raised against the phosphorylated formsof ERKs (p-ERKs) on cortical neurons and astrocytes exposed torhGDNF. Then, aliquots of whole-cell lysates were separated bySDS-PAGE and incubated with the anti-p-ERKs antibody. A representativetemporal pattern of ERKs phosphorylation under GDNF exposure isshown in neurons (Fig. 2A) and in astrocytes (Fig. 2B). In bothcortical neurons and astrocytes, addition of rhGDNF (10 ng/ml)resulted in a rapid increase (15 min) in the phosphorylation ofp44 (ERK1) and p42 (ERK2) that was maintained for the next 60min of rhGDNF exposure to cortical neurons. The same blots werestripped and reprobed for total ERKs, showing that the treatmentwith rhGDNF modifies the phosphorylation level of ERKs but notthe total level of ERK protein (Fig. 2A,B).

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Figure 2. GDNF induces a phosphorylation of ERKs. Mouse primary cortical neurons (A) or astrocytes (B) were treated with rhGDNF (10 ng/ml) for the indicated times. Aliquots of whole-cell lysates were separated by SDS-PAGE, transferred to membranes, and incubated with the anti-p-ERKs antibody or anti-total ERK antibody. The immunoblots are representative of three independent experiments.

GDNF protects neurons against NMDA-induced cell death

To test whether GDNF modulates neuronal outcome after an ischemic insult, we studied the effects of rhGDNF on murine corticalcell cultures exposed to different paradigms of cell death (apoptosisand necrosis) identified during cerebralischemia.

To induce apoptosis, near pure cortical neuronal cultures after 7 DIV were transferred to a serum-deficient medium (Martinet al., 1988), which provoked the death of ~80% of neurons over24 hr. This paradigm evidenced three features typical of apoptosis:(1) neurons exhibited a gradual shrinkage of the cell body; (2)death was almost completely abolished by the addition of cycloheximide(1 µg/ml), a protein synthesis inhibitor (Fig. 3C,D); and (3)death was accompanied by a nuclear condensation (Fig. 3A) andappearance of DNA fragmentation (Fig. 3B). Addition of rhGDNFto the bathing medium (1-10 ng/ml) failed to modify the progressionand the extent of neuronal degeneration (Fig. 3C). Neuronal apoptosiswas also induced by exposing mixed neuron-glia cultures (14 DIV)to staurosporine (200 nM), a nonspecific protein kinase inhibitor,which caused a neuronal degeneration evolving over 24 hr (Kohet al., 1995). Although cycloheximide treatment blocked the staurosporine-inducedneuronal death, the addition of rhGDNF (1-10 ng/ml) was withouteffect (Fig. 3D).

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Figure 3. rhGDNF does not protect neurons against apoptotic cell death. To induce apoptosis, near pure cortical neuronal cultures (DIV 7) were transferred to a serum-deficient medium (SD). A, B, 24 hr after serum deprivation, the neurons were fixed and stained with DAPI to observe DNA condensation (A) or the DNA of cortical neurons was extracted and loaded onto an agarose gel to evidence DNA fragmentation (B). C, D, Neuronal death percentage was assessed after 24 hr by trypan blue dye staining (mean ± SEM; n = 12) after SD (C) or by LDH release (mean ± SEM; n = 12) after exposure of mixed cortical cultures (14 DIV) to staurosporine 200 nM (Stp) (D). SD and Stp exposure were performed in the presence (gray bars) or absence (white bars) of rhGDNF and with or without 1 µg/ml cycloheximide (CHX). In both apoptotic paradigms, MK-801 was systematically added to block the secondary activation of NMDA receptors. * indicates significantly different from SD or STP by ANOVA, followed by Bonferroni-Dunn's test (p < 0.05).

