Glutamate-Dependent Phosphorylation of Elongation Factor-2 and Inhibition of Protein Synthesis in Neurons

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Volume 17, Number 10, Issue of May 15, 1997 pp. 3445-3454
Copyright ©1997 Society for Neuroscience

Glutamate-Dependent Phosphorylation of Elongation Factor-2 and Inhibition of Protein Synthesis in Neurons

Philippe Marin¹, Kent L. Nastiuk², Nadine Daniel¹, Jean-Antoine Girault¹, Andrew J. Czernik², Jacques Glowinski¹, Angus C. Nairn², and Joël Prémont¹
¹ Chaire de Neuropharmacologie, Institut National de la Santé et de la Recherche Médicale U114, Collège de France, 75231 Paris Cedex 05, France, and ² Laboratory of Molecular and Cellular Neuroscience, The Rockefeller University, New York, New York 10021

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Postischemic delayed neuronal death is attributed to excitotoxic activation of glutamate receptors. It is preceded by a persistentinhibition of protein synthesis, the molecular basis of whichis not known. Here we have examined in cortical neurons in culturethe regulation by glutamate of phosphorylation of eukaryotic elongationfactor-2 (eEF-2) by eEF-2 kinase, a Ca²⁺/calmodulin-dependent enzyme. Using a phosphorylation state-specificantibody, we show that glutamate, which triggers a large influxof Ca²⁺, enhances dramatically the phosphorylation of eEF-2. On the basisof kinetic and pharmacological analysis, we demonstrate a closecorrelation among the increase in cytosolic Ca²⁺ concentration, the degree of eEF-2 phosphorylation, and the inhibitionof protein synthesis. A 30 min treatment with NMDA induced a transientphosphorylation of eEF-2 and delayed neuronal death. However,pharmacological inhibition of protein translation was not neurotoxicby itself and protected neurons against the toxicity evoked bylow concentrations of NMDA. Thus, phosphorylation of eEF-2 andthe resulting depression of protein translation may have protectiveeffects against excitotoxicity and open new perspectives for understandinglong-term effects of glutamate.
Key words: elongation factor-2; phosphorylation; calcium; protein translation; glutamate; neuron

INTRODUCTION

Glutamate is the major excitatory neurotransmitter in vertebrate brain, and stimulation of glutamate receptors plays a criticalrole in long-term synaptic plasticity (Bliss and Collingridge,1993; Nicoll and Malenka, 1995). Overstimulation of glutamatereceptors can induce delayed neuronal death, which has been implicatedin the deleterious consequences of brain ischemia as well as inseveral neurodegenerative diseases (Coyle and Puttfarcken, 1993).Several lines of evidence suggest that glutamate inhibits proteinsynthesis in neurons. First, the massive release of glutamateoccurring during cerebral ischemia (Benveniste et al., 1984) seemsto be responsible for a persistent inhibition of neuronal proteinsynthesis, which precedes delayed neuronal death (Thilmann etal., 1986; Raley-Susman and Lipton, 1990). Second, the exposureof brain slices and cultured cerebellar granule cells to glutamateleads to a marked decrease in radioactive amino acid incorporationinto proteins (Orrego and Lipmann, 1967; Vornov and Coyle, 1991;Dessi et al., 1994). However, the mechanism of this inhibitionof protein synthesis is not known.

One important consequence of stimulation of glutamate receptors is a marked increase in cytosolic free Ca²⁺, a necessary step for the effects of glutamate on synaptic plasticityand for the induction of delayed neuronal death (Choi, 1992; Blissand Collingridge, 1993; Nicoll and Malenka, 1995). Studies onprotein translation in non-neuronal systems have indicated a rolefor Ca²⁺ in the inhibition of polypeptide elongation, which results fromthe phosphorylation of eukaryotic elongation factor-2 (eEF-2;for review, see Palfrey and Nairn, 1995). eEF-2 catalyzes thetranslocation of peptidyl-tRNA from the A site to the P site onthe ribosome (Moldave, 1985). This protein is phosphorylated byeEF-2 kinase, a Ca²⁺/calmodulin-dependent enzyme (Nairn and Palfrey, 1987; Ryazanov,1987). eEF-2 is the sole substrate of this kinase and does notappear to be phosphorylated by any other kinase (Mitsui et al.,1993; Redpath and Proud, 1993). Three threonyl residues locatedat the NH₂ terminus of eEF-2 can be phosphorylated by eEF-2 kinasein vitro (Ovchinnikov et al., 1990; Price et al., 1991; Redpathet al., 1993). Phosphorylation of Thr 56 alone seems to be responsiblefor the inhibition of mRNA translation in various cell-free systems(Nairn and Palfrey, 1987; Ryazanov et al., 1988; Redpath et al.,1993). Increases in eEF-2 phosphorylation on Thr 56 have beenreported in living cells exposed to stimuli known to raise intracellularCa²⁺ levels (Palfrey et al., 1987; Mackie et al., 1989; Hincke andNairn, 1992). However, protein synthesis was not studied in theseexperimental systems.

The aim of the present study was to examine in neurons the possible role of phosphorylation of eEF-2 in the regulation ofprotein synthesis by glutamate. For that purpose we used culturedneurons from mouse cerebral cortex and took advantage of a novelapproach, using an antibody that specifically recognizes eEF-2phosphorylated at Thr 56.

MATERIALS AND METHODS
Primary culture of cortical neurons. Primary neuronal cultures were prepared as previously described (Weiss et al., 1986).Cultures, used 11-13 d after seeding, were shown to be highlyenriched in neurons by immunocytochemistry for microtubule-associatedprotein 2 (MAP2; data not shown). Less than 7% of the cells wereimmunoreactive for glial fibrillary acid protein (data not shown).

Production and characterization of antibodies against total or phosphorylated eEF-2 and synapsin I. We previously have developedprocedures to prepare antibodies that specifically recognize theunphosphorylated and phosphorylated forms of identified phosphorylationsites (Snyder et al., 1992; Czernik et al., 1995). The serum thatspecifically recognizes the phosphorylated form of eEF-2 (serumCC81) was obtained by immunization of rabbits with a peptide encompassingeEF-2 phosphorylation sites [GETRFT(P)DTRK]. This peptide wassynthesized, and the threonine at the position corresponding toThr 56 in the native protein was phosphorylated chemically, asdescribed previously (Czernik et al., 1995). The serum recognizingtotal eEF-2 (serum G271) was obtained by immunization of rabbitswith a peptide derived from the same region of the protein (ARAGETRFTDTRKD).

