Dopamine Induces a PI3-Kinase-Independent Activation of Akt in Striatal Neurons: A New Route to cAMP Response Element-Binding Protein Phosphorylation

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The Journal of Neuroscience, October 15, 2002, 22(20):8911-8921

Dopamine Induces a PI3-Kinase-Independent Activation of Akt in Striatal Neurons: A New Route to cAMP Response Element-Binding Protein Phosphorylation
Karen Brami-Cherrier¹, Emmanuel Valjent¹, Marta Garcia¹, Christiane Pagès¹, Robert A. Hipskind², and Jocelyne Caboche¹
¹ Laboratoire de Neurobiologie des Processus Adaptatifs, Centre National de la Recherche Scientifique/Université Pierre et Marie Curie, Unité Mixte de Recherche 7102, 75005 Paris, France, and ² Institut de Génétique Moléculaire, Unité Mixte de Recherche 5535, Centre National de la Recherche Scientifique, 34293 Montpellier, France

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Akt is classically described as a prosurvival serine/threonine kinase activated in response to trophic factors. After activationby phosphoinositide 3-kinase (PI3-kinase), it can translocateto the nucleus where it promotes specific genetic programs bycatalyzing phosphorylation of transcription factors. We reporthere that both dopamine (DA) D1 (SKF38393) and D2 (quinpirole)agonist treatments rapidly increase, in primary striatal neuronsin culture, phosphorylation levels of Akt on Thr³⁰⁸, a residue that is critically involved in its kinase activity.These treatments also activate the extracellular signal-regulatedkinase (ERK) pathway in the same population of striatal neurons.Induction of active, phospho-Thr³⁰⁸ Akt by dopamine D1 and D2 agonists is insensitive to wortmanninand thus PI3-kinase independent, in contrast to growth factor-inducedAkt activity. D1- and D2-induced phospho-Thr³⁰⁸ Akt is decreased by the mitogen-activated protein kinase kinase(MEK) inhibitor, U0126, as well as by overexpression of a dominant-negativeversion of MEK, thus implicating the Ras/ERK signaling cascadein this process. Furthermore, overexpression of a mutant formof Akt that cannot be activated impaired cAMP response element-bindingprotein (CREB) phosphorylation induced by SKF38393 and quinpiroletreatments. Activation of Akt on Thr³⁰⁸ was also found in vivo in striatal neurons after acute administrationof cocaine, a psychostimulant that strongly increases DA transmission.Thus, multiple intracellular pathways can transduce signals fromdopamine receptors to CREB in striatal neurons, one of these beingAkt. We propose that this signaling pathway plays a pivotal rolein DA-induced regulation of gene expression and long-term neuronaladaptation in thestriatum.

Key words: extracellular signal-regulated kinase; phospho-Thr³⁰⁸ Akt; PI3-kinase; cAMP; gene regulation; nuclear translocation; cocaine

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Originally characterized on the basis of its sequence homology with the v-akt oncogene and with protein kinase A (PKA) (Bellacosaet al., 1991; Coffer and Woodgett, 1991; Jones et al., 1991),the protein kinase B (PKB)/Akt is an important mediator of thephysiological effects of several growth and survival factors;notably, it promotes cell survival through the inhibition of apoptosis(for review, see Downward, 1998; Datta et al., 1999). Akt is amember of the serine/threonine kinase family (Alessi et al., 1997)and is a major target, via its pleckstrin homology (PH) domain,of the phosphoinositide 3-kinase (PI3-kinase) (Burgering and Coffer,1995; Franke et al., 1995). During growth factor stimulation,PI3-kinase increases levels of the lipid second messenger, phosphatidylinositol3,4,5-triphosphate (PI-3,4,5P3) (Hemmings, 1997; Toker and Cantley,1997; Falasca et al., 1998). This binds to the PH domain of Aktand promotes its translocation from the cytosol to the plasmamembrane, where its is activated by phosphorylation on two criticalresidues, Thr³⁰⁸ and Ser⁴⁷³. Then, Akt detaches from the membrane and targets both cytosolicand nuclear substrates. Within the nucleus, Akt controls expressionof genes involved in cell survival via the transcription factorsForkhead, NF- $kappa$ B, and cAMP response element-binding protein (CREB)(for review, see Brunet et al., 2001).

The dopaminergic system plays a significant role in motor function and associative learning (for review, see Berke and Hyman,2000). Alteration in dopamine signaling has been involved in manyneuropsychiatric disorders, including Parkinson's disease, schizophrenia,and attention deficit hyperactivity disorder, as well as drugaddiction. One mechanism that underlies the dopaminergic regulationof physiology involves gene regulation, which can contribute tothe long-term changes in synaptic plasticity observed during thesedisorders. Through the stimulation of D1 and D2 subfamilies ofG-protein-coupled receptors, dopamine can activate CREB phosphorylationand gene transcription via distinct mechanisms. By elevating intracellularcAMP levels and activating PKA, DA-D1 receptor stimulation leadsto phosphorylation of cAMP response element-binding protein (CREB)(Konradi et al., 1994). On the other hand, although D2 receptorsare classically linked to reduction of cAMP production, they cancouple to phospholipase C $beta$ (PLC $beta$ ) via G_q, mobilize intracellularcalcium stores, and also phosphorylate CREB (Yan et al., 1999).The mitogen-activated protein kinase (MAPK) of the extracellularsignal-regulated kinase (ERK) family, a serine/threonine kinaseclassically associated with cell proliferation and survival, isalso a possible downstream effector of both D1 and D2 receptorstimulation (Yan et al., 1999; Zanassi et al., 2001). In thisway, it is now well established that in post-mitotic neurons,this signaling cascade can have important roles in gene regulationand synaptic plasticity underlying cognitive functions such aslearning and memory, as well as drug addiction (for review, seeValjent et al., 2001).

In non-neuronal cells, certain survival stimuli activate Akt independently of PI3-kinase, including agonists of the PKA pathway(Moule et al., 1997; Sable et al., 1997; Filippa et al., 1999),as well as increases in cytoplasmic calcium levels (Yano et al.,1998). We thus investigated in the present study a possible activationof Akt by DA. We show a rapid activation and nuclear translocationof Akt after both D1 and D2 agonist treatments. In both cases,this activation is independent of PI3-kinase, instead dependingon cAMP production for D1 receptors and ERK activation for bothD1 and D2 receptor stimulation. Overexpression of a dominant-negativeform of Akt diminishes CREB phosphorylation induced by the dopaminergicagonists. Together with the in vivo observation that systemicadministration of cocaine also activates Akt in striatal neurons,our data strongly support the possibility that this pathway representsa new route to CREB phosphorylation downstream of DAtransmission.

