Phosphorylation of cAMP Response Element-Binding Protein in Hippocampal Neurons as a Protective Response after Exposure to Glutamate In Vitro and Ischemia In Vivo

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The Journal of Neuroscience, December 1, 2001, 21(23):9204-9213

Phosphorylation of cAMP Response Element-Binding Protein in Hippocampal Neurons as a Protective Response after Exposure to Glutamate In Vitro and Ischemia In Vivo
Takuma Mabuchi¹, Kazuo Kitagawa¹, Keisuke Kuwabara¹, Kenichiro Takasawa¹, Toshiho Ohtsuki¹, Zhengui Xia³^,⁴, Daniel Storm⁴, Takehiko Yanagihara², Masatsugu Hori¹, and Masayasu Matsumoto¹^,²
¹ Division of Strokology, Department of Internal Medicine and Therapeutics and ² Department of Clinical Neuroscience, Osaka University Graduate School of Medicine, Osaka 565-0871, Japan, and Departments of ³ Environmental Health and ⁴ Pharmacology, University of Washington, Seattle, Washington 98195

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although accumulating evidence indicates that cAMP response element-binding protein (CREB) phosphorylation mediates not onlysynaptic plasticity but also survival of certain neurons, it remainsuncertain whether CREB phosphorylation induced after metabolicinsult leads to CRE-mediated gene transcription and is involvedin cell survival or not. In the present study, we clarified that(1) CREB phosphorylation and ischemic tolerance induced afterpreconditioning ischemia in the hippocampal neurons was abolishedby MK801 administration in gerbil global ischemia model, (2) CREBphosphorylation induced after exposure to glutamate in culturedneurons was inhibited by removal of extracellular calcium, byMK801 and by an inhibitor of calcium-calmodulin-dependent proteinkinase (CaMK) II and IV, (3) inhibitor of CaMK II-IV or CRE-decoyoligonucleotide suppressed upregulation of BCL-2 expression andaccelerated neuronal damage after exposure to glutamate, and (4)CREB phosphorylation induced in the hippocampal neurons afterischemia and in cultured neurons after exposure to glutamate wasfollowed by CRE-mediated gene transcription in transgenic micewith a CRE-LacZ reporter. Our results suggest that CREB phosphorylationin neurons after ischemia and exposure to glutamate is inducedby NMDA receptor-gated calcium influx and subsequent activationof CaMK II-IV and that CREB phosphorylation after metabolic stressmight show a neuroprotective response through CRE-mediated geneinduction.

Key words: CREB; ischemia; BCL-2; $beta$ -galactosidase; glutamate; CRE-decoy oligonucleotide

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ischemic stress has been known to induce expression of various genes in neurons (Lipton, 1999), and some of the gene productsare believed to play key roles in cellular adaptive responses,such as ischemic tolerance (Kitagawa et al., 1990; Kirino et al.,1991) and cell death mechanisms such as apoptosis (Ninatori etal., 1995). Therefore, elucidation of the molecular mechanismfor gene expression in neurons after ischemic insult is importantin developing novel strategies against stroke. It is widely knownthat heat shock protein (HSP) genes are induced after ischemicinsult (Yagita et al., 1999), in which activation and bindingof heat shock factor to heat shock element in the promotor regionof each HSP gene (Morimoto, 1993) is a key step in induction ofHSP expression (Higashi et al., 1995). Several other genes inducedafter ischemia, including c-Fos (Kiessling et al., 1993) and brain-derivedneurotrophic factor (BDNF) (Lindvall et al., 1992), have a consensuscAMP response element (CRE, TGACGTCA) in the promoter region (Shenget al., 1990; Shieh et al., 1998), suggesting the activation ofCRE-binding protein (CREB) after ischemia. CREB is abundant inthe brain and particularly in neurons. Phosphorylation of theSer-133 residue is necessary but not sufficient for activationof CRE-mediated gene transcription (Hu et al., 1999). Diverseextracellular stimuli cause phosphorylation of CREB by proteinkinase A (PKA), extracellular signal-related protein kinase (ERK),and calcium-calmodulin-dependent protein kinase (CaMK) (Finkbeiner,2000), and CREB phosphorylation has recently been found to beimportant in both activity-dependent neuronal plasticity and neurotrophin-mediatedneuronal survival (Ghosh and Greenberg, 1995; Bonni et al., 1999;Riccio et al., 1999). It was also suggested that CREB phosphorylationin response to brain insults (Walton and Dragunow, 2000) or activitydeprivation by deafferentation (Zirpel et al., 2000) might beinvolved in nerve cell survival. Although CREB phosphorylationin the cultured neurons after glutamate (Hardingham et al., 1999)and NMDA (Sala et al., 2000) treatment was examined, the signalpathway leading to CREB phosphorylation and its functional roleafter ischemic stress or exposure to glutamate are not fully elucidated.In the present study, we aimed at clarifying the relation betweenthe severity of insults and CREB phosphorylation, and the relationbetween CREB phosphorylation and CRE-mediated gene transcription,and finding the upstream pathway leading to CREB phosphorylationand the functional role of CREB phosphorylation in neuronalinjury.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Animals used in the present study were fed standard laboratory chow and given ad libitum access to water before surgery.All experimental procedures were approved by the InstitutionalAnimal Center Use Committee of the Osaka University Graduate Schoolof Medicine. CRE-LacZ transgenic mice were obtained from a colonyat the University of Washington (Seattle, WA) (Imprey et al.,1996) and backcrossed at least six generations to wild-type C57BL/6mice (Charles River, Yokohama, Japan). The transgene was maintainedexclusively in heterozygotes. Mice were genotyped by PCR as described(Imprey et al., 1996).