The phosphorylation of purified rabbit eEF-2 was achieved by incubating 350 ng of eEF-2 for increasing times at 30°C in 100µl of medium containing 50 mM HEPES/KOH buffer, pH 7.6, 10 mMMg-acetate, 150 µM CaCl₂, 5 mM dithiothreitol, 20 µg/ml calmodulin,0.4 µg/ml purified eEF-2 kinase, 0.1 mg/ml bovine serum albumin,and [ $gamma$ -³²P]ATP (50 µM, 3000 cpm/pmol; Amersham, Les Ulis, France). Rabbitreticulocyte eEF-2 and eEF-2 kinase were purified as describedpreviously (Mitsui et al., 1993). eEF-2 phosphorylation was determinedby Cerenkov counting after SDS-PAGE. Proteins also were transferredelectrophoretically to nitrocellulose sheets (Hybond-C, Amersham),which were incubated with the antibody directed against the phosphorylatedform of eEF-2 (1:1000 dilution) or with the antibody raised againsttotal eEF-2 (1:1000 dilution). Immunoreactivity was detected withan enhanced chemiluminescence method (Renaissance kit from NewEngland Nuclear, France) using horseradish peroxidase-coupleddonkey anti-rabbit secondary antibodies (Amersham). Immunoreactivebands were quantified by a computer-assisted densitometer (Agfa-GevaertSA, France).

The serum that specifically recognizes synapsin I phosphorylated at site 3 (CaM kinase II phosphorylation site, serum RU19)was produced in rabbit using a phosphopeptide corresponding toresidues 597-607 [GPIRQAS(P)QAGP-amide] of rat synapsin I andwas characterized as described previously (Czernik et al., 1995).The serum recognizing total synapsin I (serum G486) was producedagainst rat synapsin I and was purified over a synapsin I affinitycolumn.

Analysis of eEF-2 and synapsin I phosphorylation in cortical neurons. Neurons grown for 11-13 d in six-well culture disheswere incubated for 2 min, unless otherwise indicated, in 2 mlof Krebs' bicarbonate buffer containing (in mM): 124 NaCl, 3.5KCl, 1.25 K₂HPO₄, 26.3 NaHCO₃, 1.2 CaCl₂, and 10 glucose, previouslyequilibrated with 95% O₂/5% CO₂ and prewarmed at 37°C in the presenceof drugs. Incubations were stopped by replacing the medium with0.2 ml of boiling SDS (1%, w/v) to prevent protein dephosphorylationby phosphatases. Protein concentration was determined with a bicinchoninicacid method (Smith et al., 1985), using bovine serum albumin asstandard. Samples containing 50 µg of protein were resolved on8% polyacrylamide gels and transferred to nitrocellulose. eEF-2phosphorylation was analyzed by sequential immunoblotting withthe antibody specifically recognizing the phosphorylated formof eEF-2 (1:1000 dilution) and that recognizing total eEF-2 (1:1000dilution). The chemiluminescence signals corresponding to differentamounts of purified eEF-2 were used as a calibration curve toestimate the amount of eEF-2 in neuronal homogenates. Similarly,the chemiluminescence signals corresponding to different amountsof purified ³²P-phospho-eEF-2 were used as a calibration curve to determinethe stoichiometry of neuronal eEF-2 phosphorylation. Because theamino acid sequence of eEF-2 is very highly conserved betweenspecies, with the sequence surrounding the phosphorylation sitesbeing completely conserved in human, rat, and hamster, we assumedthat the antibodies reacted equally well with rabbit and mouseeEF-2. Synapsin I phosphorylation was analyzed by sequential immunoblottingwith the antibody specifically recognizing synapsin I phosphorylatedon Ser 603 (1:1000 dilution) and that recognizing synapsin I independentlyof its state of phosphorylation (1:5000 dilution).

Immunocytochemistry experiments. Immunostaining experiments were performed on cortical neurons cultured on glass slides for9-10 d by indirect immunofluorescence, as described by Chamaket al. (1987). Phospho-eEF-2 and total eEF-2 were detected inneurons treated or not for 5 min with glutamate (100 µM), usingthe antibody recognizing either the phosphorylated form of eEF-2(1:1000 dilution) or eEF-2 regardless of its phosphorylation state(1:1000 dilution). These antibodies were visualized by a fluorescein-conjugatedgoat antibody to rabbit IgG (1:100 dilution; Southern BiotechnologyAssociates, Birmingham, AL).

Measurement of eEF-2 kinase activity in cytosolic extracts. Neurons were homogenized in 20 mM Tris HCl, pH 7.6, 1 mM EDTA,and 1 mM EGTA. Samples were centrifuged at 450,000 × g for 6 min.eEF-2 kinase activity was determined in supernatants (cytosolicextracts) as described above, using 5 µg of protein, by measuringthe incorporation of ³²P in 100 ng of purified rabbit eEF-2 in the presence of 1 mM EGTAand, when indicated, 1.5 mM Ca²⁺ and 20 µg/ml calmodulin.

Measurement of [³⁵S]methionine and [³H]leucine incorporation. Neurons grown in 12-well culture dishes were washed twice in 1ml of Krebs' bicarbonate buffer and then incubated for 5 min inthis medium in the presence of drugs and 4 µCi/ml of either [³⁵S]methionine (1000 Ci/mmol, Amersham) or [³H]leucine (159 Ci/mmol, Amersham). The labeling was stopped bytwo washes in 1 ml of ice-cold PBS and the addition of 1 ml ofice-cold trichloroacetic acid (TCA; 10%, w/v). Cells were scraped,and suspensions were centrifuged for 10 min at 10,000 × g. Aminoacid uptake into neurons and incorporation into proteins wereestimated by counting the radioactivity in the supernatant andthe pellet, respectively.

Cytosolic Ca²⁺ measurement. Cytosolic free Ca²⁺ was monitored in neurons cultured on glass slides by quantitative ratio imagingof the fluorescent Ca²⁺ probe INDO-1 (Molecular Probes, Eugene, OR), as described previously(Murphy et al., 1994). Cytosolic Ca²⁺ concentration was calculated according to the equation describedby Grynkiewicz (Grynkiewicz et al., 1985), with a dissociationconstant for INDO-1 (kDa) of 250 nM: [Ca²⁺] = kDa × (F_480f/F_480b) × (R $-$ R_min)/(R_max $-$ R), in which F_480fis the fluorescence of free INDO-1 and F_480b is the fluorescenceof INDO-1 bound to Ca²⁺, R is the ratio between fluorescences measured at 405 and 480nm, and R_min and R_max were determined in the presence of ionomycin(10 µM) and either EGTA (2 mM) or CaCl₂ (2 mM), respectively.