  MATERIALS AND METHODS

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MATERIALS AND METHODS
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Chemicals and reagents. U0126 (Calbiochem) and wortmannin (Calbiochem), were diluted in DMSO. Rp-cAMP (Sigma) was dilutedin H₂O. For each treatment, cells were incubated with the inhibitors,15 (wortmannin) or 30 (other inhibitors) min before the additionof SKF38393 (RBI), quinpirole (RBI), or insulin growth factor1 (IGF-1;RBI).

Neuronal cell cultures and treatments. Striata were dissected out from 14-d-old Swiss mouse embryos (Janvier) and mechanicallydissociated by gently pipetting in modified L-15 medium. Afterdecantation for 10 min at room temperature (RT) to eliminate tissuedebris, cells were collected by centrifugation at 1000 × g for5 min. Cell pellets were suspended in Neurobasal medium [B27 supplement(Invitrogen), 500 nM L-glutamine, 60 µg/ml penicillin G, 25 µM $beta$ -mercaptoethanol] and then plated into 24-well (1.8 × 10⁵ cells per well) or 6-well (8.6 × 10⁵ cells per well) Nunc multi-well plates coated with 10 µg/ml poly-D-lysine(Sigma). After removal of the coating solution, cells were seededin the Neurobasal medium and cultured at 37°C in a humidifiedatmosphere of 95% air and 5% CO₂ and were used after 8 d in vitro(DIV), when most of the cells were of neuronal phenotype withno detectable glial elements. On the day of the experiments, themedium was removed and replaced by Neurobasal medium containingSKF38393 (100 µM) (Paolillo et al., 1998; Zanassi et al., 2001)and quinpirole (10 µM). Then cells were replaced at 37°C for theappropriate time. Inhibitors were added before agonist treatmentsas detailedabove.

Immunocytochemistry. After the appropriate time of agonist treatment, cells were fixed in 24-well plates with PBS containing4% paraformaldehyde (PFA) for 40 min at RT and then incubatedwith methanol/acetone solution (50:50) for 10 min at 4°C. Afterthree rinses in PBS, cells were treated with blocking buffer (fetalcalf serum 10%, BSA 1% in PBS) for 2 hr at RT. Polyclonal antibodiesraised against phospho-Thr³⁰⁸ Akt (P-T-Akt, 1:1000; UBI, Euromedex), phospho-Ser⁴⁷³ Akt (P-S-Akt, 1:200; Promega), phospho-Ser¹³³ CREB (P-CREB, 1:1000; UBI, Euromedex), and dually phosphorylatedERK (Thr²⁰²-Tyr²⁰⁴ p44/42 MAPK) (P-ERK, 1:500; New England Biolabs, Ozyme, France)were incubated overnight (ON) at 4°C in PBS containing 1% BSA,0.05% Tween 20. Then, anti-rabbit Cy3-conjugated antibodies (1:750;Amersham) were incubated for 2 hr at RT. For control of the specificityof P-T-Akt antibody, 10 µg of immunogen peptide correspondingto amino acids KDGATMK[pT]FCGT or 10 µg of nonactive Akt 1-glutathioneS-transferase (GST) agarose protein (UBI, Euromedex) was preincubatedfor 30 min at RT with 1 µg of P-T-Akt antibody. For double immunostaining,a polyclonal antibody raised against P-T-Akt was incubated simultaneouslywith a monoclonal antibody raised against P-ERK (Thr²⁰²-Tyr²⁰⁴ p44/42 MAPK) (1:500, Sigma). Plates were rinsed in PBS and incubatedsequentially with an anti-rabbit Cy3-conjugated antibody (1:750;Amersham) and an anti-mouse FITC-conjugated antibody (1:500; Sigma)for 2 hr each at RT. After counterstaining with Hoechst, cellswere mounted under coverslips using Vectashield (VectorAbcys).

Subcellular fractionation. Neurons were cultured in six-well plates, placed on ice, and lysed in buffer A containing 5 mMHEPES, pH 7.9, 1.5 mM MgCl₂, 10 mM KCl, and a mix of proteaseand phosphatase inhibitors (100 mM Na₃VO₄, 0.5 mM DTT, 100 nMokadaic acid, 2.5 µg/ml aprotinin, 2.5 µg/ml pepstatin, 0.5 mMPMSF, 0.5 mM benzamidine, 2.5 µg/ml leupeptin, 1 µM microcystinL-R). Lysates were centrifuged for 10 min at 4000 × g at 4°C.The supernatant corresponding to the cytosolic fraction was removed,and pellets were washed twice with buffer A and suspended in bufferB containing 20 mM HEPES, pH 7.9, 20% glycerol, 0.1 M KCl, 0.5mM MgCl₂, and the same mix of protease and phosphatase inhibitorsas buffer A. Pellets were washed twice and suspended in bufferC containing 20 mM HEPES, pH 7.9, 25% glycerol, 0.5 mM NaCl, 0.5mM MgCl₂, 0.5 mM EDTA, and a mix of protease and phosphatase inhibitors.This fraction corresponded to the nuclear fraction. Protein extracts(10 µg from each fraction) were separated by 10% SDS-PAGE beforeelectrotransfer. Blots were blocked with 5% nonfat milk and incubatedwith rabbit polyclonal antisera raised against phospho-Thr³⁰⁸ Akt (1:1000; UBI) ON at 4°C. After rinsing, the blots were incubatedwith goat horseradish peroxidase-conjugated antibody (1:5000;Amersham Biosciences) for 2 hr at RT before exposure to the ECLkit (AmershamBiosciences).