Thereafter, we investigated the influence of GDNF on excitotoxic necrosis, a process morphologically distinct from apoptosisand characterized by a prominent and early cell swelling. A 24hr incubation with the ionotropic glutamatergic agonists NMDA,AMPA, and kainate induced necrosis (Rose et al., 1993). Exposureof mixed cortical neuron-glia cultures (14 DIV) to these agonistsproduced acute swelling of neuronal cell bodies that was followed24 hr later by a widespread neuronal degeneration, whereas theglia remained intact. Although the rhGDNF (1-10 ng/ml) failedto produce any neuroprotective effect against neuronal death inducedby the exposure to non-NMDA agonists (AMPA and kainate) (Fig.4A) (n = 10), this growth factor significantly reduced NMDA-inducednecrotic neuronal death in mixed neuron-glia cultures. This neuroprotectiveeffect was dose dependent (Fig. 4B) (n = 12; p < 0.05). We furtherinvestigated the influence of rhGDNF on excitotoxic neuronal deathby applying NMDA (12.5 µM) for 24 hr in near pure neuronal cultures(14 DIV) containing <5% of astrocytes, as determined by GFAP immunostaining(data not shown). In these cultures, rhGDNF (10 ng/ml) showeda neuroprotective activity against NMDA-induced necrotic deathsimilar to that observed in mixed neuron-glia cultures (Fig. 4C)(n = 12; p < 0.05).

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Figure 4. rhGDNF is neuroprotective against NMDA-induced neuronal death. A, Cultures were exposed for 24 hr to AMPA (10 µM) or kainate (50 µM) (with 10 µM MK-801 added to block secondary NMDA receptor-mediated toxicity), without (white bars) or with (gray bars) 10 ng/ml rhGDNF. Medium LDH was assessed at the end of the exposure to excitotoxins (mean ± SEM; n = 10 cultures per condition). B, C, Mixed neuron-glia cortical cultures (B) or near pure cortical neuron cultures (C) were exposed for 24 hr to NMDA (12.5 µM) without (white bars) or with (gray bars) increasing concentration of rhGDNF or MK-801 (10 µM). Medium LDH was assessed at the end of the exposure to excitotoxin (mean ± SEM; n = 12 cultures per condition. * indicates significantly different from NMDA; # indicates significantly different from control (sham wash) by ANOVA, followed by Bonferronni-Dunn's test (p < 0.05).

A GPI-linked protein mediates the neuroprotective activity of GDNF

To further characterize the neuroprotective activity of GDNF, we attempted to demonstrate whether the GFR $alpha$ -1 receptor, a GPI-anchoredprotein, mediates the neuroprotective effect of GDNF. Mixed glialcultures were treated with phosphoinositide-specific phospholipaseC (PIPLC; 0.3 IU/ml), an enzyme that cleaves the GPI moiety tothe cell surface. As illustrated in Figure 5A, cultures exposedto NMDA (12.5 µM for 24 hr) exhibited 50% neuronal death. Thecoincubation with rhGDNF (10 ng/ml) reduced by ~50% the NMDA-inducedneuronal death (Fig. 5A). The PIPLC pretreatment (0.3 IU/ml for2 hr at 37°C) abolished the neuroprotective effect of rhGDNF (Fig.5A,B) (n = 12; p < 0.05). PIPLC pretreatment alone did not affectneuronal survival and was without effect on the NMDA-induced neuronaldeath (Fig. 5B). Overall, these results suggest that a GPI-linkedprotein mediates the neuroprotective activity of GDNF.

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Figure 5. A GPI-linked protein mediates the neuroprotective activity of rhGDNF. A, Phase-contrast photomicrographs of mixed neuron-glia cortical cultures pretreated or not with PIPLC (0.3 IU/ml for 2 hr at 37°C) after NMDA application (12.5 µM) in the presence or absence of rhGDNF. Top left, Sham-washed cultures; top right, NMDA-treated cells; bottom left, NMDA-treated cells coincubated with rhGDNF (10 ng/ml); bottom right, cells pretreated with PIPLC and incubated with NMDA and rhGDNF. B, Neuronal death percentage was estimated by LDH release (mean ± SEM; n = 12) after a 24 hr exposure to NMDA (12.5 µM) in mixed neuron-glia cortical cultures in the presence (gray bars) or absence (white bars) of rhGDNF and pretreated or not pretreated with 0.3 IU/ml PIPLC for 2 hr at 37°C. * indicates significantly different from NMDA; # indicates significantly different from NMDA plus GDNF by ANOVA, followed by Bonferroni-Dunn's test (p < 0.05).