Measurement of neuronal survival. After exposures to glutamate, neurons were incubated with 3-(4,5-dimethylthiazol-2-yl)-2,5,diphenyl tetrazolium bromide (MTT; 0.5 mg/ml) in PBS supplementedwith glucose (33 mM) for 30 min. The blue formazan produced wassolubilized in 1 ml of dimethyl sulfoxide, and optical densitywas read at 560 nm.

RESULTS

Phosphorylation of eEF-2 in cortical neurons exposed to glutamate
The phosphorylation of eEF-2 expressed in cultured cortical neurons was assessed by immunoblot experiments, using an antibodyraised against a peptide encompassing the eEF-2 phosphorylationsites and phosphorylated on a threonyl residue corresponding toThr 56 in the native protein. This antibody specifically recognizedthe phosphorylated form of eEF-2 (phospho-eEF-2). Indeed, whenpurified rabbit eEF-2 was incubated with purified eEF-2 kinaseand [ $gamma$ -³²P]ATP, a time-dependent increase in immunoreactivity measuredby using this antibody occurred concurrently with the increasein phosphorylation level measured by ³²P incorporation (Fig. 1). Treatment of cortical neurons with glutamate(100 µM) resulted in a marked increase in eEF-2 phosphorylation,as measured by using the phospho-eEF-2-specific antibody (Fig.2). The maximal level of eEF-2 phosphorylation induced by glutamatewas achieved in <30 sec and was maintained for at least 5 min(Fig. 2). Immunoblotting experiments performed with an antibodythat recognized total eEF-2 indicated that its amount remainedunchanged in neurons during treatment with glutamate (Fig. 2).
Fig. 1. Analysis of eEF-2 phosphorylation with a phospho-eEF-2 specific antibody. Purified rabbit eEF-2 was incubated with purifiedeEF-2 kinase and [ $gamma$ ³²P]ATP for increasing times. a, Incorporation of ³²P in eEF-2 (35 ng/lane) was detected by autoradiography. b, Aliquotsfrom the same samples were examined by immunoblotting with anantibody raised against a peptide encompassing eEF-2 phosphorylationsites and synthesized with a chemically phosphorylated threoninecorresponding to Thr 56 in the native protein. Immunoreactivitywas detected with a horseradish peroxidase-coupled secondary antibodyusing an enhanced chemiluminescence method and autoradiography.c, Incorporation of ³²P in eEF-2 and in phospho-eEF-2 immunoreactivity was quantifiedby Cerenkov counting and computer-assisted densitometric analysis,respectively.
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Fig. 2. Increase in eEF-2 phosphorylation in cortical neurons exposed to glutamate. Cortical neurons grown in culture for 11-13 dwere incubated with 100 µM glutamate for the indicated times.Cells were harvested in boiling SDS, and proteins (50 µg/lane)were resolved on 8% SDS-polyacrylamide gels and transferred tonitrocellulose sheets. Immunoblotting was performed with the anti-phospho-eEF-2antibody or the antibody reacting with total eEF-2. Immunoreactivebands were detected with a horseradish peroxidase-coupled secondaryantibody, chemiluminescence, and autoradiography. Neurons alsowere preincubated with okadaic acid (OA, 1 µM) for 30 min, andglutamate (GLU, 100 µM) was added to cells for an additional 2min incubation period. The data illustrated are representativeof three experiments, each performed on different sets of culturedneurons.
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The stable level of eEF-2 phosphorylation observed from 0.5 to 5 min after glutamate application suggests an equilibrium betweenthe activities of eEF-2 kinase and phosphatase, which is likelyto be phosphatase 2A (Nairn and Palfrey, 1987; Redpath and Proud,1990). However, during the first minutes of glutamate treatment,phosphatase activity did not appear to be a limiting factor foreEF-2 phosphorylation because okadaic acid, a nonselective inhibitorof phosphatase 2A at the concentration used in our experiments(1 µM), did not significantly enhance the phosphorylation of eEF-2induced by a 2 min exposure to glutamate (112 ± 9% of the glutamateeffect, mean ± SEM of densitometric analyses of immunoreactivebands obtained with the anti-phospho-eEF-2 antibody in three independentexperiments; see also Fig. 2). On the other hand, when it wasadded alone, okadaic acid was unable to increase the phosphorylationof eEF-2 (Fig. 2), suggesting that the activity of eEF-2 kinaseis very low in the absence of glutamate.