Immunoprecipitation and in vitro kinase assay. Cells were lysed in lysis buffer (10 mM Tris-HCl, 50 mM NaCl, 1% Triton X-100,30 mM sodium pyrophosphate, 50 mM NaF, 5 µM ZnCl₂, 100 µM Na₃VO₄,1 mM DTT, 5 nM okadaic acid, 0.5 µM PMSF, 0.5 mM benzamidine,1 µM microcystin L-R, 2.5 µg/ml aprotinin, pepstatin, and leupeptin).Insoluble cell debris was removed by centrifugation at 13,000× g for 15 min at 4°C. One-hundred micrograms of striatal lysateswere incubated overnight at 4°C with 2 µg of anti-Akt/PKB, PHdomain antibody (UBI, Euromedex) previously coupled to proteinG-Agarose. Immunoprecipitates were washed three times with lysisbuffer and twice in buffer B containing 50 mM Tris-HCl, pH 7.5,0.03% (w/v) Brij-35, 0.1 mM EGTA, and 0.1% (v/v) 2-mercaptoethanol.Then, immunoprecipitates were resuspended in kinase buffer (50mM Tris-HCl, pH 7.5, 0.02% Brij-35, 0.1 mM EGTA, 10 mM Mg(C₂H₃O₂)₂,20 µM ATP, 10 µM cAMP-dependent kinase (PKA) inhibitor, 2 mM DTT,5 nM okadaic acid, 100 µM Na₃VO_4, 2.5 µg/ml aprotinin, pepstatin,and leupeptin). The suspended immunoprecipitates were incubatedwith 4 µM [ $gamma$ -³²P] ATP (3000 Ci/mmol; DuPont NEN) and 2 µg of recombinant GST-CREB(aa 1-166) bound to glutathione-agarose at RT for 30 min. Thereactions were stopped by dilution with 500 µl HBB (20 mM HEPES,pH 7.6, 2.5 mM MgCl₂, 50 mM NaCl, 0.05% Triton X-100, 20 mM $beta$ -glycerolphosphate, 10 mM p-nitrophenyl phosphate). After two washes withHBB, samples were denatured and analyzed on 10% SDS-PAGE. Thegel was Coomassie stained to confirm equal amounts of substratein all lanes and dried. The GST-CREB_1-166 protein preparationalso contains a truncated protein containing primarily GST thatshowed nolabeling.

Transfections and DNA constructs. Dominant-negative Akt (DN-Akt) was hemagglutinin (HA)-tagged PKB $alpha$ , Asp¹⁷⁹/Ala-Thr³⁰⁸/Ala-Ser⁴⁷³/Ala cloned in the mammalian expression vector pCMV5 (kindly providedby Dr. Dario R Alessi, Dundee, UK) (Andjelkovic et al., 1997).Expression of DN-Akt was visualized by immunocytochemical detectionof HA using a monoclonal anti-HA antibody (1:2000; BoehringerMannheim) and revealed by anti-mouse Cy3-conjugated antibody (1:600;Jackson ImmunoResearch, Intershim). Dominant-negative form ofmitogen-activated protein kinase kinase (DN-MEK), S222A, was fromDrs. G. Pagès and J. Pouyssegur (Pagès et al., 1994). Transienttransfection of primary striatal cultures was performed with Lipofectamine2000 (Invitrogen). Cells (1.8 × 10⁵) were transfected with 1 µg of green fluorescent protein (GFP)plasmid (pEGFP-N3, Clontech) or cotransfected with 1 µg of GFPplasmid and 5 µg of DN-Akt or DN-MEK plasmid with Lipofectamine2000 as recommended by the manufacturer's protocol. After 6 hr,the cultures were rinsed with fresh medium. After 24 hr, cellswere treated with SKF38393 or quinpirole as describedabove.

Immunocytochemical and statistical analysis. For each experiment, cells were analyzed under a fluorescent inverted microscope(Nikon) directly into the wells. Images from immunofluorescencewere digitized (magnification 400×) in parallel with Hoechst staining,from five independent fields for each experiment (n = 3 for eachtreatment). The percentage of P-T-Akt- or P-ERK-positive neuronswas calculated by comparison with total Hoechst-stained neurons.Data were analyzed using one-way ANOVA between subjects, and posthoc comparisons were made using the Newman-Keuls test. In allcases, significance was set at p < 0.05.

In vivo analysis: animals, drugs, and treatments. Animal care was conducted in accordance with the standard ethical guidelines(National Institutes of Health, publication 85-23, revised 1985,and European Community Guidelines on the Care and Use of LaboratoryAnimals) and approved by the local ethics committee. Male CD-1mice (22-24 gm) (Charles River) were intraperitoneally injectedwith cocaine (20 mg/kg; Sigma) dissolved in 0.9%NaCl.

Tissue preparation and immunohistochemistry. Tissue preparation was performed as described by Valjent et al. (2000). Briefly,mice were rapidly anesthetized by intraperitoneal injection ofpentobarbital (Sanofi) before intracardiac perfusion of 4% PFAin 0.1 M Na₂HPO₄/NaH₂PO₄ buffer, pH 7.5, delivered with a peristalticpump at 20 ml/min for 5 min. Brains were then postfixed overnightin the same fixative solution and stored at 4°C. Sections (30µm) were cut with a Vibratome (Leica) and then kept in a solutioncontaining 30% ethylene glycol, 30% glycerol, 0.1 M phosphatebuffer, and 0.1% diethylpyrocarbonate (Sigma, Deisenhofen, Germany)at $-$ 20°C until they were processed for immunohistochemistry asdescribed by Valjent et al. (2000). For detection of phosphorylatedproteins, 0.1 mM NaF was included in all buffers and incubationsolutions. On day 1, free-floating sections were rinsed in Tris-bufferedsaline (TBS; 0.25 M Tris and 0.5 NaCl, pH 7.5) and incubated for15 min with 0.2% Triton X-100 in TBS. After three rinses, floatingsections were saturated for 1 hr with 3% BSA, 0.2% Triton in TBS.Then, the sections were rinsed three times in TBS and incubatedwith the primary antibody (P-T-Akt, 1:500; UBI, Euromedex) overnightat 4°C in TBS containing 1% BSA and 0.1% Triton. On day 2, afterthree rinses in TBS, sections were incubated for 2 hr at roomtemperature with the anti-rabbit Cy3-conjugated antibody (1:250;Amersham). After three rinses in TBS, tissue sections were mountedunder coverslips using Vectashield (Vector) for fluorescent confocalmicroscopicexamination.