Chemicals and reagents. The following drugs were used: (+)-MK801 (Sigma, St. Louis, MO), CNQX (Sigma), nifedipine (Sigma),EGTA (Sigma), Rp-8-Cl-cAMPs (Biolog, Hayward, CA), KT5720 (Calbiochem,San Diego, CA), chelerythrine (Calbiochem), Rp-8-Br-cGMPs (Biolog),KN93 (Seikagaku, Tokyo, Japan; Alexis, San Diego, CA), PD98059(Calbiochem), genistein (Sigma), wortmannin (Sigma), and staurosporine(Alexis). All polyclonal antibodies, anti-CREB (Upstate Biotechnology,Lake Placid, NY), anti-phosphoCREB (Upstate Biotechnology), andanti-microtubule-associated proteins (MAPs) (Sigma) had been raisedin rabbits. Anti-NeuN (Chemicon, Temecula, CA), anti- $alpha$ -tubulin(Sigma), anti-microtubule-associated protein 2 (MAP2) (Sigma),anti-BCL-2 (Santa Cruz Biotechnology, Santa Cruz, CA), and anti- $beta$ -galactosidase(Santa Cruz Biotechnology) were monoclonalantibodies.

Transient global ischemia in gerbils. Adult Mongolian gerbils of both sexes, weighing 60-80 gm, were used. Transient forebrainischemia was produced by bilateral occlusion of the common carotidartery with aneurysm clips for 1, 2, or 5 min under anesthesiawith 2% halothane. During surgical procedures, rectal temperaturewas maintained at 37 ± 0.5°C with a heat lamp. The clips wereremoved after the occlusion procedure. For histologic analysis,30 gerbils were used. Six sham-operated animals were used as controls.For induction of tolerance, 24 gerbils were subjected to 2 minof ischemia (n = 12) or sham operation (n = 12), and 4 d laterthey were subjected to 5 min of ischemia as described previously(Kitagawa et al., 1990). MK801 (3 mg/kg) or vehicle was administeredintraperitoneally 60 min before 2 min of preconditioning ischemiaor sham operation. Seven days after the last ischemia, gerbilswere decapitated, and their brains were promptly removed, dividedinto coronal sections (5 mm in thickness), and fixed in 5% aceticacid in ethanol at 4°C for 4 hr and embedded in paraffin. Coronal5 µm sections corresponding to the stereotactic planes 1.4-1.6mm caudal to the bregma were stained with hematoxylin and eosin.Intact neurons in the hippocampal CA1 sector were counted in ablind manner, and neuronal density per millimeter was calculated.For Western blot analysis, control gerbils (n = 7) and ischemicgerbils at 0, 2, 5, 15, 30, 60, and 180 min (n = 7 for each reperfusionperiod) after 5 min ischemia and at 15 min after 1 min and 2 minischemia (n = 7 for each ischemic period) were decapitated underdeep ether anesthesia, and the hippocampi were rapidly dissectedout in iced saline and frozen in liquid nitrogen. Additional controlgerbils (n = 3) and ischemic gerbils were perfusion-fixed withZamboni's solution (2% paraformaldehyde and 0.2% picric acid)at 5, 15, 30, and 60 min (n = 3 for each reperfusion period) after5 min ischemia under deep pentobarbital anesthesia, and brainswere post-fixed in the same fixative overnight at 4°C. After threewashes in PBS containing 20% sucrose, the brains were frozen inpowdered dry ice and cut into 4-µm-thick coronal sections witha freezing microtome for immunohistochemicalexamination.

Transient global ischemia in CRE-LacZ transgenic mice. We also used male transgenic mice, age 12-16 weeks, carrying a CRE-LacZreporter to confirm that CREB phosphorylation after ischemia inducesCRE-mediated transcription. Transient forebrain ischemia was producedin CRE-LacZ transgenic mice as previously described (Kitagawaet al., 1998). In brief, a polyacrylamide column for measurementof cortical microperfusion by a laser Doppler flowmetry (UniqueMedical, Osaka, Japan) was attached to the intact skull underhalothane anesthesia. Both common carotid arteries were then exposedat the neck, occluded with microanerysmal clips for 15 min, andthen reperfused. Only mice (n = 6) that showed <10% of baselinecortical microperfusion were used. After reperfusion for 60 min,brains were processed for immunohistochemistry as described before.Four sham-operated transgenic mice were used ascontrols.

Neuronal cell culture. Primary cultures of the rat hippocampal neurons were obtained as described previously (Mattson andKater, 1988). Briefly, neuronal cultures were prepared from thehippocampus of embryonic day 18 (E18)~19 rat embryos. The cellswere dissociated with papain (papain dissociation system; Worthington,Lakewood, NJ) and plated onto six-well plates (Falcon, BectonDickinson, and Company, Franklin Lakes, NJ) or two-chamber glassslides (Falcon) coated with polyethylenimine. Cells at a finalconcentration of 5.0~7.0×10⁵ cells/ml were cultured in high-glucose DMEM (Sigma) containing10% fetal calf serum (FCS) (Sigma), 100 IU of penicillin per milliliterand 100 µg of streptomycin sulfate per milliliter. At 24 hr afterseeding, the medium was changed to Neurobasal medium (Life Technologies,Rockville, MD) supplemented with B-27 (Life Technologies). Cellswere cultured at 37°C in a humidified atmosphere of 95% air and5% CO₂ and were used after 6~7 d in vitro when the majority ofcells showed a neuronal phenotype. We also used transgenic micewith a CRE-LacZ reporter gene to investigate whether CREB phosphorylationafter exposure to glutamate induced CRE-mediated transcription.Primary cultures were prepared from the hippocampi of E17~E18mouse embryos after mating of heterozygotes as describedbefore.