The neuroprotective effect of GDNF is independent of an antioxidant effect of GDNF treatment

The characteristic features of glutamate receptor activation are an intracellular accumulation of Ca²⁺ that induces the production of cytotoxic molecules, includingnitric oxide (Dawson et al., 1991), and the production of freeradicals (Coyle and Puttfarcken, 1993; Lafon-Cazal et al., 1993).To determine the mechanisms by which GDNF reduces the NMDA-inducedneurotoxicity, we tested the influence of rhGDNF incubation againstfree radical-mediatedinjury.

To induce free radical injury, mixed cultures of cortical neurons and glia (14 DIV) were exposed continuously for 24 hr to35 µM FeCl₂. The Fe²⁺ treatment induces the production of hydroxyl free radicals throughthe Fenton reaction (Halliwell, 1992). As previously reported(Gwag et al., 1995), mixed cortical cell cultures exhibit a markedneuronal cell body swelling that resulted in a widespread neuronaldeath 24 hr later, whereas the glia remained intact. The coincubationof Trolox (100 µM), an antioxidant agent, totally blocked thisFe²⁺-mediated neuronal death, as reported by Chow et al. (1994). Incontrast, cotreatment with 10 ng/ml rhGDNF did not reduce neuronaldeath (Fig. 6) (n = 12). This result suggests that the GDNF neuroprotectiveactivity on NMDA-mediated neuronal death is not caused by a freeradical scavenging effect.

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Figure 6. GDNF does not protect against neuronal death induced by reactive oxygen species. Mixed neuron-glia cortical cultures were exposed for 24 hr to FeCl₂ (35 µM) without (white bars) or with (gray bars) 10 ng/ml rhGDNF and with or without Trolox (100 µM). Medium LDH was assessed at the end of FeCl₂ exposure (mean ± SEM; n = 12 cultures per condition). * indicates significantly different from FeCl₂ by ANOVA, followed by Bonferroni-Dunn's test (p < 0.05).

The neuroprotective effect of GDNF results from a decrease of the NMDA-induced Ca²⁺ response in cortical neurons

Because the massive Ca²⁺ influx through the glutamate receptors has been shown to be a critical event in excitotoxic neuronaldeath (MacDermott et al., 1986), we examined the question of whetherrhGDNF reduces NMDA and non-NMDA-induced Ca²⁺ influx through the use of fura-2 fluorescencevideomicroscopy.

To investigate the effect of rhGDNF on the NMDA response, we performed a 10 min exposure to NMDA (100 µM) which produced arapid increase in neuronal [Ca²⁺]_i that quickly achieved a plateau. The incubation with rhGDNF(10 ng/ml for 45 min at 37°C) before NMDA application reducedthe plateau value (Fig. 7A,B) (three experiments; 60 cells; p< 0.05). This GDNF-mediated reduction of the NMDA-induced intracellularCa²⁺ rise was abolished by a PIPLC pretreatment (0.3 IU/ml, 2 hr at37°C) (Fig. 7B). To test whether the GDNF-mediated reduction inthe intracellular Ca²⁺ rise might be the consequence of an enhanced Ca²⁺ buffering capacity, we studied the effect of rhGDNF pretreatmenton the KCl-induced Ca²⁺ influx in the presence of an NMDA antagonist (MK-801; 10 µM),a paradigm that induces an intracellular Ca²⁺ rise independent of the NMDA receptor. A 50 mM KCl exposure produceda rapid increase in [Ca²⁺]_i influx into neurons with a peak value similar to that observedafter an NMDA exposure (Fig. 7C). The rhGDNF treatment beforethe KCl exposure failed to modify the rise in intracellular Ca²⁺ influx. Together, these results suggest that the GDNF neuroprotectiveeffect might be attributable to a specific modulation of NMDA-inducedCa²⁺ influx.