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INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effects of D1 and D2 receptor stimulation on phosphorylation levels of Akt in striatal neurons

Akt activation in response to mitogenic factors is mediated by PI3-kinase, which phosphorylates Akt on two critical residues,Ser⁴⁷³ and Thr³⁰⁸ (Alessi et al., 1996; Alessi and Cohen, 1998). To determine whetherDA agonists could activate Akt in striatal neurons, we used immunocytochemicaldetection with antibodies that specifically recognize P-T-Aktand P-S-Akt. We chose doses of DA-D1 (100 µM) and DA-D2 (10 µM)agonists known to activate ERK in striatal neurons (Yan et al.,1999; Zanassi et al., 2001).

Primary striatal neurons in culture showed very low immunoreactivity for both antibodies in control conditions. Although P-T-Aktimmunoreactivity was strongly and rapidly increased after incubationwith the selective D1 receptor agonist SKF38393 and D2 receptoragonist quinpirole, we failed to detect any increase in P-S-Aktimmunoreactivity by these treatments (Fig. 1A). In light of thisunexpected observation, we analyzed the effect of IGF, which stronglyactivates Akt on both Ser⁴⁷³ and Thr³⁰⁸ residues (Alessi et al., 1996). In contrast to DA agonists, IGFtreatment increased the levels of both P-T-Akt and P-S-Akt instriatal neurons (Fig. 1A).

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Figure 1. Activation of Akt occurs in response to D1 and D2 receptor agonists in striatal neurons. A, Phosphorylation levels of Akt were detected by immunocytochemistry using anti-active anti-phospho-Thr³⁰⁸ (P-T-Akt) and anti-phospho-Ser⁴⁷³ (P-S-Akt) antibodies in control conditions (cont) and in striatal neurons treated for 20 min with the selective D1 agonist SKF38393 (SKF 20) (100 µM), the D2 agonist quinpirole (Quin 20) (10 µM), or IGF (IGF 20) (200 nM). B, Control of specificity of P-T-Akt in the presence of an excess of the immunogen peptide: KDGATMK[pT] FCGT (+pept) or unphosphorylated GST-Akt1 (+Gst-Akt) (bottom panel). C, Western blot analysis of P-T-Akt from subcellular fractionation of striatal neurons. Specific labeling corresponding to the expected molecular weight for Akt was detected in the nuclear compartment during SKF38393, quinpirole, and IGF treatment. As a control of fractionation, CREB immunoblotting was performed showing a specific nuclear immunostaining. D, P-T-Akt-immunoreactive nuclei were quantified during treatment with the D1 and D2 agonists for 10 min (SKF 10 and Quin 10, respectively) and 20 min (SKF 20 and Quin 20, respectively). Data report the percentage of P-T-Akt-positive nuclei when compared with the total number of Hoechst nuclei and are representative of three independent experiments for each treatment. For each experiment, cells were counted from five independent fields (~100 cells for each field). Statistical comparisons were performed using one-way ANOVA followed by post hoc comparison (Newman-Keuls test). *p < 0.05 and **p < 0.01 when compared with the control group.

Thus D1 and D2 agonists induced phosphorylation of Akt solely on Thr³⁰⁸. To confirm the specificity of the immunocytochemical stainingby the P-T-Akt antibody, we added an excess of the peptide correspondingto phosphorylated Thr³⁰⁸ as well as the surrounding amino acids (KDGATMK[pT]FCGT) thatcompletely blocked the immunoreactivity induced by the D1 (Fig.1B) and D2 (data not shown) agonists. The specificity of P-T-Aktantibody was further confirmed using an excess of nonactive Akt1-GSTprotein that did not block P-T-Akt immunolabeling (Fig. 1B). TheThr³⁰⁸ residue lies within the Akt activation loop, a region that whenunphosphorylated negatively regulates the kinase activity of Akt.Therefore, phosphorylation of Thr³⁰⁸ by upstream kinases offers an alternative mechanism to activateAkt. Accordingly, phosphorylation of Akt at Thr³⁰⁸ is sufficient to trigger activation of specific substrates forAkt in some model systems (Yano et al., 1998; Filippa et al.,1999), an observation that we further confirmed using a kinaseassay (see Fig. 6A).

P-T-Akt immunostaining was localized to the nucleus. To confirm this biochemically, we fractionated striatal extracts intothe nucleus and the cytoplasm. As a control of our fractionationprocedure, CREB immunoblotting was performed and showed an immunoreactiveband at 45 kDa, the expected molecular weight for CREB, in thenuclear extract exclusively. From these fractions, we then analyzedthe distribution of P-T-Akt by immunoblotting. This revealed astrong increase in nuclear P-T-Akt after D1, D2, and IGF treatments(Fig. 1C), corresponding to the nuclear labeling found by immunocytochemistry(Fig. 1A). The cytosolic fraction showed considerable reactivityeven in the control extract, in contrast to the immunocytochemicalanalysis, which suggests that this reactivity is nonspecific anda consequence of the denaturing conditions of SDS-PAGE.

P-T-Akt-immunoreactive nuclei were quantified and corresponded to 25% (p < 0.05) and 40% (p < 0.01) of striatal neurons at10 and 20 min of D1 agonist application, respectively (Fig. 1D).Positive nuclei for P-T-Akt appeared with the same kinetics forthe D2 agonist and occurred in 21 and 26% of striatal neuronsafter 10 min (p < 0.05) and 20 min (p < 0.05) of quinpirole treatment,respectively (Fig. 1D).

D1 and D2 receptor stimulation coactivate Akt and ERK in the same striatal neurons

Similarly to Akt, several recent reports indicate that the ERK signaling pathway is activated in response to D1 and D2 receptorstimulation in striatal neurons (Yan et al., 1999; Zanassi etal., 2001). In these studies, ERK1 and ERK2 activation were analyzedby immunoblotting with an antibody that specifically labels theirdually phosphorylated, activated form, namely anti-phospho Tyr²⁰²-Thr²⁰⁴ ERKs. Using this antibody for immunocytochemical analysis, wefound activated ERKs localized to the nucleus at 20 min, afterboth D1 and D2 agonist treatments (Fig. 2A-C). Interestingly,double immunolabeling for activated Akt (polyclonal antibody directedagainst phospho Thr³⁰⁸ Akt; revealed by anti-rabbit Cy3) and activated ERKs (monoclonalantibody directed against phospho Tyr²⁰²-Thr²⁰⁴ ERKs; revealed by anti-mouse FITC), showed colocalization ofP-ERK and P-T-Akt immunolabeling after incubation with DA agonists(Fig. 2A).