Cells were treated with glutamate (20, 50, or 100 µM) for 15 min after 6 or 7 d in vitro. Glutamate and all other chemicalswere added directly to the medium. Before exposure to glutamate,neurons were pretreated for 30 min with one of the following chemicals;non-NMDA receptor antagonist CNQX (10 µM), NMDA receptor antagonistMK-801 (10 µM), L-type Ca²⁺ channel blocker nifedipine (10 µM), Ca²⁺-free medium with Ca-chelator EGTA (1 mM), PKA inhibitor Rp-8-cAMPs(100 µM), KT5720 (2 µM), PKC inhibitor chelerythrine (10 µM),PKG inhibitor Rp-8-Br-cGMPs (50 µM), CaMK inhibitor KN93 (30 µM),mitogen-activated protein kinase kinase (MEK) inhibitor PD98059(50 µM), tyrosine kinase inhibitor genistein (200 µM), phosphatidylinositol3-kinase (PI3K) inhibitor wortmannin (400 nM), and the broad spectrumprotein kinase inhibitor staurosporine (100 nM). Neurons werealso coincubated with these drugs during exposure to glutamatefor 15 min that followed pretreatment. The incubation medium wasthen changedcompletely.

Treatment of cells in culture with CRE-decoy oligonucleotide. Treatment with CRE-decoy oligonucleotide was performed as describedrecently with some modifications (Park et al., 1999, 2001). CRE-decoyand control oligonucleotides used in the present study were phosphorothioateoligonucleotides (OligoExpress; Amersham Pharmacia Biotech, Tokyo,Japan). Their sequences were as follows: 24 mer CRE-decoy, 5'-TGACGTCATGACGTCATGACGTCA-3'and 24 mer nonsense-sequence control, 5'-CTAGCTAGCTAGCTAGCTAGCTAG-3'.Because the CRE cis-element, TGACGTCA, is palindromic, it wasshown that CRE-decoy oligonucleotide self-hybridized to form aduplex-hairpin and compete with CRE enhancers for binding transcriptionfactors, and specifically interfere with CRE-directed transcriptionin vivo (Park et al., 1999). To increase the delivery of oligonucleotideinto the cell, cationic lipid N-[1-(2,3-dioleoyloxy)propyl]-N,N,N-trimethylammoniummethylsulfate (DOTAP; Boehringer Mannheim, Mannheim, Germany)was used in the oligonucleotide treatment. The CRE-decoy and controloligonucleotides were added (1 d before exposure to glutamate)to the cells at 150 nM in the presence of DOTAP. At 24 hr of incubation,glutamate (100 µM) were added directly to the medium as describedbefore.

For cellular localization of CRE-decoy oligonucleotide, cells were incubated with 150 nM of fluorescein isothiocyanate (FITC)-labeledCRE-decoy oligonucleotide (5'-end labeled; Oligoexpress; AmershamPharmacia Biotech, Arlington Heights, IL) in the presence of DOTAP.Six hours after incubation, the medium was removed, and cellswere washed twice with PBS and were cultured in fresh growth medium.The distribution of FITC-labeled oligonucleotides was analyzedby fluorescence invertedmicroscope.

Western blot analysis. Cultured neurons were extracted, and the adult frozen hippocampi were homogenized in 2% SDS solutionand boiled for 5 min. Protein concentrations were determined witha DC Protein Assay (Bio-Rad, Hercules, CA), and samples were mixedwith 2× Laemmli sample buffer. An equal amount of protein foreach sample was separated by 12.5% SDS-PAGE and transferred ontoa polyvinylidine difluoride sheet (Immobilon P; Millipore, Bedford,MA). Membranes were then incubated in a blocking buffer (PBS and0.1% Tween 20) containing 5% skimmed milk powder for 1 hr at roomtemperature. Blots were then incubated with polyclonal anti-CREB(1:400), anti-phosphorylated CREB (anti-pCREB; 1:200), anti- $alpha$ -tubulin(1:1000), or anti-BCL-2 (1: 100) at 4°C overnight. The membraneswere then washed three times in the blocking buffer and incubatedfor 1 hr with anti-rabbit IgG or anti-mouse IgG conjugated toHRP (1:1000; Amersham Pharmacia Biotech). The final reaction productswere visualized using enhanced chemiluminescence (ECL; AmershamPharmacia Biotech, Buckinghamshire, UK), and the membranes wereexposed to x-ray film. Densitometric analysis of CREB, pCREB,and other proteins was performed with a microcomputer imagingdevice (MCID/M2, version 3.0 Image Analysis; Imaging ResearchInc., St. Catharines, Ontario,Canada).

Immunohistochemistry and immunocytochemistry. After treatment with 2% H₂O₂ for 10 min to eliminate endogenous peroxidase activity,brain sections were incubated with anti-CREB antibody (1:400),anti-pCREB antibody (1:200), or anti-NeuN antibody (1:200) overnightat 4°C. Sections were then incubated with secondary antibody:biotinylated anti-rabbit IgG (1:120), rhodamine-conjugated anti-rabbitIgG (Calbiochem; 1:200), or FITC-conjugated anti-mouse IgG (Calbiochem;1:200). Sections reacted with biotinylated anti-rabbit IgG wereincubated further with avidin-biotinylated horseradish peroxidasecomplex (ABC) (1:50 in 50 mM Tris-NaCl; ABC Elite kit; VectorLaboratories, Burlingame, CA) for 45 min. Reaction products werevisualized by treatment for 1-5 min with 0.05% 3,3-diaminobenzidinetetrahydrochloride (DAB) solution in 50 mM Tris-NaCl containing0.005% hydrogen peroxide or with 3-amino-9-ethylcarbazole (AEC)solution (Vector Laboratories). To evaluate the specificity ofthe anti-pCREB antibody, an absorption test was performed withthe antibody pre-absorbed with the synthetic peptide (KRREILSRRPpSYRK)specific to the recognition site. Brain sections reacted withimmunofluorescent secondary antibodies were examined under laserconfocal-scanning microscopy (ZEISS LSM 410). X-gal staining wasperformed as follows: frozen sections after perfusion fixationwith Zamboni's solution were washed three times with PBS whileon ice and then incubated overnight at 37°C in the reaction solutionconsisting of 5 mM potassium ferricyanide, 5 mM potassium ferrocyanide,2 mM MgCl_2, and 1 mg/ml 5-bromo-4-chloro-3-indoyl- $beta$ -D-galactopyranoside(X-gal) (Sigma) in PBS. After reaction with X-gal, the sectionswere immunostained with anti-pCREB antibody as described aboveand finally visualized with the AECsolution.