Immunocytochemical staining performed with the phospho-eEF-2-specific antibody indicated that a 5 min exposure to 100 µM glutamatestrongly increased the phosphorylation of eEF-2 in ~50% of culturedcortical neurons, whereas no detectable response or a slight increasein immunoreactivity was observed in other neurons (Fig. 3b,d;200 neurons originating from two independent cultures were counted).The phosphorylated form of eEF-2 was not detected in cells withglial morphology after glutamate treatment (data not shown). Asexpected, all cells, including glial cells, were stained withthe antibody recognizing eEF-2 regardless of its phosphorylationstate (Fig. 3e,f). In cells with neuronal morphology, eEF-2 waslocalized in cell bodies as well as in neuronal processes (Fig.3e,f). In contrast, the increase in eEF-2 phosphorylation withinstimulated neurons was detected only in cell bodies and proximalneurites, but not in distal processes (Fig. 3d).
Fig. 3. Immunofluorescent localization of total and phospho-eEF-2 in cortical neurons. a, c, Phase-contrast photomicrographs of untreatedcortical neurons (a) and neurons exposed for 5 min to 100 µM glutamate(c). b, d, Corresponding immunofluorescence photomicrographs usingthe anti-phospho-eEF-2 antibody. e, f, Representative immunofluorescencephotomicrographs of cells exposed to sham treatment (e) or glutamate(f) and immunostained with the antibody recognizing eEF-2 regardlessof its phosphorylation state. No detectable staining was observedin cells incubated only with the secondary antibody to rabbitIgG (not shown). Arrowhead, Neuron insensitive to glutamate treatment.Scale bar, 20 mm.
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Involvement of NMDA and AMPA receptors in the glutamate-induced phosphorylation of eEF-2
We investigated the pharmacological profile of the glutamate response to identify the receptors involved in the regulationof eEF-2 phosphorylation. A 2 min application of maximally effectiveconcentrations of either NMDA (200 µM) or AMPA (30 µM) increasedthe phosphorylation of eEF-2, although AMPA was less efficientthan NMDA (Fig. 4, Table 1). It should be noted that all treatmentswere performed in the absence of extracellular Mg²⁺ to avoid the Mg²⁺- and voltage-dependent block of NMDA-gated channels (Nowak etal., 1984). The study of the effects of antagonists confirmedthe role of both AMPA and NMDA receptors in the regulation ofeEF-2 phosphorylation. Indeed, complete inhibition of the glutamateresponse required the joint application of NMDA and AMPA antagonists,(+)-5-methyl-10,11-dihydro-5H-dibenzo[a,d]-cyclohepten-5,10-iminehydrogen maleate (MK-801, 2 µM) and 6-cyano-2,3-dihydroxy-7-nitroquinoxaline-2,3-dione(CNQX, 100 µM), respectively, whereas either antagonist alonehad only a small effect (Fig. 4). Finally, the selective metabotropicreceptor agonist 1S,3R-trans-(±)-1-amino-1,3-cyclopentanedi-carboxylicacid (trans-ACPD, 300 µM) did not increase significantly eEF-2phosphorylation (Fig. 4, Table 1), indicating that this classof receptor does not contribute to the glutamate-induced phosphorylationof eEF-2 in cortical neurons in culture.
Fig. 4. Role of Ca²⁺ in the phosphorylation of eEF-2 induced by glutamatergic receptor agonists or cell depolarization. Left panel (+Ca²⁺), Cortical neurons were exposed for 2 min to drugs at the followingconcentrations: GLU (100 µM), NMDA (200 µM), AMPA (30 µM), trans-ACPD(ACPD, 300 µM), KCl, 50 mM, MK-801 (MK, 2 µM), and CNQX (100 µM)in Krebs' bicarbonate buffer in the presence of extracellularCa²⁺ and in the absence of Mg²⁺. MK-801 and CNQX were added to cells 1 min before glutamate application.Phosphorylation of eEF-2 was measured by immunoblotting with theanti-phospho-eEF-2 antibody, as described in the legend to Figure2. MK-801 and CNQX, added alone or simultaneously, did not significantlyalter the basal level of eEF-2 phosphorylation in neurons. Rightpanel ( $-$ Ca²⁺), Neurons were incubated in the absence of extracellular Ca²⁺ and in the presence of EGTA (1 mM) for 5 min before drug application.The data illustrated are representative of three experiments,each performed on different sets of cultured neurons.
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Table 1. Correlation between eEF-2 phosphorylation level and cytosolic Ca²⁺ concentration

Treatment Phospho-eEF-2 (% of glutamate effect) [Ca²⁺] (nM)

None 15 ± 5 90 ± 10

trans-ACPD (300 µM) 17 ± 4 94 ± 17

KCl (50 mM) 62 ± 7 489 ± 11

AMPA (30 µM) 78 ± 10 596 ± 44

NMDA (200 µM) 95 ± 1 1080 ± 50

Glutamate (100 µM) 100 1154 ± 65

The phosphorylation level of eEF-2 was estimated after a 2 min incubation period in the presence of the indicated compoundsby immunoblotting, using the anti-phospho-eEF-2 antibody. Dataare the means ± SEM of results obtained by densitometric analysisof immunoreactive bands originating from at least three independentexperiments, each performed on different sets of cultured neurons,and have been expressed in the percentage of the signal evokedby glutamate treatment. Cytosolic Ca²⁺ concentration ([Ca²⁺]) was estimated in INDO-1-loaded cortical neurons 2 min afterthe onset of drug application, as indicated in Materials and Methods.Data represent the means ± SEM of cytosolic Ca²⁺ concentration measured in 14 single neurons originating fromtwo different cultures. The amount of phosphorylated eEF-2 andthe cytosolic Ca²⁺ concentration were significantly correlated (Spearman rank correlationcoefficient, r_s = 1, p < 0.02).

Role of Ca²⁺ in the glutamate-induced phosphorylation of eEF-2
It has been demonstrated that Ca²⁺ is the main factor responsible for the activation of eEF-2 kinase (Mitsui et al., 1993; Redpathand Proud, 1993). Accordingly, a strong correlation was observedbetween the increase in cytosolic free Ca²⁺ concentration and the phosphorylation of eEF-2 induced by varioustreatments in cortical neurons (Table 1). Glutamate and NMDA,which induced the highest increase in cytosolic Ca²⁺ concentration, were also the most effective agonists in stimulatingeEF-2 phosphorylation (Table 1). A 2 min application of the maximallyeffective concentration of AMPA (30 µM) or potassium-induced depolarization(KCl, 50 mM) led to both intermediate elevations of cytosolicCa²⁺ concentration and phosphorylation level of eEF-2 (Table 1).Despite its ability to stimulate phospholipase C in cortical neurons(Trovéro et al., 1994), trans-ACPD was unable to increase cytosolicCa²⁺ in this neuronal population. This is in agreement with its lackof effect on eEF-2 phosphorylation (Table 1). Further supportingthe role of Ca²⁺ in the regulation of eEF-2 phosphorylation, both the elevationof cytosolic Ca²⁺ (data not shown) and the phosphorylation of eEF-2 induced bythe aforementioned treatments were suppressed in the absence ofextracellular Ca²⁺ and the presence of 1 mM EGTA (Fig. 4). However, it should benoted that removal of extracellular Ca²⁺ by itself caused a slight increase in the level of eEF-2 phosphorylation(Fig. 4).