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Figure 2. Akt and ERK activation occur in the same striatal subpopulation. A, Double immunostaining of active-Akt [polyclonal phospho-Thr³⁰⁸ Akt (P-T-Akt)] and active-ERK [monoclonal diphospho-Thr²⁰²-Tyr²⁰⁴ p44/p42 MAPK (P-ERK)] was performed using anti-rabbit Cy3- and anti-mouse FITC-coupled secondary antibodies, respectively. Note the colocalization of P-T-Akt and P-ERK immunostaining after 20 min of treatment with the D1 (SKF 20) and D2 (Quin 20) agonists (arrows). B, Single immunostaining of P-T-Akt and P-ERK was performed using polyclonal phospho-Thr³⁰⁸ Akt (P-T-Akt) and polyclonal diphospho-Thr²⁰²-Tyr²⁰⁴ p44/p42 MAPK (P-ERK), respectively. Immunoreactive cells were quantified 20 min after SKF38393 (SKF 20) and quinpirole (Quin 20) treatments (3 independent experiments each). For each experiment and each antibody, cells were counted from five independent fields (~100 cells for each field). Statistical comparisons: *p < 0.05 and **p < 0.01 when compared with the control group (Newman-Keuls test).

These results show that ERKs and Akt activation occur in the same striatal population in response to D1 and D2 stimulation.They also implicate these two intracellular signaling pathwaysas possible downstream effectors of D1 and D2 receptors to nuclearevents.

Signaling pathways underlying D1 receptor regulation of Akt phosphorylation

To assess the role of PI3-kinase in the activation of Akt induced by D1 receptors, we pretreated the primary cultures withthe inhibitor wortmannin at 100 nM, a dose that selectively blocksPI3-kinase (Davies et al., 2000). The cultures were then inducedfor 20 min with D1 agonist or IGF, which correspond to the peaktime point for Akt activation. Although wortmannin totally blockedIGF-induced P-T-Akt (Fig. 3A), it caused no reduction in the numberof D1-induced P-T-Akt-immunoreactive neurons (Fig. 3A-C). Similarresults (data not shown) were observed with LY294002 (50 µM),another commonly used but much less potent inhibitor of PI3-kinase(Davies et al., 2000).

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Figure 3. Signaling pathways underlying Akt phosphorylation during D1 receptor stimulation. A, Immunocytochemical detection of P-T-Akt was analyzed as described in Figure 1 in the presence of wortmannin (Wort) (100 nM) applied 15 min before D1 agonist or IGF treatment (20 min each) (SKF 20 and IGF 20, respectively). B, Immunostaining of P-T-Akt in the presence of the selective inhibitor of PKA, Rp-cAMP (50 µM), or the selective MEK inhibitor, U0126 (10 µM). C, Quantification of P-T-Akt immunolabeling was performed as described in Figure 1. Statistical analysis: *p < 0.05, **p < 0.01 when compared with the corresponding control group; ^#p < 0.05 and ^##p < 0.01 when compared with SKF38393 treatment alone (Newman-Keuls test). D, P-T-Akt (bottom panel) was analyzed as described in Figure 1 in neurons transfected with GFP (top panel) alone (GFP) or in neurons cotransfected with GFP and DN-MEK (GFP/DN-MEK). Arrowheads indicate the same neuron analyzed with filters corresponding to FITC (for GFP-positive neuron) (top panel) or Cy3 (for P-T-Akt) (bottom panel). Note the disappearance of P-T-Akt immunostaining in cells coexpressing GFP and DN-MEK. E, Quantification of P-T-Akt-immuno-reactive neurons was performed from GFP- or GFP/DN-MEK-transfected neurons (C, arrowheads) in control conditions (Cont) and after D1 (SKF 20) agonist treatments. For each experiment, P-T-Akt immunostaining was quantified from 100 transfected cells. Data are representative of three independent experiments for each treatment. **p < 0.01 when compared with the control group; ^##p < 0.01 when compared with neurons transfected with GFP alone (Newman-Keuls test).

D1 receptors elevate intracellular cAMP and thereby activate PKA, which in turn could regulate Akt phosphorylation in striatalneurons. Indeed, preincubation with Rp-cAMP, the selective inhibitorof PKA, totally abolished P-T-Akt immunoreactivity induced bySKF38393 (Fig. 3B-C).

Given the colocalization of P-T-Akt and P-ERK immunolabeling (Fig. 2A,B) we analyzed a possible cross-talk between these twosignaling pathways. Striatal neurons were pretreated with U0126,a selective inhibitor of MEK, the activating kinase for ERK1/2(Favata et al., 1998), before SKF38393 addition. U0126 totallyblocked P-ERK immunoreactivity as expected (Fig. 4A) and significantlyreduced ( $-$ 50%; p < 0.01) the number of P-T-Akt-immunoreactivenuclei (Fig. 3B,C). A similar reduction in P-T-Akt-positive neuronswas found in cells overexpressing a dominant-negative form ofMEK (DN-MEK) (Fig. 3D,E). These results indicate that activationof the ERK pathway is involved in the phosphorylation and nucleartranslocation of Akt induced by D1 receptor stimulation.

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Figure 4. Signaling pathways underlying ERK phosphorylation during D1 receptor stimulation. A, Immunocytochemical detection of SKF38393-induced P-ERK was analyzed as described in Figure 2C, in the presence of wortmannin (Wort) (100 nM), Rp-cAMP (50 µM), or U0126 (10 µM). B, Quantification of P-ERK immunolabeling was performed as described in Figure 2C. Statistical analysis: *p < 0.05, **p < 0.01 when compared with the corresponding control group; ^#p < 0.05, ^##p < 0.01 when compared with groups in the presence or not of the inhibitors (Newman-Keuls test).

Because recent evidence implicates PI3-kinase in the activation of ERK in striatal neurons (Perkinton et al., 1999), we analyzedthe effect of wortmannin on D1-induced ERK activation. As withAkt, the inhibitor did not reduce P-ERK immunoreactivity but actuallyled to a slight increase (Fig. 4A,B) that was also observed withoutD1 agonist treatment (Fig. 4A,B). This indicates that PI3-kinaseexerts a tonic inhibitory control on basal and D1-induced ERKactivity. Notably, Rp-cAMP pretreatment, which totally inhibitedP-T-Akt induction (Fig. 3A,B), only partially reduced (Fig. 4B)( $-$ 50%; p < 0.01) P-ERK immunoreactivity after D1 agonisttreatment.