For immunocytochemical studies, neurons were cultured in two-chamber glass slides and incubated as described above. Afterexposure to glutamate, the neurons were fixed immediately in 4%paraformaldehyde (PFA) for 15 min and permeabilized with 0.01%Triton X-100. Cells were then incubated with anti-CREB (1:400),anti-pCREB (1:400), anti-MAPs (1:200), monoclonal anti-MAP2 (1:100),anti- $beta$ -galactosidase (1:100), or anti-BCL2 antibody (1:100) for1 hr at room temperature. The sections were then washed in threechanges of PBS, incubated for 1 hr in a 1:200 dilution of rhodamine-or FITC-labeled secondary antibody, and evaluated using a confocalmicroscope.

Cell viability assay. Quantitative assessments of neuronal injury were accomplished by measuring the lactate dehydrogenase(LDH) activity in the media 24 hr after exposure to glutamate(20, 50, or 100 µM for 15 min) with the cytotoxicity detectionkit (Boehringer Mannheim) and by counting the viable cells inthe photographs taken under phase-contrastmicroscopy.

Statistical analysis. Statistical analysis was performed by one-way ANOVA followed by Scheffe's test. p < 0.05 was consideredstatisticallysignificant.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Phosphorylation status of CREB after transient global ischemia in gerbils

We performed Western blot analyses to examine the temporal profile of the phosphorylation status of CREB in the post-ischemichippocampus after 5 min of ischemia. As shown in Figure 1A, totalCREB levels were unchanged in the non-ischemic (control) animalsand during ischemia and reperfusion. In contrast, pCREB levelsdecreased during ischemia, but increased during reperfusion peakingat 15 min, and then gradually declined.

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Figure 1. CREB phosphorylation at Ser¹³³ in gerbil hippocampus after transient forebrain ischemia. A, Western blot of proteins isolated from post-ischemic hippocampal tissues at time 0-180 min after transient ischemia for 5 min. In the top panel, total CREB levels were not changed. However, pCREB levels were below the detection limit at the end of ischemia (0 min) but began to increase relative to controls and remained phosphorylated for at least 3 hr after reperfusion. The data in the bottom panel (bar graph) are presented as fold increase in pCREB, as determined by the optical density analysis of phosphorylated and total CREB levels. CREB phosphorylation was increased significantly from 5 to 30 min after reperfusion. Each column and bar represents mean ± SD (n = 7 for each recirculation period); *p < 0.05 versus control. B, Immunostaining for pCREB in the gerbil hippocampus after reperfusion for 15 min. pCREB was detected primarily in the nuclei of pyramidal cells, dentate granule cells, and neocortical neurons from 15 to 60 min after reperfusion. Left panel, Lower magnification image of the hippocampus. Scale bar, 500 µm. Middle panel, Higher magnification image of CA1 pyramidal neurons. Scale bar, 50 µm. Right panel, Absorption test to confirm the specificity of the anti-pCREB antibody.

To study pCREB levels in neurons, we also performed an immunohistochemical study using ABC-DAB and immunofluorescent stainingof brain sections from animals after recirculation for 15 min.pCREB was detected in the nuclei of hippocampal pyramidal cells,dentate granule cells, and neocortical neurons during recirculationfor 15 min (Fig. 1B) to 60 min (data not shown). The immunoreactionwas effectively blocked by preabsorption of the anti-pCREB antibodywith the synthetic peptide (KRREILSRRPpSYRK) (Fig. 1B).

We investigated the presence of pCREB in CA1 pyramidal neurons by double immunostaining for pCREB and NeuN, a neuron-specificmarker, to confirm that pCREB was expressed primarily in neurons.Although the level of staining and the distribution of NeuN werenot affected by ischemia (Fig. 2, top), the number of ischemia-inducedpCREB-positive cells was increased markedly after reperfusionfor 15 min (Fig. 2, middle). In the hippocampus, most pCREB-positivecells were also NeuN-positive (Fig. 2, bottom).

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Figure 2. Expression of pCREB in hippocampal neurons after ischemia. High-magnification confocal images of double immunostaining of NeuN (green) and pCREB (red) in CA1 pyramidal neurons 15 min after reperfusion (right column) compared with sham-operated animals (left column). Top, The number of pyramidal neurons in the CA1 region was unchanged with an antibody specific for NeuN (green). Middle, The number of pCREB-positive cells (red) was increased markedly after reperfusion for 15 min. Bottom, Double immunofluorescence with both antibodies (yellow), showing colocalization in many neurons after reperfusion.

We also investigated the effects of milder ischemia (i.e., 1 or 2 min) on CREB phosphorylation. There was no enhancement ofCREB phosphorylation in the gerbil hippocampus after reperfusionfor 15 min after global ischemia for 1 min, however, after ischemiafor 2 min, CREB phosphorylation was significantly enhanced comparedwith that in control animals, although it was still less thanthat after ischemia for 5 min (Fig. 3A). We also investigatedwhether the NMDA receptor played a role in CREB phosphorylationand induction of tolerance after forebrain ischemia. We foundthat enhancement of CREB phosphorylation after transient forebrainischemia was prevented by intraperitoneal injection of 3 mg/kgof an NMDA receptor antagonist MK801, 60 min before ischemia (Fig.3B). Two minutes of transient bilateral carotid occlusion inducedtolerance in the CA1 neurons against subsequent lethal (5 min)ischemic insult (Fig. 3C), as described previously (Kitagawa etal., 1990). Administration of MK801 before preconditioning ischemiafor 2 min also diminished induction of tolerance in CA1 neurons(Fig. 3C), as described previously (Kato et al., 1992).