Reversibility of the glutamate-induced phosphorylation of eEF-2
To investigate the reversibility of the glutamate-induced phosphorylation of eEF-2, we added glutamate (100 µM) to cells for30 sec. In this experimental condition, cytosolic Ca²⁺ concentration increased transiently and returned to the basallevel in <2 min (Fig. 5). The level of eEF-2 phosphorylation decreasedwith a slower time course, the complete dephosphorylation of eEF-2occurring within 5 min (Fig. 5).
Fig. 5. Reversibility of eEF-2 phosphorylation induced by glutamate. Cortical neurons, loaded with INDO-1, were exposed for 30 secto 100 µM glutamate. Variations in cytosolic Ca²⁺ concentration (ratio between the fluorescence measured at 405and 480 nm: F₄₀₅/F₄₈₀) were measured for 5 min. A typical tracerepresentative of those obtained in 28 neurons originating fromtwo independent cultures is illustrated. The black horizontalbar indicates the period of exposure to glutamate. eEF-2 phosphorylationwas measured at various times after glutamate application (filledsymbols). Quantified data were obtained from the densitometricanalysis of a representative immunoblot by using the anti-phospho-eEF-2antibody and were expressed in the percentage of the phosphorylationlevel, measured at 30 sec of glutamate incubation time. Anotherexperiment performed on a different set of cultured neurons yieldedsimilar results.
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Correlation between eEF-2 phosphorylation and protein synthesis inhibition
Using purified unphosphorylated and phosphorylated rabbit eEF-2 as standards, we estimated that cortical neurons contained7.5 ± 0.5 µg of eEF-2/mg protein (mean ± SEM of three determinationsperformed on different cultures, n = 3) and that 44 ± 5% (n =3) of eEF-2 was phosphorylated after a 2 min glutamate treatment.This relatively high stoichiometry of phospho-Thr 56 raised thepossibility that eEF-2 phosphorylation was involved in glutamate-dependentinhibition of protein translation in cortical neurons. We observeda strong inhibition of [³⁵S]methionine incorporation into proteins in cortical neurons exposedto agonists of ionotropic glutamate receptors or a depolarizingconcentration (50 mM) of KCl (Fig. 6). Similar results were obtainedwith [³H]leucine (data not shown). It should be noted that the uptakeof either amino acid, as estimated by the radioactivity recoveredin the TCA soluble fraction, was not affected significantly byglutamatergic agonists or cell depolarization (data not shown).A striking correlation was observed between the ability of thevarious treatments to increase eEF-2 phosphorylation and theirefficacy to inhibit protein synthesis (Fig. 6). Moreover, as demonstratedabove for eEF-2 phosphorylation, the inhibition of protein synthesisevoked by a 5 min exposure to glutamate involved both NMDA andAMPA receptors. The inhibitory effect of glutamate on proteinsynthesis was antagonized only by the combined application ofMK-801 and CNQX, whereas either antagonist applied separatelyreversed only partially the response to glutamate (Table 2).As expected, trans-ACPD, which failed to increase cytosolic Ca²⁺ concentration and eEF-2 phosphorylation, did not inhibit [³⁵S]methionine incorporation into proteins in cortical neurons (Fig.6). In agreement with the major role of Ca²⁺ in eEF-2 phosphorylation, the inhibition of protein synthesisinduced by glutamate receptor agonists was suppressed when Ca²⁺ was removed and 1 mM EGTA was added to the incubation medium(data not shown). Interestingly, in this experimental conditionthe basal incorporation of [³⁵S]methionine into proteins was inhibited by 21 ± 2% (mean ± SEMfrom three independent experiments). This might be explained bythe concomitant increase in the level of eEF-2 phosphorylationafter the removal of extracellular Ca²⁺ (Fig. 4).
Fig. 6. Correlation between the increase in eEF-2 phosphorylation and inhibition of [³⁵S]methionine incorporation into proteins. The increase in eEF-2phosphorylation induced by a 2 min application of GLU (100 µM),NMDA (200 µM), AMPA (30 µM), trans-ACPD (ACPD, 300 µM), and KCl(50 mM), expressed in arbitrary units, was quantified by densitometricanalysis of immunoreactive bands in immunoblotting experimentsperformed with the anti-phospho-eEF-2 antibody and plotted asa function of the inhibition of [³⁵S]methionine incorporation into proteins induced by the same treatmentsperformed in Krebs' bicarbonate buffer (r = 0.996, p < 0.001).[³⁵S]Methionine incorporation was calculated as the ratio of TCA-precipitableto TCA-soluble radioactivity and expressed as the percentage ofinhibition of the basal incorporation measured during 5 min (230,500± 17,000 dpm/mg protein, n = 3). Values are mean ± SEM of thedata obtained in three experiments, each performed in triplicateon different cultures.
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Table 2. Contribution of AMPA and NMDA receptors to the glutamate-induced inhibition of protein synthesis

Treatment [³⁵S]Methionine incorporation (% of basal)

None 100 ± 7

MK-801 (2 µM) 112 ± 8

CNQX (100 µM) 94 ± 11

CNQX + MK-801 108 ± 11

GLU (100 µM) 54 ± 5^a

GLU + MK-801 71 ± 9^a

GLU + CNQX 59 ± 5^a

GLU + MK-801 + CNQX 91 ± 5

Neurons were exposed to antagonists for 1 min in Krebs' bicarbonate buffer before a 5 min incubation period in the presenceof [³⁵S]methionine (4 µCi/ml). [³⁵S]Methionine incorporation, expressed in the percentage of themean of basal [³⁵S]methionine incorporation measured in the absence of any treatment(230,500 ± 17,000 dpm/mg protein, n = 3), was measured as indicatedin the legend to Figure 6. None of these treatments altered significantlythe amount of TCA-soluble [³⁵S]methionine, indicating that they did not modify methionine uptakeinto neurons. All values are the means ± SEM of data obtainedin three experiments, each performed in triplicate on three differentsets of cultured neurons. ^a Significantly different (p < 0.01) from basal [³⁵S]methionine incorporation (ANOVA, followed by Dunnett's test).