Thus, D1 receptor signaling to Akt in striatal neurons does not require PI3-kinase activation but instead is totally linkedto PKA activation with a contribution ofERK.

Signaling pathways underlying D2 receptor regulation of Akt phosphorylation

The D2 agonist quinpirole induced P-T-Akt in a subpopulation of striatal neurons (Fig. 1A,D). Although $beta$ $gamma$ subunits of G_o/i-coupledreceptors activate PI3-kinase in some model systems (Stephenset al., 1994; Hawes et al., 1996; Lopez-Ilasaca et al., 1997),we failed to detect any effect of wortmannin on the inductionof either P-T-Akt or P-ERK by quinpirole [(Fig. 5A,B) and datanot shown]. In contrast, the MEK inhibitor U0126, applied beforequinpirole, totally abolished P-T-Akt (Fig. 5A,B). Similarly,quinpirole-induced P-T-Akt was inhibited in striatal neurons expressingDN-MEK (Fig. 5C,D). Thus, D2 signaling to the Thr³⁰⁸ residue of Akt is entirely coupled to the ERK cascade in ourmodel system.

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Figure 5. Signaling pathways underlying Akt phosphorylation during D2 receptor stimulation. A, Immunocytochemical detection of quinpirole-induced P-T-Akt was analyzed as described in Figure 1, in the presence of wortmannin (Wort) (100 nM) or U0126 (10 µM). B, Quantification of P-T-Akt immunolabeling was performed as described in Figure 1. Statistical analysis: **p < 0.01 when compared with the corresponding control group; ^##p < 0.01 when compared with SKF38393 treatment alone (Newman-Keuls test). C, During quinpirole treatment, P-T-Akt (bottom panel) was analyzed as described in Figure 3 in neurons transfected (arrowheads) with GFP alone (GFP) or with GFP and DN-MEK (GFP/DN-MEK) (bottom panel). D, Quantification of P-T-Akt-immunoreactive neurons in transfected neurons as described in Figure 3E. Statistical analysis: **p < 0.01 when compared with the control group; ^##p < 0.01 when compared with neurons transfected with GFP alone (Newman-Keuls test).

Overexpression of a dominant-negative form of Akt inhibits CREB phosphorylation induced by D1 but not D2 receptor stimulation

Although D1 and D2 receptors are differentially coupled to intracellular cAMP production, i.e., positively for D1 and negativelyfor D2 (Stoof and Kebabian, 1981), CREB phosphorylation at Ser¹³³ can occur in response to stimulation of both DA receptor subtypes.CREB phosphorylation can occur in response to multiple kinases,including PKA, Ca²⁺/calmodulin kinases (CaMKs) II and IV, and kinases activated byERK, such as pp90 ribosomal S6 kinase (RSK) (for review, see Shaywitzand Greenberg, 1999) and mitogen- and stress-activated proteinkinase 1 (MSK1) (Deak et al., 1998). In fact, D1 agonist-inducedCREB phosphorylation is controlled, at least in part, by ERK (Zanassiet al., 2001), whereas D2 agonist-induced CREB phosphorylationinvolves the CaMK pathway (Yan et al., 1999).

CREB phosphorylation has recently been shown to occur in response to Akt in vitro as well as in vivo (Du and Montminy, 1998).Given this, we tested whether Akt is linked to CREB phosphorylationinduced by DA agonists. As a first assay, we immunoprecipitatedAkt from striatal neuron extracts after various treatments andtested its activity toward recombinant GST-CREB_1-166 (Fig.6A). This test first confirmed that D1-induced P-T-Akt was associatedwith increased kinase activity. Furthermore, it showed clearlythat CREB was a direct substrate of the activated Akt after D1agonist treatment. Surprisingly, the D2 agonist failed to activateAkt in this test, a result that could be explained by the lowpercentage of striatal neurons activated for Akt after this treatment(26%) (Fig. 1A-D).

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Figure 6. Activated Akt controls CREB phosphorylation induced by D1 agonist treatment. A, Striatal neurons were treated for 20 min with SKF, quinpirole, and IGF as indicated. Akt was immunoprecipitated from neuronal lysates using an antibody corresponding to the PH domain, and

We next assayed the effect of transfecting striatal neurons with DN-Akt, which lacks most phosphorylation sites for its activation,including Thr³⁰⁸, together with a GFP expression clone to identify the transfectedcells. Overexpressed DN-Akt showed both nuclear and cytosoliclocalization (Fig. 6B), thus illustrating that inactive Akt isfound in both compartments. Although Akt has been show to playa key role in cell survival, we failed to detect any apoptoticcharacteristics in striatal neurons overexpressing DN-Akt (4 vs3.3% of apoptotic nuclei in neurons transfected with GFP + DN-Aktwhen compared with GFPalone).

CREB phosphorylation induced by the DA agonists in cellulo was analyzed by immunocytochemistry, using an anti-P-CREB antibodyfrom neurons transfected with GFP, used as a control for transfection.After D1 agonist treatment, striatal neurons, including the transfectedneurons positive for GFP, showed a strong increase of CREB phosphorylationin the nucleus (Fig. 6C) after 10 and 20 min. This occurred in40% (10 min) and 46% (20 min) of transfected neurons (Fig. 6C,D).The D2 agonist treatment also induced CREB activation in the majorityof cultured striatal neurons, including the GFP-positive, transfectedneurons (52 and 65% for 10 and 20 min treatment, respectively;p < 0.01) (Fig. 6C,D). More neurons showed P-CREB-positive nucleiafter D2 agonist treatment relative to D1 (65 vs 46% at 20min).

CREB activation was then analyzed in striatal neurons cotransfected with GFP and DN-Akt expression vectors. No CREB activationwas found before induction. After D1 agonist treatment, the percentageof P-CREB-immunoreactive nuclei was strongly reduced in cotransfectedneurons at both 10 and 20 min (approximately $-$ 50%; p < 0.01) (Fig.6C,D). These data implicate the Akt pathway as an important effectorof CREB phosphorylation in response to D1 stimulation. Quinpirole-inducedCREB phosphorylation was unchanged in the presence of DN-Akt 10min after induction, but then showed a slight but significantreduction ( $-$ 9%; p < 0.05) at 20 min (Fig. 6C,D).