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Figure 7. rhGDNF pretreatment reduces the NMDA-evoked calcium increase in cortical neurons. A, Intracellular free Ca²⁺ ([Ca²⁺]_i) was measured using fura-2 fluorescence videomicroscopy. Neurons (13-14 DIV) were exposed to a serum-free medium for 45 min in the absence (control, vehicle treated) or presence of rhGDNF (10 ng/ml). Resting [Ca²⁺ ]_i was recorded, and NMDA (100 µM) was applied. [Ca²⁺]_i was measured and analyzed as described in Materials and Methods. B, Representative graph of NMDA-induced Ca²⁺ response in neurons pretreated with rhGDNF (gray bars) or vehicle (control; white bars) for 45 min. Time course of the effect of rhGDNF on the NMDA-induced [Ca²⁺] increase, with (hatched bars) or without (unhatched bars) pretreatment with 0.3 IU/ml PIPLC for 2 hr. Data are expressed as an NMDA-induced fold increase in [Ca²⁺]_i. Results represent the mean ± SEM of three separate preparations (3 coverslips; 20 neurons being imaged per coverslip in a single microscopic field). * indicates significantly different from NMDA; # indicates significantly different from NMDA plus GDNF by ANOVA for repeated measures, followed by a Bonferroni-Dunn's test for multiple comparisons (p < 0.05). C, Neurons (13-14 DIV) were exposed to serum-free medium containing MK-801 (10 µM) for 45 min in the absence (control; vehicle treated) or presence of rhGDNF (10 ng/ml). Resting [Ca²⁺ ]_i was recorded, and KCl (50 mM) was applied. Representative graph of KCl-induced Ca²⁺ response in neurons pretreated with rhGDNF or vehicle (control) for 45 min.

The ERKs signaling pathway is necessary for GDNF attenuation of NMDA-induced Ca²⁺ response

To determine whether the activation of the ERKs pathway by GDNF (Fig. 2B) mediates the neuroprotection against NMDA-inducedneuronal death, we treated mixed cortical neuron-glia cultureswith the MAPK kinase (MEK) inhibitor, U0126. This compound hasbeen described as a specific inhibitor of MEK without any effecton other kinases (Favata et al., 1998). We showed that, althoughthe addition of U0126 alone does not significantly affect cellviability in the presence or absence of NMDA, the neuroprotectiveactivity of GDNF is blocked by the addition of U0126 (1 µM) (Fig.8B) (n = 12; p < 0.05). Concurrently, an immunoblotting studyrevealed that a treatment with U0126 (1 µM) blocks the appearanceof p-ERKs induced by a 15 min application of rhGDNF (10 ng/ml)(Fig. 8A) without modifying the level of p-P38 or p-JNK (datanot shown). We have determined the p-ERK Western blot signal forGDNF in the presence of NMDA with or without U0126. In these experiments,we showed that NMDA plus GDNF induces a greater increase in p-ERKsthan NMDA alone at 15 min (Fig. 8A) and 1 hr (data not shown).This effect is blocked by the addition of the inhibitor of ERKactivation, U0126.