Effects of prolonged treatment with glutamate on eEF-2 phosphorylation and protein synthesis
A persistent and Ca²⁺-dependent inhibition of protein synthesis, together with a massive release of glutamate, has been describedafter cerebral ischemia (Benveniste et al., 1984; Raley-Susmanand Lipton, 1990). To mimic the effects of the pathological releaseof glutamate, we exposed cortical neurons to glutamate (100 µM)for prolonged periods of time (up to 60 min). This treatment resultedin a sustained increase in cytosolic Ca²⁺ concentration (Fig. 7a). Neuronal viability was not altered immediatelyafter the 60 min glutamate treatment because cellular respiration,assessed by the MTT staining method, was not decreased significantly(data not shown). This contrasted with the delayed neuronal deathobserved 24 hr after this treatment (26 ± 5% of cell survivalmeasured in three independent experiments).
Fig. 7. Effects of prolonged treatments with glutamate on cytosolic Ca²⁺, protein synthesis, eEF-2 and synapsin I phosphorylation, andCa²⁺ dependency of eEF-2 kinase activity. a, Cytosolic Ca²⁺ concentration was measured for 60 min in INDO-1-loaded corticalneurons exposed to 100 µM glutamate. A typical trace representativeof those obtained in 28 different neurons originating from twoindependent cultures is illustrated. The horizontal black barindicates the incubation period in the presence of glutamate.b, Cortical neurons were exposed to 100 µM glutamate added directlyto the culture medium for the indicated times. [³⁵S]Methionine (1000 Ci/mmol, 4 µCi/ml) or [³H]leucine (159 Ci/mmol, 4 µCi/ml) then was added to the culturemedium for the last 5 min of the incubation period in the presenceof glutamate. Results were calculated as indicated in the legendto Figure 6 and expressed in the percentage of basal [³⁵S]methionine (99,500 ± 1950 dpm/mg protein, n = 3) or [³H]leucine (76,900 ± 5900 dpm/mg protein, n = 3) incorporationinto proteins. c, The phosphorylation state of eEF-2 was measuredby immunoblotting, using the anti-phospho-eEF-2 antibody and theantibody recognizing total eEF-2 after various times of exposureto glutamate. The phosphorylation state of synapsin I on site3 was estimated in the same experimental conditions by sequentialimmunoblotting with an anti-phospho-synapsin I antibody (1:1000dilution) and an antibody that reacts with synapsin I independentlyof its state of phosphorylation (1:5000 dilution). d, eEF-2 kinaseactivity was determined in cytosolic extracts obtained from corticalneurons exposed for the indicated times to glutamate (Glu) andcontaining 5 µg of protein by measuring the incorporation of ³²P in 100 ng of purified rabbit eEF-2 in the presence of either1 mM EGTA, 1.5 mM Ca²⁺ and 20 µg/ml calmodulin (+ Ca/CaM), or 1 mM EGTA alone ( $-$ Ca/CaM).Incorporation of ³²P in eEF-2 was quantified by Cerenkov counting. Results are themeans of three determinations, each performed on different setsof cultured neurons.
[View Larger Version of this Image (29K GIF file)]

The rate of protein synthesis was studied in the same experimental conditions by measuring amino acid incorporation duringthe last 5 min of glutamate treatment. To prevent any modificationof endogenous amino acid concentration and, therefore, any changein the specific radioactivity of labeled amino acids, we addedglutamate and radioactive amino acids directly to the culturemedium without washing. With this procedure, a short (5 min) exposureto glutamate (100 µM) decreased the incorporation of [³⁵S]methionine and [³H]leucine by 58 ± 5 and 69 ± 2% (n = 3), respectively (Fig. 7b),similarly to what was measured in Krebs' bicarbonate buffer. Theinhibition of [³⁵S]methionine and [³H]leucine incorporation remained sustained during prolonged glutamateapplication periods (up to 60 min, Fig. 7b). In the same experimentalconditions, the level of eEF-2 phosphorylation remained elevatedas compared with the basal level, although a slow decrease wasobserved during prolonged treatment ( $>=$ 30 min) of cortical neuronswith glutamate (Fig. 7c). This decrease in immunoreactivity measuredwith the anti-phospho-eEF-2 antibody was not attributable to proteolysis,because the total amount of eEF-2 remained unchanged (Fig. 7c).

The autophosphorylation of eEF-2 kinase has been reported to lead to a partial Ca²⁺-independent activity (Mitsui et al., 1993; Redpath and Proud,1993). However, this process seems unlikely to contribute to theprolonged increase in eEF-2 phosphorylation, because eEF-2 kinaseactivities measured in cytosolic extracts from neurons exposedto glutamate (100 µM) for 5 or 60 min remained strictly Ca²⁺-dependent (Fig. 7d). On the other hand, a prolonged exposureto glutamate (60 min) resulted in a partial decrease in Ca²⁺-dependent eEF-2 kinase activity (Fig. 7d). This decreased activitymay account for the decrease in the amount of phosphorylated eEF-2measured after prolonged glutamate treatments.

It has been reported that the multifunctional Ca²⁺/calmodulin-dependent protein kinase II (CaM kinase II) is strongly downregulatedin neurons during prolonged exposure to glutamate (Churn et al.,1995; Morioka et al., 1995). We compared the phosphorylation ofeEF-2 with that of synapsin I, a major neuronal substrate forCaM kinase II, using an antibody that reacts specifically withsynapsin I phosphorylated on Ser 603 (site 3), a residue onlyphosphorylated by CaM kinase II (Czernik et al., 1995). Duringprolonged treatment with glutamate, the phosphorylation of synapsinI was transient (Fig. 7c), in contrast to the persistent phosphorylationof eEF-2.

Role of eEF-2 phosphorylation in NMDA receptor-mediated neurotoxicity
Further experiments were performed to determine the role of eEF-2 phosphorylation and the associated inhibition of proteintranslation in a classical paradigm of NMDA receptor-mediatedneurotoxicity. When cortical neurons were exposed for 30 min toNMDA (100 µM), a transient phosphorylation of eEF-2 preceded neuronaldeath by several hours (Fig. 8). The transitory phosphorylationof eEF-2 was followed by a decrease in the Ca²⁺-dependent eEF-2 kinase activity, which was observed after theremoval of NMDA (Fig. 8c). This decrease in eEF-2 kinase activitymay contribute to the transient nature of eEF-2 phosphorylationdespite the persistent elevation of intracellular free Ca²⁺, which occurs after prolonged NMDA treatments (Schinder et al.,1996). The residual eEF-2 kinase activity measured in these experimentalconditions also remained strictly Ca²⁺-dependent (data not shown).
Fig. 8. Comparison of the amount of phosphorylated eEF-2, eEF-2 kinase activity, and neuronal survival after NMDA treatment. Corticalneurons were exposed to 100 µM NMDA for 30 min. The phosphorylationstate of eEF-2 was measured at various times after the onset ofNMDA application by sequential immunoblotting, using the anti-phospho-eEF-2antibody (a) and the antibody recognizing total eEF-2 (b). Thedata illustrated are representative of two experiments, each performedon different sets of cultured neurons. c, Phospho-eEF-2 immunoreactivityhas been quantified by computer-assisted densitometric analysis.Ca²⁺/CaM-dependent eEF-2 kinase activity also was determined in thesame experimental conditions. Neuronal survival (indicated ininset) was measured at the indicated times and is expressed asthe percentage of cells surviving compared with that in the absenceof any treatment. Results are the mean ± SEM of values obtainedin three independent experiments.
[View Larger Version of this Image (35K GIF file)]