Akt is activated in striatal neurons in vivo

Having established that Akt was activated by DA agonists in primary striatal neurons in culture, we wished to analyze thephysiological relevance of these in vitro observations. For thispurpose, we used in vivo administration of cocaine, a psychotropedrug known for its addictive properties. Cocaine considerablyincreases DA levels in the striatum. Activation of Akt was analyzedafter acute cocaine administration, using the same approach asabove, i.e., immunocytochemical detection of P-T-Akt and P-S-Aktfrom striatal sections. Similarly to the in vitro study, no P-S-Aktimmunoreactivity was found after acute cocaine administration(data not shown). In striatal sections from mice treated withsaline, no P-T-Akt immunoreactivity was found (Fig. 7). This immunoreactivitywas increased significantly in striatal neurons, 10 and 20 minafter cocaine administration. Confocal analysis clearly showednuclear labeling of P-T-Akt at 20 min of cocaine treatment. Thusthese data give in vivo evidence that Akt is activated in striatalneurons by DA.

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Figure 7. In vivo activation of Akt in striatal neurons after cocaine administration. P-T-Akt immunostaining was performed in striatal sections of mice treated with saline or cocaine. P-T-Akt immunoreactivity was increased 10 and 20 min after cocaine (20 mg/kg, i.p.) administration (coc 10 and coc 20, respectively). Shown is fluorescent confocal analysis of P-T-Akt immunolabeling. Note its nuclear labeling during cocaine treatment (coc 20). Data are representative of at least four independent mice for each treatment. its kinase activity was determined with GST-CREB_1-166 as a substrate. After washing to eliminate unincorporated radioactivity, samples were subjected to 10% SDS-PAGE (data are representative of 3 independent experiments). B, Immunolocalization of HA-tagged-DN-Akt (DN-Akt) was analyzed with an anti-HA antibody. Note the localization of DN-Akt in both cytosolic (including neuritic extension) and nuclear compartments. Note also the nuclear integrity (Hoechst) of neuronal cells overexpressing DN-Akt. C, CREB phosphorylation was analyzed by immunocytochemical detection of the anti-P-CREB antibody. Note that P-CREB immunostaining is strongly induced during SKF38393 treatment (SKF 20), including in a GFP-transfected neuron (arrowhead). During SKF (arrowhead) but not quinpirole (Quin 20) (arrowhead) treatment, note the disappearance of P-CREB immunostaining in cells cotransfected with GFP and DN-Akt (GFP/DN-Akt). D, Quantification of P-CREB-immunoreactive neurons was performed from GFP or GFP + DN-Akt-transfected neurons in control conditions (Cont), after D1 (SKF 10 and SKF 20) or D2 (Quin 10 and Quin 20) agonist treatments. For each experiment, P-CREB immunostaining was quantified from 100 transfected cells. Data are representative of three independent experiments for each group. *p < 0.05 and **p < 0.01 when compared with the corresponding control group; ^#p < 0.05 and ^##p < 0.01 when compared with neurons transfected with GFP alone (Newman-Keuls test).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We show here that the activation of Akt occurs in response to both DA-D1 and DA-D2 receptor stimulation in striatal neurons.This activation, which occurs independently of PI3-K, leads toits nuclear translocation where it controls CREB phosphorylation,at least after D1 treatment. Together with the in vivo demonstrationthat Akt is activated in striatal neurons after acute cocainetreatment, our data provide the first evidence that Akt is aneffector of DA signaling to gene expression and thereby providesa new signaling pathway to long-term neuronal adaptation in thestriatum.

In our model system, phosphorylation of Akt induced by the D1 agonist was totally dependent on increases in intracellularcAMP levels. This is not the first demonstration that Akt canbe activated, i.e., phosphorylated at Thr³⁰⁸ residues by increases of intracellular cAMP levels (Sable etal., 1997) independently of PI3-kinase. It was demonstrated recentlythat forskolin-induced stimulation of Akt was dependent on PKA,although not directly, because overexpression of the constitutivelyactive catalytic subunit of PKA was able to activate Akt, butmutation of the sole consensus phosphorylation site for PKA intoinactive residue did not impair this activation (Filippa et al.,1999).

One possible intermediate could be the ERK pathway, because both the MEK inhibitor U0126 and overexpression of the DN-MEKinhibited P-T-Akt immunoreactivity, at least in part. In thisway, recent data support the possibility that MSK1, a kinase activatedby ERK, controls the activation of Akt (Nomura et al., 2001).Among second messengers that are responsible for the link betweenD1 receptor stimulation and ERK activation can be the small Ras-relatedG-protein Rap1, activated by PKA or cAMP-guanine nucleotide exchangefactor (Kawasaki et al., 1998; Yao et al., 1998; York et al.,1998). However, signaling to ERK by D1 agonists is complex andmay also implicate indirect pathways, such as increased levelsof intracellular calcium by PKA and subsequent activation of PYK2and PKC (Zanassi et al., 2001). Besides ERK, increased calciumlevels can also activate calcium-calmodulin (CaM)-dependent proteinkinases, including CaM kinase kinase which is known to phosphorylatedirectly Akt on Thr³⁰⁸ independently of Ser⁴⁷³, as demonstrated recently in neuroblastoma cell lines (Yano etal., 1998). Thus multiple and complex intracellular intermediatesmight be responsible for the PKA-dependent activation of Akt thatwe found in the presentstudy.

We also found an effect of the D2 agonist in the activation of Akt. Studies on other G_o/i-protein-coupled receptors, includingopioid receptors, have shown an important role of the G $beta$ $gamma$ subunitas an activator of PI3-kinase activity (Polakiewicz et al., 1998;for review, see Luttrell et al., 1999). In our study, we foundno inhibition of D2-induced phosphorylation of Akt by wortmannin,but instead a total inhibition by the MEK inhibitor and the DN-MEK.Of interest, although G $beta$ $gamma$ subunits are also responsible for ERKactivation in some model systems (for review, see Luttrell etal., 1999), it was demonstrated recently that D2 receptor signalingto ERK implicates a G_q-protein activation of PLC $beta$ , which in turncan control intracellular calcium levels and activation of PKC(Yan et al., 1999). Thus, it is likely that intracellular signalingby D2 receptor stimulation does not require G $beta$ $gamma$ subunits. Differencesin cell lines (Chinese hamster ovary vs primary culture of neurons)as well as experimental procedures (overexpression of a receptorvs natural stimulation) could account for these apparentdiscrepancies.