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Figure 8. The MEK kinase inhibitor U0126 blocks the rhGDNF-induced reduction of NMDA-evoked calcium influx. A, Mouse primary cortical neurons were treated for 15 min with rhGDNF (10 ng/ml) in the presence of U0126 (1 µM) and with or without NMDA (12.5 µM). Aliquots of whole-cell lysates were separated by SDS-PAGE, transferred to membranes, and incubated with the anti-MAPK antibody (p-ERKs, ERKs). Representative immunoblots are shown, demonstrating the specific blockade of ERKs phosphorylation by U0126 treatment. B, Neuronal death percentage was estimated by LDH release (mean ± SEM; n = 12) after a 24 hr exposure to NMDA (12.5 µM) in mixed neuron-glia cortical cultures in the presence (gray bars) or absence (white bars) of rhGDNF and treated or not treated with 1 µM U0126. * indicates significantly different from NMDA alone; # indicates significantly different from NMDA plus GDNF by ANOVA, followed by Bonferroni-Dunn's test (p < 0.05). C, Calcium imaging was performed as described in the legend to Figure 7. Neurons (13-14 DIV) were exposed to serum-free medium for 45 min in the absence (control; vehicle treated; white bars) or presence (gray bars) of rhGDNF (10 ng/ml) and with (hatched bars) or without (unhatched bars) U0126 (1 µM). Time course of the effect of rhGDNF on the NMDA-induced [Ca²⁺] increase, with or without treatment with 1 µM of U0126. Data are expressed as an NMDA-induced fold [Ca²⁺]_i. Results represent the mean ± SEM of three separate preparations (3 coverslips; 20 neurons being imaged per coverslip in a single microscopic field). * indicates significantly different from NMDA; # indicates significantly different from NMDA plus GDNF by ANOVA for repeated measures followed by a Bonferroni-Dunn's test for multiple comparisons (p < 0.05).

Finally, to further demonstrate that the ERKs phosphorylation induced by GDNF mediates the neuroprotective activity of GDNF,we studied the effect of the treatment with U0126 on the intracellularCa²⁺ influx induced by NMDA application (100 µM). Although U0126 alone(1 µM for 45 min before NMDA application) did not modify the NMDA-inducedCa²⁺ response, this MEK inhibitor totally abolished the reductionof the NMDA-induced intracellular Ca²⁺ influx that followed incubation with rhGDNF (10 ng/ml for 45min) (Fig. 8C).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Among the multiple roles played by TGF- $beta$ in the CNS, recent studies have suggested that it could be synthesized in responseto different types of injury and act as an endogenous neuroprotectivefactor (Krieglstein and Krieglstein, 1998; Ruocco et al., 1999).According to this hypothesis, GDNF, a distant member of the TGF- $beta$ family, the expression of which is increased in the cortex afterMCAo (Abe et al., 1997), has been identified as a potent neuroprotectiveagent. Indeed, various studies have revealed that the applicationof GDNF reduces the extent of neuronal injury induced by MCAoin rats (Abe et al., 1997; Wang et al., 1997; Kitagawa et al.,1998). However, little is known about the molecular mechanismsinvolved in this effect. Here, we characterize the influence ofGDNF on cortical neurons subjected to two paradigms of injury(necrosis and apoptosis) (Choi, 1992) that have been identifiedduring cerebral ischemia and determine the intracellular mechanism(s)involved. The major findings are as follows: (1) in cortical neurons,GDNF exerts a selective neuroprotective activity against NMDA-inducedneuronal death; (2) this neuroprotective activity of GDNF is causedby a reduction of the NMDA-induced Ca²⁺ influx; and (3) the neuroprotective effect of GDNF involves theactivation ofERKs.

Cortical neurons and astrocytes express functional GDNF receptor complex

To investigate the role of GDNF during ischemic brain injury, we used cortical murine cultures (Goldberg and Choi, 1993).First, we checked whether this culture system was suitable forthe study of the effect of GDNF. We demonstrated that both culturedneurons and astrocytes express the mRNA and the protein for bothGDNF and its receptor complex, GFR $alpha$ -1 and c-Ret. The profile ofexpression identified in cortical cultures is similar to thatobserved in the adult murine cerebral cortex. These data are inaccordance with previous studies (Kitagawa et al., 1999; Wei etal., 2000) and validate the use of cortical murine cultures tostudy the effect of GDNF. Our results also suggest that corticalneurons and astrocytes express the receptor complex necessaryfor the transduction of GDNF signaling. This possibility was confirmedby showing that a GDNF application induces a phosphorylation-mediatedactivation of ERKs in both cortical astrocytes andneurons.