To determine the possible role of protein synthesis inhibition in neuronal death, we have examined the effects of cycloheximideand diphtheria toxin, two drugs that block polypeptide chain elongation,as does eEF-2 phosphorylation. Neither cycloheximide (1 µg/ml,12 hr) nor diphtheria toxin (10 nM, 12 hr) treatments, both ofwhich depressed strongly neuronal protein synthesis (by 89 ± 4and 73 ± 6%, n = 3, respectively), triggered neuronal death. Onthe contrary, both treatments protected neurons against the neurotoxiceffect evoked by a low concentration of NMDA (10 µM), but notthat evoked by a higher concentration (100 µM; Table 3). Pretreatmentof neurons with cycloheximide or diphtheria toxin had no effecton the increase in cytosolic Ca²⁺ induced by both 10 and 100 µM NMDA (data not shown). These observationssuggest that eEF-2 phosphorylation and the resulting inhibitionof protein translation may constitute a protective mechanism againstNMDA receptor-mediated neurotoxicity.

Table 3. Effects of protein translation inhibitors on NMDA receptor-mediated neurotoxicity

Treatment Neuronal survival (%)

None Cycloheximide Diphtheria toxin

None 100 100 ± 1 99 ± 2

NMDA (10 µM) 79 ± 4 96 ± 4^a 100 ± 5^a

NMDA (100 µM) 47 ± 2 55 ± 6 42 ± 1

Cortical neurons were exposed to the indicated concentrations of NMDA for 30 min. Cycloheximide (1 µg/ml) was added to cellsfor 30 min before, during, and for 2 hr after the NMDA incubationperiod. Diphtheria toxin (10 nM) was applied to cells 12 hr beforethe NMDA treatment. Neuronal survival was estimated 24 hr afterthe onset of NMDA application by measuring the rate of MTT reduction.Results, expressed in the percentage of the neuronal survivalestimated in the absence of any treatment, are the means ± SEMof values obtained in three independent experiments, each performedin triplicate on different sets of cultured neurons. ^a Significantly different (p < 0.01) from the neuronal survival estimated 24 hr after a 10 µM NMDA treatment (ANOVA, followedby Student-Newman-Keuls test).

DISCUSSION
Inhibition of protein synthesis in brain slices by excitatory amino acids was reported almost 30 years ago (Orrego and Lipmann,1967). Our results provide a possible mechanism that may contributeto this hitherto unexplained observation. Indeed, several linesof evidence suggest strongly that Ca²⁺-dependent phosphorylation of eEF-2 is involved in the inhibitionof protein synthesis by glutamate. First, it has been clearlydemonstrated in reconstituted systems in vitro that phosphorylationof eEF-2 by eEF-2 kinase, a Ca²⁺-dependent enzyme, inhibits protein translation (Nairn and Palfrey,1987; Ryazanov et al., 1988). Second, treatment of cortical neuronswith glutamate resulted concomitantly in the phosphorylation ofeEF-2 to a stoichiometry of ~0.5 and in a 50% inhibition of proteinsynthesis. Moreover, immunofluorescence experiments using theanti-phospho-eEF-2 antibody indicated that only one-half of theneurons were strongly stained in response to glutamate. This suggeststhat the stoichiometry of eEF-2 phosphorylation is very high ina subset of glutamate-treated neurons. Third, a perfect correlationwas observed among the increase in cytosolic Ca²⁺ concentration, the degree of eEF-2 phosphorylation, and the amplitudeof protein synthesis inhibition in cortical neurons exposed toglutamatergic agonists or a depolarizing agent (glutamate > NMDA> AMPA > KCl $>>$ trans-ACPD). Finally, the phosphorylation of eEF-2and the inhibition of protein synthesis were both totally dependenton the presence of extracellular Ca²⁺.

The role of the phosphorylation of eEF-2 by eEF-2 kinase in the inhibition of protein synthesis has, to date, been investigatedonly in cell-free translation systems (Nairn and Palfrey, 1987;Ryazanov et al., 1988). Our study provides strong evidence thatan increase in cytosolic Ca²⁺ and the resulting eEF-2 phosphorylation are also responsiblefor an inhibition of protein synthesis in living cells. Phosphorylationof eEF-2 may be of particular importance in neurons in which glutamateinduces sustained and prolonged cytosolic Ca²⁺ elevations differing from the transient nature of Ca²⁺ increases induced by different effectors in most non-neuronaltissues (Palfrey and Nairn, 1995).

Besides the phosphorylation of eEF-2, the phosphorylation of the eukaryotic initiation factor eIF-2 $alpha$ by double-stranded RNA-regulatedprotein kinase (PKR) constitutes another potential Ca²⁺-dependent mechanism contributing to inhibition of protein synthesis(Prostko et al., 1995; Srivastava et al., 1995). The phosphorylationof eIF-2 $alpha$ by PKR apparently is not related to an increase in cytosolicCa²⁺ concentration but, rather, to a depletion of intracellular Ca²⁺ stores after long-term Ca²⁺ deprivation or treatment with Ca²⁺ mobilizing agents (Prostko et al., 1995; Srivastava et al., 1995).Because the inhibition of protein synthesis induced by glutamatewas strictly dependent on the presence of extracellular Ca²⁺, a role of intracellular Ca²⁺ stores is unlikely. On the other hand, Ca²⁺ store depletion could be involved in the slight inhibition ofprotein synthesis observed when cortical neurons were incubatedfor 5 min in the absence of extracellular Ca²⁺ and in the presence of EGTA. However, this decrease in proteinsynthesis also could be related to the small increase in eEF-2phosphorylation observed in this experimental condition.