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Figure 3. CREB phosphorylation and ischemic tolerance induced after sublethal stress were inhibited by MK801. Effects of the length of ischemia and NMDA receptor antagonist MK801 on CREB phosphorylation after reperfusion for 15 min (A, B). A, Western blot analyses of proteins extracted from the gerbil hippocampus after reperfusion for 15 min after transient forebrain ischemia for 1, 2, or 5 min (top panel). The bar graph (bottom panel) is presented as fold increase in pCREB levels after global ischemia. There was no enhancement of CREB phosphorylation after 1 min of ischemia, whereas both 2 and 5 min of ischemia induced significant increase in pCREB levels. Each column and bar represents the mean ± SD (n = 7 for each ischemic period); *p < 0.05 versus sham-operated animals. B, Intraperitoneal administration of MK801 60 min before transient forebrain ischemia prevented CREB phosphorylation observed after ischemia-reperfusion (n = 3 each). C, Intraperitoneal administration of MK801 before 2 min of preconditioning ischemia abolished neuronal protection. Ischemic tolerance was induced by 2 min of ischemia 4 d before 5 min of ischemia. Each column and bar represents the mean ± SD of neuronal density in the CA1 (n = 6 for each experiment). *p < 0.05 versus all other groups with 5 min of ischemia.

CREB phosphorylation after exposure to glutamate in cultured neurons

Glutamate (100 µM) induced phosphorylation of Ser¹³³ in CREB in primary cultures from rat hippocampus. CREB phosphorylation peakedat 10 min and returned to the baseline level by 180 min afterexposure to glutamate (Fig. 4). The pattern with rapid and transientenhancement of CREB phosphorylation was similar to that observedin gerbil hippocampus after global ischemia (Fig. 1).

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Figure 4. CREB phosphorylation at Ser¹³³ induced by exposure to glutamate in cultured neurons. Top panel, Immunoblots of primary cultures from rat hippocampus after exposure to glutamate (100 µM) for the indicated periods. Levels of CREB proteins were unchanged, but those of pCREB peaked at 10 min after exposure and returned to the basal level 180 min later. The bar graph is presented as fold increase in pCREB levels with the optical density analysis of pCREB and total CREB. Each column and bar represents the mean ± SD (n = 6 for each exposure period); *p < 0.05 versus control.

To confirm the notion that the observed transient enhancement of CREB phosphorylation reflected the neuronal response to glutamateexcitotoxicity, a double immunocytochemical study was performedfor pCREB and NeuN. The number of pCREB-positive cells increasedmarkedly compared with the number in untreated cells, whereasthe number of NeuN-positive neurons was unchanged at 10 min afterexposure to glutamate (Fig. 5). The increase in the number ofdouble-positive neurons indicated that pCREB expression was enhancedin glutamate-stimulated neurons.

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Figure 5. pCREB in cultured neurons after exposure to glutamate. NeuN (green) and pCREB (red) immunofluorescence in cultured hippocampal neurons 10 min after exposure to glutamate (right column) compared with controls (left column). Top, The number of neurons stained with an anti-NeuN antibody (green) was unchanged. Middle, The number of pCREB-positive cells (red) increased markedly 10 min after exposure to glutamate. Bottom, NeuN-positive-pCREB-positive cells (yellow). CREB phosphorylation was enhanced in most neurons after exposure to glutamate.

We also investigated CREB phosphorylation after milder exposure to glutamate in cultured neurons. LDH assay revealed thatthe concentration of glutamate ranging from 50 to 100 µM causeddeath in 30-50% of cultured neurons, whereas neurons exposed to20 µM of glutamate were undamaged (Fig. 6A). CREB phosphorylationstatus then studied after 10 min of exposure at each glutamateconcentration. There was a significant increase in pCREB at 20,50, and 100 µM of glutamate (Fig. 6B). These results suggest thatCREB phosphorylation may also be induced by sublethal stimuliand that CREB phosphorylation may play an important role in theneuronal response to metabolic stress.

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Figure 6. Glutamate-induced CREB phosphorylation after sublethal stress. A, Evaluation of neuronal death by the measurement of LDH released into culture media or by the counting of damaged cells. Open columns indicate the percentage of cell death (LDH release) 24 hr after treatment with the indicated concentrations of glutamate, and shaded columns indicate the percentage of loss of cells (cell counting) 24 hr after exposure to 100 µM glutamate. B, Effects of different concentrations of glutamate (20, 50, and 100 µM) on CREB phosphorylation 10 min after an addition of glutamate, as determined by Western blot analysis. Although the total CREB level in each lane was similar, CREB phosphorylation was enhanced by 20, 50, and 100 µM glutamate. Fold increase in CREB phosphorylation is quantified in a bar graph. Each column and bar represents mean ± SD (n = 6 for each glutamate concentration); *,p < 0.05 versus controls.

Signal transduction pathway inducing CREB phosphorylation after exposure to glutamate in cultured neurons

To examine the involvement of Ca²⁺ influx and protein kinases in CREB phosphorylation, cultures were pretreated with variousantagonists and inhibitors for 30 min before exposure to glutamate(Fig. 7). Glutamate-mediated CREB phosphorylation was dependenton extracellular Ca²⁺. Removal of Ca²⁺ from the medium prevented CREB phosphorylation. MK801 blockedglutamate-induced CREB phosphorylation, but CNQX and nifedipinedid not. The increased pCREB expression after exposure to glutamatewas effectively blocked by KN93 (a specific inhibitor of CaMK),and by staurosporine (a broad spectrum protein kinase inhibitor).However, glutamate-induced CREB phosphorylation was not blockedin the presence of PKA inhibitors (Rp-8-Cl-cAMPs and KT5720),PKC inhibitor (chelerythrine), PKG inhibitor (RP-8-Br-cGMPs),MEK inhibitor (PD98059), tyrosine kinase inhibitor (genestein),or PI3K inhibitor (wortmannin) (Fig. 7).