GDNF reduces NMDA-induced neuronal death

To investigate the influence of GDNF during cerebral ischemia, cultured cortical neurons and astrocytes were submitted toapoptotis or excitotoxicity. To examine the effects of GDNF onapoptosis, cortical cell cultures were exposed to two apoptoticchallenges (serum deprivation and staurosporine exposure). Inboth cases, the application of rhGDNF failed to prevent neuronaldeath, whereas cycloheximide succeeded. Because various reportshave described survival-promoting properties of GDNF on dopaminergicand peripheral sensory neurons (Lin et al., 1993; Henderson etal., 1994; Yan et al., 1995), this lack of neuroprotective effectof rhGDNF against apoptosis in cortical cultures is surprising.However, Sawada et al. (2000) recently described a similar lackof neuroprotection exerted by GDNF on mesencephalic neurons exposedto serum deprivation. To the best of our knowledge, there is nodirect proof of an antiapoptotic effect of GDNF on cortical neuronsin the literature. In vivo, although the neuroprotective effectof GDNF evidenced in rats subjected to focal cerebral ischemiawas accompanied by a reduction of apoptotic markers, there wasalso an important reduction in edema formation, one of the landmarksof the necrotic pathway. These authors suggested that GDNF, byattenuating necrosis, could reduce the severity of the insultand, consequently, minimize the appearance of apoptotic markers(Abe et al., 1997). For these reasons, we determined the influenceof rhGDNF incubation on cortical neurons exposed to an excitotoxicinsult. Accordingly, cortical neuronal cultures were exposed todifferent glutamatergic ionotropic receptor agonists. Althoughthe application of rhGDNF failed to prevent AMPA/kainate receptor-mediatedneuronal death, it did protect neurons against NMDA receptor-inducednecrosis. Astrocytes do not seem to be necessary for the antiexcitotoxicactivity of GDNF, because the beneficial effects against NMDA-inducedneuronal death were still observed in pure neuronal cultures.We thus validated the previous observation of an antiexcitotoxiceffect of GDNF demonstrated in a model of excitotoxicity inducedby injection of glutamatergic agonists (Martin et al., 1995; Perez-Navarroet al., 1996; Ho et al., 2000). We demonstrated that rhGDNF directlytargets neurons to protect them against NMDA-inducedinsult.

We further characterized the influence of GDNF on excitotoxicity by demonstrating that pretreatment with PIPLC, an enzymethat specifically cleaves GPI linkages, blocks the beneficialeffect of rhGDNF on NMDA-induced neuronal death. These resultsunderline the implication of a GPI-anchored protein in the neuroprotectionexerted by GDNF against excitotoxicity. The GDNF receptor, GFR $alpha$ -1,is a protein attached to the cell surface by a GPI link. Basedon the above, it can be suggested that GFR $alpha$ -1 is necessary forGDNF to exert its neuroprotective activity against NMDA-inducedneuronaldeath.

Molecular mechanisms of GDNF neuroprotective activity

Among the characteristic features of NMDA receptor activation, two have been particularly implicated in excitotoxicity: first,the initial rise in intracellular calcium concentrations (MacDermottet al., 1986); and second, the consequent production of free radicals(Coyle and Puttfarcken, 1993; Lafon-Cazal et al., 1993). To investigatethe mechanisms by which GDNF is neuroprotective, we tested theeffect of rhGDNF application against free radical-induced neuronaldeath. rhGDNF failed to exert any effect against Fe²⁺-induced neuronal death, a paradigm of neuronal death totallyblocked by the coincubation of the free radical scavenger: thecell permeant derivative of vitamin E, Trolox. The absence ofeffect of GDNF treatment on Fe²⁺-induced neurotoxicity demonstrates that GDNF is not neuroprotectiveby directly scavenging free radicals. However, we cannot excludethat GDNF is protective by reducing intracellular free radicalproduction.