Neuronal, but not glial, protein synthesis is believed to be persistently inhibited during the reperfusion phase of cerebralischemia (Raley-Susman and Lipton, 1990). The massive releaseof glutamate that occurs in this pathological situation (Benvenisteet al., 1984) may be responsible for the sustained inhibitionof neuronal protein synthesis. During prolonged treatments ofcortical neurons with glutamate, we observed a persistent phosphorylationof eEF-2, which was accompanied by a prolonged inhibition of proteinsynthesis. The prolonged phosphorylation of eEF-2 probably resultedfrom the persistent increase in cytosolic Ca²⁺. Indeed, eEF-2 kinase activity remained completely Ca²⁺-dependent, even after a prolonged exposure to glutamate, rulingout a role for the autophosphorylation of the kinase (Mitsui etal., 1993; Redpath and Proud, 1993). eEF-2 phosphorylation observedduring a 60 min exposure to glutamate may be explained by theslight diminution of eEF-2 kinase activity, which occurs in thesame experimental condition. In contrast to the sustained phosphorylationof eEF-2 observed during prolonged exposure to glutamate, thephosphorylation of synapsin I was only transient in cortical neurons.The rapid decrease in the phosphorylation of synapsin I may resultfrom the rapid downregulation of CaM kinase II, already describedin hippocampal neurons (Churn et al., 1995; Morioka et al., 1995).The contrast between the phosphorylation of eEF-2 and that ofsynapsin I during a prolonged treatment with glutamate emphasizesthe diversity in the time course of various Ca²⁺-activated processes in response to persistent increases in cytosolicCa²⁺.

It has been proposed recently that glutamate induces either apoptotic or necrotic neuronal cell damage, depending on the intensityand the duration of the stimulation of NMDA receptors (Bonfocoet al., 1995). Apoptosis is an active process requiring proteinsynthesis and thus is suppressed by protein synthesis inhibitors.Accordingly, cycloheximide, an elongation inhibitor, protectedselectively cortical neurons against the neurotoxicity inducedby a low concentration of NMDA, as it already has been describedfor retinal ganglion cells (Dreyer et al., 1995). Furthermore,diphtheria toxin treatment, which leads to ADP-ribosylation ofeEF-2 and inhibition of its activity, also protected corticalneurons against cell damage evoked by a low concentration of NMDA.Therefore, inhibition of protein translation resulting from eEF-2phosphorylation may represent a self-protective mechanism againstglutamate neurotoxicity.

In addition to its possible role in glutamate-induced neuronal death, eEF-2 phosphorylation and the associated inhibitionof protein synthesis also may be involved in the modulation ofnormal physiological processes. It has been proposed that transientinhibition of protein synthesis by Ca²⁺-induced phosphorylation of eEF-2 may lead to an alteration inthe pattern of protein expression (Ryazanov and Spirin, 1993;Palfrey and Nairn, 1995). Several mechanisms have been proposedto account for changes in protein expression after a transientinhibition of protein synthesis. First, it has been suggestedthat short-lived proteins are involved in the destabilizationof specific mRNAs (for review, see Palfrey and Nairn, 1995). Transientinhibition of protein synthesis resulting from eEF-2 phosphorylationcould lead to the rapid disappearance of these destabilizing proteinsand, consequently, to a decrease in the degradation of normallyunstable mRNAs. For instance, a striking effect of inhibitorsof protein synthesis such as cycloheximide is the superinductionof the expression of immediate-early gene mRNAs, including c-fos,c-jun, and c-myc, that have very short half-lives (Greenberg etal., 1986; Cleveland and Yen, 1989). Inhibition of protein translationalso can lead to the disappearance of proteins involved in thestabilization of some mRNAs. This may account for the destabilizationof ligatin mRNA via a Ca²⁺-dependent mechanism observed in cultured hippocampal neuronstreated with glutamate (Jakoi et al., 1995; Panchision et al.,1995). Second, many transcription factors are themselves turnedover rapidly, and it has been speculated that eEF-2 phosphorylation,by regulating the level of such factors, leads to a new patternof gene expression (Ryazanov and Spirin, 1993; Palfrey and Nairn,1995). Finally, elongation block, by stalling polypeptide extension,could force free ribosomal subunits to engage other mRNAs (Palfreyand Nairn, 1995). Thus, transient phosphorylation of eEF-2 couldreset the protein translation machinery and participate in thetranscriptional and translational regulations brought about bythe various Ca²⁺-activated pathways.

Translational control involving eEF-2 phosphorylation potentially could contribute to the regulation of other glutamate-dependentprocesses in neurons. The induction of long-term potentiation(LTP) in several brain regions, including the CA1 area and thedentate gyrus of the hippocampus, requires a rise in cytosolicCa²⁺ concentration resulting from the activation of postsynaptic NMDAreceptors (Bliss and Collingridge, 1993; Nicoll and Malenka, 1995).The application of protein synthesis inhibitors during the inductionof LTP reduces its duration to 3-6 hr, indicating that a criticallevel of protein synthesis is required for extension of LTP beyondseveral hours (for review, see Bliss and Collingridge, 1993).Transient phosphorylation of eEF-2 during the induction of LTPcould interrupt ongoing protein synthesis, allowing the establishmentof a new pattern of protein translation required for the maintenanceof LTP. Interestingly, a selective enrichment in dendrites ofspecific mRNAs, including those encoding for MAP2 and the $alpha$ subunitof CaM kinase II, has been reported (for review, see Steward,1995). Despite the homogenous distribution of eEF-2 in corticalneurons, the location of its phosphorylated form appears to berestricted to cell bodies and proximal processes. This offersthe potential for local regulation of the translation of specificproteins in the vicinity of postsynaptic sites in response tolocal increases in cytosolic Ca²⁺ concentration, which are required for the subsequent events leadingto LTP. Therefore, the phosphorylation of eEF-2 and its consequenceson translational control in neurons open up new perspectives forunderstanding acute as well as long-term effects of glutamate.

FOOTNOTES

Received Dec. 23, 1996; revised Feb. 21, 1997; accepted Feb. 27, 1997.

This research was supported by grants from Institut National de la Santé et de la Recherche Médicale (INSERM), Directiondes Recherches, Etudes et Techniques (DRET, contract 94/158),and Rhône Poulenc Rorer to J.P.; and United States Public HealthService Grant GM 50402 to A.C.N. We thank Gloria Bertuzzi fortechnical assistance and Dr. Kenichi Mitsui for preparation ofeEF-2 and eEF-2 kinase.

Correspondence should be addressed to Dr. Joël Prémont, Chaire de Neuropharmacologie, Institut National de la Santé etde la Recherche Médicale U114, Collège de France, 11, PlaceMarcelin Berthelot, 75231 Paris Cedex 05, France, or Dr. AngusC. Nairn, Laboratory of Molecular and Cellular Neuroscience, TheRockefeller University, New York, New York 10021.

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Glutamate-Dependent Phosphorylation of Elongation Factor-2 and Inhibition of Protein Synthesis in Neurons

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