An important finding was nuclear translocation of activated Akt after D1 and D2 agonist treatments. Cellular mechanisms underlyingphosphorylation of Akt at Thr³⁰⁸ residues have been well studied during growth factor stimulation.They necessitate a preliminary essential step, which is translocationof Akt from the cytosol to the membrane, by a mechanism that requiresPI3-kinase activation (Hemmings, 1997; Toker and Cantley, 1997;Falasca et al., 1998). This translocation allows a correct conformationfor the activating phosphorylation by PDK1. Then Akt detachesfrom the membrane, which enables it to translocate to the nucleus.In conditions during which Akt is activated independently of PI3-kinase,for example by a PKA-dependent pathway, the same sequence of intracellularevents occurs, i.e., translocation to the plasma membrane, followedby its dissociation and nuclear translocation. However, blockingmembrane translocation by wortmannin treatment had no effect onthe phosphorylation of Akt at Thr³⁰⁸ and failed to affect its nuclear localization (Filippa et al.,1999). Thus, the precise cellular mechanisms underlying nucleartranslocation of Akt during stimuli that do not require PI3-kinaseactivity remain to beestablished.

During growth factor stimulation, the best characterized nuclear substrates of Akt are Forkhead and CREB (Du and Montminy,1998; Brunet et al., 1999; for review, see Datta et al., 1999;Brunet et al., 2001). By controlling the phosphorylation stateof these transcription factors, Akt is critically involved incell survival. CREB phosphorylation has long been considered acritical event involved in memory formation (for review, see Mayfordand Kandel, 1999) as well as neuronal adaptation to drugs of abuse(Blendy and Maldonado, 1998). Thus, by controlling the transcriptionalrate of anti-apoptotic genes such as Bcl-2 (Riccio et al., 1999),genes involved in synaptic plasticity, including c-fos (Ginty,1997) or BDNF (Shieh and Ghosh, 1999), as well as precursors ofneurotransmitters implicated in drug addiction, such as dynorphin(Carlezon et al., 1998), CREB is a key mediator of long-term phenotypicchanges inneurons.

CREB phosphorylation can be induced in striatal neurons, during D1 and D2 receptor stimulation, via distinct pathways. Thus,in striatal slices or primary striatal cultures, D1 receptor-mediatedCREB phosphorylation is highly dependant on PKA (Das et al., 1997)but also, albeit partly, on the ERK pathway (Zanassi et al., 2001).Our data showing that overexpression of DN-Akt impairs P-CREBimmunolabeling strongly support the possibility that Akt is alsoinvolved in CREB phosphorylation during D1 receptor stimulation.Thus, CREB is a common target to multiple kinases activated byD1 receptors: PKA and Akt, which directly phosphorylate Ser¹³³-CREB, and ERK via Rsk and/orMSK.

It was shown recently that D2 receptor-induced CREB phosphorylation requires activation of PKC and CaMK, but not ERK (Yanet al., 1999). We show here that overexpression of DN-Akt failedto affect CREB phosphorylation after 10 min of D2 agonist treatment.However, a slight but significant reduction was found after 20min, thus implicating, at least partly, Akt in CREB phosphorylationat this time point. An important observation here is that duringD2 receptor stimulation, the number of P-CREB-immunoreactive nucleiwas higher (60%) than P-ERK and P-T-Akt (25%). From these resultswe can conclude that activated ERK, and thereby Akt, controlsCREB phosphorylation only in a subpopulation of striatal neuronsexpressing D2 receptors. This might explain why, from global Westernblot analysis, Yan et al. (1999) failed to detect any effect ofERK signaling in D2-induced CREB phosphorylation. It could beinteresting now to analyze whether the ERK/Akt/CREB module issimilarly regulated by D2 agonists in striatopallidal neurons,which mainly express D2 receptors (i.e., ~50% of medium spinyneurons) (Bloch and Le Moine, 1994), and in striatonigral neurons,which mainly express D1 but also a significant level of D2 receptors(Aizman et al., 2000). This could provide a new basis for furtherunderstanding how synergistic actions of D1 and D2 can occur instriatalneurons.

An important finding was that the same activation of Akt occurred in vivo in response to cocaine, a psychotrope drug knownto induce long-term neuronal changes in the striatum. Similarkinetics of P-T-Akt immunoreactivity was found when compared withstriatal neurons in culture. We note that ERK activation was alsofound to be activated in the striatum during acute cocaine administration,again with kinetics similar to those found in vitro (Valjent etal., 2000). In this article we clearly showed that ERK activationwas involved in both gene regulation and addictive behavior, measuredin the place preference test. Thus, further elucidation of therole of Akt in drug addiction is now a criticalissue.

To conclude, we propose that Akt participates in a sequential activation of CREB phosphorylation in response to D1 receptorstimulation. Thus, this transduction pathway, along with otherseveral different protein kinases, including PKA and MAPK/ERK,could convey the prolonged phosphorylation of CREB that is necessaryto control gene expression (Wu et al., 2001) and thereby long-termneuronal adaptation in thestriatum.

  FOOTNOTES

Received June 3, 2002; revised July 23, 2002; accepted July 26, 2002.

This work was supported by the Université Pierre et Marie Curie (UPMC), the Centre National de la Recherche Scientifique (CNRS),the Ministère de la Recherche (Action Contertée Incitative Développementet Physiologie Intégrative), and the Association pour la Recherchesur le Cancer (contract 5618 to J.C. and 5890 to R.A.H.). K. Brami-Cherrierwas supported by the CNRS and Fondation Lejeune. E. Valjent wassupported by a grant from "Fondation pour la Recherche Médicale."We thank Dr. Dario Alessi for the generous gift of DN-Akt plasmid,Dr. Marie Körner for technical help, and Richard Schwartzmannfor confocalanalysis.

Correspondence should be addressed to Jocelyne Caboche, Laboratoire de Neurobiologie des Processus Adaptatifs, Centre Nationalde la Recherche Scientifique/UPMC, Unité Mixte de Recherche 7102,9 quai Saint Bernard, 75005 Paris, France. E-mail: Jocelyne.Caboche{at}snv.jussieu.fr.

E. Valjent's present address: Laboratoire Transduction du Signal et Plasticité dans le Système Nerveux Central, InstitutNational de la Santé et de la Recherche Médicale Unité 536,17 rue du Fer à Moulin, 75005 Paris,France.

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