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Figure 7. Effects of receptor antagonists, Ca²⁺ channel blocker, Ca²⁺ depletion, and protein kinase inhibitors on CREB phosphorylation in cultured hippocampal neurons after exposure to glutamate. As indicated, reagents used in this study were MK-801 (10 µM), nifedipine (10 µM), Ca-free medium with CA²⁺-chelator EGTA (1 mM), Rp-8-cAMPs (100 µM), KT5720 (2 µM), chelerythrine (10 µM), Rp-8-cGMPs (100 µM), KN93 (30 µM), PD98059 (50 µM), genistein (200 µM), wortmannin (400 nM), and staurosporine (100 nM). Cultured neurons were treated for 30 min before the addition of and during the 10 min exposure to 100 µM glutamate. Enhanced CREB phosphorylation induced by exposure to glutamate was prevented in the Ca²⁺-free condition and in the presence of MK-801, KN93, and staurosporine as indicated in the graphical quantification. Data are mean ± SD (n = 6 for each treatment); *p < 0.05 versus control.

CREB phosphorylation mediates neuronal survival through BCL-2 production after exposure to glutamate

The data shown in Figure 7 suggests that CaMK may participate in the signaling pathway that mediates the neuronal responseto glutamate. To examine the role of CREB phosphorylation by CaMKon neuronal survival, BCL-2 expression by cultured neurons wasinvestigated after exposure to glutamate (100 µM) because theBCL-2 gene contains a CRE in the promoter region (Riccio et al.,1999) and shows protection against cell death (Martinou et al.,1994). Immunocytochemical analyses revealed that, after exposureto glutamate, BCL-2 was identified to localize in those cellsthat showed immunoreactivity to a specific neuronal marker, MAPs(Fig. 8A). Western blot analysis showed that BCL-2 expressionwas upregulated 6 hr after exposure to glutamate. The glutamate-inducedincrease in BCL-2 production was inhibited by pretreatment withKN93 (Fig. 8B). We also investigated the effect of KN93 on neuronalsurvival. Pretreatment with KN93 (30 µM) for 30 min before exposureto glutamate significantly increased the level of neuronal damagecompared with that in controls (Fig. 8C), suggesting that CaMK-mediatedCREB phosphorylation may contribute to neuronal survival.

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Figure 8. Pretreatment with KN93 inhibits glutamate-induced BCL-2 production and exacerbates the neuronal cell damage observed after exposure to glutamate. A, High-magnification confocal images of MAPs (green) and BCL-2 (red) immunostaining in cultured hippocampal neurons 6 hr after exposure to glutamate (100 µM). The double-immunofluorescence image suggests that the MAP-positive cells are all BCL-2-positive (yellow). B, Western blot analyses showing upregulation of BCL-2 6 hr after exposure to glutamate; this increase was prevented by pretreatment with KN93 (top panel). The bar graph is presented as fold increase of BCL-2 expression. The densitometric values were normalized to $beta$ -tubulin levels. Data are mean ± SD (n = 6 for each treatment); *p < 0.05 versus controls; p < 0.05 versus glutamate treatment without KN93. C, Neuronal cell death 24 hr after exposure to glutamate was increased significantly when CREB phosphorylation was prevented by pretreatment with KN93 (30 µM). Data are mean ± SD (n = 6 for each treatment); *p < 0.05 versus control; p < 0.05 versus glutamate treatment without KN93.

To determine the role of CREB in neuroprotection and survival in this model, we examined the effect of CRE-decoy oligonucleotideon CREB phosphorylation, BCL-2 production and cell viability afterglutamate exposure. After 6 hr incubation at 150 nM, most neuronson the plate showed uptake of FITC-conjugated CRE-decoy oligonucleotide(Fig. 9A). CREB phosphorylation at 10 min after exposure to glutamatewas not inhibited by CRE-decoy or control oligonucleotide (Fig.9B), however, BCL-2 production at 6 hr after exposure to glutamatefor 15 min was suppressed by CRE-decoy oligonucleotide (Fig. 9B).Pretreatment with CRE-decoy oligonucleotide also significantlyincreased the level of neuronal damage compared with that in controls(Fig. 9C). Pretreatment with control oligonucleotide did not suppressBCL-2 production or increase the level of cell damage comparedwith that in controls (Fig. 9B,C). Immunocytochemistry for MAP2showed neuronal cytoplasma and dendrites in cultured neurons (Fig.9A). The number of MAP2-positive neurons decreased 24 hr afterglutamate exposure for 15 min. Again, pretreatment with CRE-decoyoligonucleotide accelerated the decrease of the number of MAP2-positiveneurons after glutamate exposure (Fig. 9A).