Our next step was to analyze whether rhGDNF incubation modulates calcium influx induced by the application of NMDA. When rhGDNFwas applied to cortical neurons, the Ca²⁺ influx induced by NMDA was reduced. Even after washing out GDNF,the NMDA receptor function is reduced, suggesting that the GDNFapplication triggered an intracellular signaling responsible forthe modulation of the NMDA receptor function. This effect likelyresults from a reduction of NMDA receptor activity rather thanfrom an enhanced Ca²⁺ buffering or extrusion, because the same rhGDNF pretreatmentdid not modify KCl-induced Ca²⁺ influx. These results are in accordance with an increasing setof data that show a tight regulation of glutamatergic receptorfunction by growth factors (Cheng et al., 1995; Boxer et al.,1999). Recent data have demonstrated that the activation of tyrosinekinase-coupled platelet-derived growth factor receptors producesa long-lasting inhibition of NMDA receptor function (Valenzuelaet al., 1996). Because the extent of neuronal injury is directlycorrelated with the intracellular concentration of Ca²⁺ (Hartley et al., 1993), our results may reflect the mechanismthrough which GDNF protects neurons against the toxicity mediatedby the NMDA receptoroverstimulation.

Finally, we investigated the intracellular signaling pathways involved in the neuroprotective effect of GDNF. Many effectsof GDNF are known to be mediated by the activation of the Ras-MAPKpathway (Messer et al., 1999; Ren et al., 1999). Accordingly,we hypothesized that the neuroprotective effect of GDNF mightbe mediated by the activation of the ERKs pathway. To test this,we blocked the ERKs pathway by using a selective inhibitor ofMEK, U0126. We demonstrated that the coapplication of U0126 blocksthe activation of the ERKs and the neuroprotection induced byGDNF on an NMDA-mediated insult, as well as the GDNF-related reductionof the NMDA-induced calcium influx. The present observation thatactivation of ERKs may lead to neuronal survival is consistentwith the previous report of Singer et al. (1999) in which theMAPK pathway mediates estrogen-induced neuroprotection after glutamatetoxicity in primary cortical neurons. Together, these resultsdemonstrate that GDNF, through the activation of the ERKs pathway,modulates the level of activity of the NMDA receptors. This modulationleads to a reduction of Ca²⁺ influx, which consequently helps to restore Ca²⁺ homeostasis and prevents neuronaldeath.

In conclusion, the present study reveals that the binding of GDNF to its neuronal receptors induces the activation of ERKs,leading to a reduction of the NMDA-mediated Ca²⁺ influx. Further investigations are required to determine thelink between ERKs activation and the down-modulation of NMDA receptoractivity. Regarding the neuroprotective profile of GDNF on apoptosisand necrosis described in this study, it can be suggested thatto be beneficial in the treatment of cerebral ischemia, GDNF wouldhave to be administered in the early phase of stroke, when excitotoxicityis predominant. An increase in GDNF expression has been detectedin both CNS and PNS, not only in several paradigms of acute injurysuch as cerebral ischemia (Abe and Hayashi, 1997) but also inmodels reproducing neurological diseases such as Huntington'sdisease and amyotrophic lateral sclerosis (Yamamoto et al., 1998;Grundstrom et al., 1999). Consequently, the inhibitory actionsof GDNF on NMDA receptor function, as evidenced in the presentstudy, could represent an efficient way to reduce the extent ofexcitotoxic neuronal death in these pathophysiologicalsituations.

  FOOTNOTES

Received Oct. 5, 2000; revised Feb. 5, 2001; accepted Feb. 26, 2001.

This work was supported by grants from the Centre National de la Recherche Scientifique and the University of Caen. Doctoralbursaries were provided by Comissariat à l'Energie Atomique (toO.N.), the Regional Council of Lower Normandy (to F.D.), and theMinistry of Education and Research (to C.A.). The investigationwas performed within the framework of the Functional NeuroimagingInstitute (IFR47).
Correspondence should be addressed to Drs. Alain Buisson and Denis Vivien, Université de Caen-Centre National de la RechercheScientifique, Unité Mixte de Recherche 6551, Cyceron, 14074 CaenCedex, France. E-mail: a.buisson{at}neuro.unicaen.fr or d.vivien{at}neuro.unicaen.fr.

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