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Figure 9. Pretreatment with CRE-decoy oligonucleotide inhibits glutamate-induced BCL-2 production and exacerbates the neuronal cell damage observed after exposure to glutamate. Aa, Cellular uptake of FITC-conjugated oligonucleotide (FITC-Oligo) after incubation for 6 hr. b-f, MAP2 immunostaining of control neurons (b, c) and of neurons 24 hr after exposure to glutamate (100 µM) (d-f). Pretreatment with CRE-decoy or control oligonucleotide was indicated with +Decoy Oligo and +Control Oligo in the figures, respectively. Most neurons on the plate showed uptake of FITC-conjugated oligonucleotide in the presence of DOTAP (a). In control neurons, immunocytochemistry for MAP2 showed neuronal cytoplasma and dendrites (b, c). The number of MAP2-positive neurons decreased 24 hr after glutamate exposure for 15 min (d). Pretreatment with CRE-decoy oligonucleotide (e), not with control oligonucleotide (f), accelerated the decrease of the number of MAP2-positive neurons after glutamate exposure. B, Effect of pretreatment with CRE-decoy or control oligonucleotide on CREB phosphorylation and BCL-2 production after exposure to glutamate (100 µM). The data in the bar graph is presented as fold increase in pCREB and BCL-2 levels. The densitometric values were normalized to CREB and $beta$ -tubulin levels, respectively. Data are mean ± SD (n = 6 for each treatment); *p < 0.05 versus controls; p < 0.05 versus glutamate treatment without oligonucleotide. C, Effect of pretreatment with CRE-decoy or control oligonucleotide on neuronal cell death after exposure to glutamate (100 µM). Neuronal cell death 24 hr after exposure to glutamate (100 µM) increased significantly by pretreatment with CRE-decoy oligonucleotide. Data are mean ± SD (n = 6 for each treatment); *p < 0.05 versus control; p < 0.05 versus glutamate treatment without oligonucleotide.

CREB phosphorylation and CRE-mediated gene transcription after ischemia and glutamate exposure in CRE-LacZ transgenic mice

In cultured neurons prepared from control transgenic mice, there were only few pCREB- or $beta$ -galactosidase-positive cells (Fig.10). However, the number of pCREB- and $beta$ -galactosidase- positivecells increased markedly 30 min after exposure to glutamate (100µM) (Fig. 10A,B). A subset of pCREB-positive neurons were also $beta$ -galactosidase-positive. Pretreatment with KN93, CaMK inhibitor,decreased the number of pCREB- and $beta$ -galactosidase-positive cells(Fig. 10).

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Figure 10. CRE-mediated LacZ transcription in cultured neurons was upregulated by exposure to glutamate. A, High-magnification confocal images of immunostaining for pCREB (red), $beta$ -galactosidase (green), and both proteins (yellow) in cultured hippocampal neurons from CRE-LacZ transgenic mice. Top, The number of pCREB-positive cells was small, and $beta$ -galactosidase expression was weak without stimulation. Middle, The number of pCREB-positive cells (red) increased markedly 60 min after exposure to glutamate (100 µM), and $beta$ -galactosidase expression was also enhanced in a subset of pCREB-positive cells (yellow). Bottom, Both CREB phosphorylation and $beta$ -galactosidase expression were inhibited by pretreatment with KN93. B, Frequency of pCREB-, $beta$ -galactosidase, or both-positive cells in control and glutamate exposure with or without KN93 (n = 4 for each group); *p < 0.05 versus control.

In brain sections from sham-operated CRE-LacZ transgenic mice, there were only few pCREB-positive or X-gal-positive cells(Fig. 11A). After reperfusion for 60 min, most pyramidal neuronsin the hippocampus were pCREB-positive (red cells in Fig. 11B,D).X-gal-positive cells (blue cells in Fig. 11B) were also observed,but the number was smaller than that of pCREB-positive cells.Most X-gal-positive cells were also pCREB-positive (Fig. 11C,D).

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Figure 11. CRE-mediated LacZ transcription was increased in pCREB-positive hippocampal neurons by ischemic stress. pCREB-positive cells were primarily neurons (red cells), and most X-gal-positive cells (blue cells) were pCREB-positive neurons (red cells) in CRE-LacZ transgenic mice after transient forebrain ischemia. A, Nonischemic control hippocampal CA1 sector. Neither pCREB nor X-gal reactivity was observed. Scale bar, 50 µm. B, Hippocampal CA1 pyramidal neurons in CRE-LacZ transgenic mice after transient ischemia. Scale bar, 50 µm. C, Higher magnification image of the rectangle in B. X-gal-positive cells (arrows) corresponded to red cells immunoreactive for pCREB. Scale bar, 10 µm. D, Frequency of pCREB-, X-gal-, or both-positive cells in control and ischemic hippocampus (n = 4 for each group); *p < 0.05 versus control.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study demonstrated that transient CREB phosphorylation and subsequent CRE-mediated gene transcription occurredafter exposure to glutamate in cultured neurons and after ischemicinsult in adult gerbil hippocampal neurons. Transient exposureto glutamate mimics the increase of the extracellular glutamateconcentration during and after transient global ischemia. Previousstudies have demonstrated that stimulation with glutamate or NMDAcaused transient CREB phosphorylation in cultured neurons andhippocampal slices (Bito et al., 1996; Hardingham et al., 1999;Hu et al., 1999; Rajadhyaksha et al., 1999; Vanhoutte et al.,1999; Sala et al., 2000).

Our first goal was to clarify the extracellular and intracellular signal pathways leading to CREB phosphorylation after exposureto glutamate. CREB phosphorylation can be induced by extracellularsignals such as glutamate, growth factors, and membrane depolarization,and is mediated through several kinases including PKA, PKC, CaMK,mitogen-activated protein kinase-activated protein (MAPKAP) kinase2, and the pp90 ribosomal S6 kinase family (Rsks) (Imprey et al.,1998; Finkbeiner, 2000). Recently, neurotrophin-mediated survivalof cerebellar granule cells was found to be at least in part becauseof CREB phosphorylation by MAPK-Rsks (Bonni et al., 1999). Ourpharmacological studies with several kinase inhibitors showedthat CREB phosphorylation after exposure to glutamate was dependenton calcium influx through NMDA-type receptors and on CaMK II-IV,but not mediated through PKA, PKC, cGMP-dependent protein kinase,PI3 kinase, or the MAPK cascade. Our results were consistent withthose observed after electrical stimulation of hippocampal neurons(Bito et al., 1996). Therefore, it is likely that the same intracellularpathway that mediates the activity-dependent neuronal plasticityis also involved in CREB phosphorylation after cytotoxic exposureto glutamate, although neurons in different brain regions, suchas the striatum, may respond to glutamate and phosphorylate CREBthrough the MAPK cascade (Perkinton et al., 1999; Rajadhyakshaet al., 1999; Vanhoutte et al., 1999). The decline of CREB phosphorylationobserved 1 hr after exposure to glutamate in our study would beascribed to activation of protein phosphatases linked to NMDAreceptors and calcium influx (Bito et al., 1996; Sala et al.,2000).

What is the role of CREB phosphorylation after exposure to glutamate?

In our study, several treatments including calcium removal and preincubation with MK801, staurosporine, and KN93 inhibitedCREB phosphorylation after exposure to glutamate. We used KN93to inhibit CaMKII-IV, because CaMKII-IV can phosphorylate CREBdirectly, and CaMKIV overexpression was shown to inhibit apoptosisinduced by potassium deprivation in cerebellar granule neurons(See et al., 2001). Pretreatment with KN93 inhibited CREB phosphorylationand increased the degree of neuronal injury after exposure toglutamate, suggesting that CREB phosphorylation after exposureto glutamate may be important for cell survival. The experimentwith CRE-decoy oligonucleotide also supported the neuroprotectiverole of CRE-mediated gene expression that follows CREB phosphorylationin exposure to glutamate. CREB overexpression in PC12 and Neuro2Acells was also shown to inhibit apoptosis induced by okadaic acid(Walton et al., 1999). Recently, the BCL-2 gene was found to havea CRE in the 5' promoter region, and cell survival mediated byneurotrophin-induced CREB phosphorylation in sympathetic and corticalneurons was associated with increased BCL-2 expression (Riccioet al., 1999). Accumulating evidence indicates that overexpressionof BCL-2 provides protection against apoptosis (Martinou et al.,1994) and ischemic neuronal death (Lawrence et al., 1996; Kitagawaet al., 1998). Thus, the protective effect of CREB phosphorylationagainst glutamate- or ischemia-induced neuronal degeneration maybe attributable to increased expression of BCL-2. In the presentstudy, we observed increased BCL-2 expression 6 hr after exposureto glutamate, which was inhibited by pretreatment of culturedneurons with KN93 or CRE-decoy oligonucleotide, suggesting thatBCL-2 expression was induced by CaMK-mediated CREB activationand involved in the neuroprotective role of CREB after exposuretoglutamate.

CREB phosphorylation has been examined in several experimental stroke models. At first, Walton et al. (1996) showed that ischemia-resistantgranule cells produced increase in pCREB immunoreactivity, peaking6 and 48 hr after a unilateral hypoxic-ischemic injury in the21-d-old rat. Later, Hu et al. (1999) demonstrated that CREB phosphorylationwas induced in the adult rat hippocampus, mainly in the resistantdentate granule cells, several hours after transient global ischemiafor 15 min. It was also shown that in the focal-ischemia model,CREB phosphorylation was marked in the peri-infarct area (Tanakaet al., 1999; Irving et al., 2000). CREB phosphorylation in thesurviving neurons was also shown in the chick cochlear nucleusafter activity deprivation by cochlea removals (Zirpel et al.,2000). However, the temporal profile of CREB phosphorylation immediatelyafter ischemia has not been fully examined, although early phosphorylationof CREB can be expected from the expression pattern of immediateearly genes such as c-Fos after ischemia (Kiessling et al., 1993),exposure to glutamate (Hardingham et al., 1999), and electricalstimulation (Bito et al., 1996; Sgambato et al., 1998). Hata etal. (1998) also reported involvement of CREB activation in c-fosmRNA expression after middle cerebral artery occlusion in CREBknock-out mice. Our study demonstrated that CREB was phosphorylatedin hippocampal neurons immediately after a brief period (5 min)of ischemia and returned to control levels by 60 min after reperfusion.The molecular pathway leading to ischemia-induced early CREB phosphorylationin vivo is primarily unknown, but our experiments with MK801 suggestedthat the activation of NMDA-type receptor was important. Thismechanism has been known for CREB phosphorylation in responseto high-frequency stimulation causing long-term potentiation (Schulzet al., 1999).

Both in vivo and in vitro findings in the present study suggested that common pathways for CREB phosphorylation were activatedin response to electrical stimulation and cytotoxic exposure toglutamate including Ca²⁺ influx, NMDA-type receptor activation, and CaM kinase. CREB phosphorylationobserved after exposure to glutamate in vitro and ischemia invivo may represent the cellular protective response against metabolicstresses. This notion is supported by the finding that both lethaland nonlethal stresses with glutamate in cultured neurons andbrief ischemia for 2 min in gerbil hippocampus induced CREB phosphorylation.The latter finding suggests that CREB phosphorylation and subsequentgene expression may play an important role in the acquisitionof ischemic tolerance, where nonlethal ischemic stress makes neuronsresistant to subsequent severe ischemic insult (Kitagawa et al.,1990; Kirino et al., 1991).

  FOOTNOTES

Received April 18, 2001; revised Sept. 6, 2001; accepted Sept. 7, 2001.

This work was supported by a Grant-in-aid for Scientific Research on Priority Areas (A). We thank Y. Nishizawa and R. Morimotofor secretarialassistance.
Correspondence should be addressed to Dr. Kazuo Kitagawa, Division of Strokology, Department of Internal Medicine and Therapeutics(A8), Osaka University Graduate School of Medicine, 2-2 Yamadaoka,Suita City, Osaka 565-0871, Japan. E-mail: kitagawa{at}medone.med.osaka-u.ac.jp.

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