Brain-Derived Neurotrophic Factor Induces Long-Term Potentiation in Intact Adult Hippocampus: Requirement for ERK Activation Coupled to CREB and Upregulation of Arc Synthesis

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The Journal of Neuroscience, March 1, 2002, 22(5):1532-1540

Brain-Derived Neurotrophic Factor Induces Long-Term Potentiation in Intact Adult Hippocampus: Requirement for ERK Activation Coupled to CREB and Upregulation of Arc Synthesis
Shui-Wang Ying¹^,^*, Marie Futter²^,^*, Kobi Rosenblum², Mark J. Webber³, Stephen P. Hunt³, Timothy V. P. Bliss², and Clive R. Bramham¹
¹ Department of Physiology and Locus on Neuroscience, University of Bergen, N-5009 Bergen, Norway, ² Division of Neurophysiology, National Institute for Medical Research, London NW7 1AA, United Kingdom, and ³ Department of Anatomy and Developmental Biology, University College London, London WC1E 6BT, United Kingdom

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Brain-derived neurotrophic factor (BDNF) is implicated in long-term synaptic plasticity in the adult hippocampus, but thecellular mechanisms are little understood. Here we used intrahippocampalmicroinfusion of BDNF to trigger long-term potentiation (BDNF-LTP)at medial perforant path-granule cell synapses in vivo. BDNF infusionled to rapid phosphorylation of the mitogen-activated protein(MAP) kinases ERK (extracellular signal-regulated protein kinase)and p38 but not JNK (c-Jun N-terminal protein kinase). These effectswere restricted to the infused dentate gyrus; no changes wereobserved in microdissected CA3 and CA1 regions. Local infusionof MEK (MAP kinase kinase) inhibitors (PD98059 and U0126) duringBDNF delivery abolished BDNF-LTP and the associated ERK activation.Application of MEK inhibitor during established BDNF-LTP had noeffect. Activation of MEK-ERK is therefore required for the induction,but not the maintenance, of BDNF-LTP. BDNF-LTP was further coupledto ERK-dependent phosphorylation of the transcription factor cAMPresponse element-binding protein. Finally, we investigated theexpression of two immediate early genes, activity-regulated cytoskeleton-associatedprotein (Arc) and Zif268, both of which are required for generationof late, mRNA synthesis-dependent LTP. BDNF infusion resultedin selective upregulation of mRNA and protein for Arc. In situhybridization showed that Arc transcripts are rapidly and extensivelydelivered to granule cell dendrites. U0126 blocked Arc upregulationin parallel with BDNF-LTP. The results support a model in whichBDNF triggers long-lasting synaptic strengthening through MEK-ERKand selective induction of the dendritic mRNA species Arc.

Key words: brain derived neurotrophic factor; BDNF; long-term potentiation; LTP; extracellular signal-regulated protein kinase; ERK; mitogen-activated protein kinase; MAPK; activity-regulated cytoskeleton-associated protein; Arc; synaptic plasticity; hippocampus; dentate gyrus

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurotrophins play diverse roles in regulating neuronal structure, function, and survival during development and into adulthood(Song and Poo, 1999; Bibel and Barde, 2000; Kaplan and Miller,2000). Recent studies suggest that one of the neurotrophins, brain-derivedneurotrophic factor (BDNF), plays a critical role in long-termsynaptic plasticity in the adult brain (Schuman, 1999; Schinderand Poo, 2000). The weight of evidence stems from studies of long-termpotentiation (LTP) of glutamatergic synapses in the adult hippocampus.LTP, evoked by high-frequency afferent stimulation (HFS-LTP),is typically divided into an early, labile phase dependent oncovalent modifications of existing proteins and a late, stablephase requiring new synthesis of mRNA and protein (Bliss and Collingridge,1993; Nguyen and Kandel, 1996). Experiments involving inhibitionof endogenous BDNF and signaling through its TrkB receptor tyrosinekinase suggest that BDNF is required for generating late LTP (Pattersonet al., 1996; Figurov et al., 1996; Kang et al., 1997; Korte etal., 1998; Chen et al., 1999; Minichiello et al., 1999). However,the mechanism of BDNF action is littleunderstood.

Exogenously applied BDNF has a range of rapid, short-lasting effects depending on the developmental stage of the preparationand the method of application (Schinder and Poo, 2000). In culturedimmature hippocampal neurons, BDNF evokes a transient facilitationof excitatory synaptic transmission lasting on the order of minutes(Lessmann and Heumann, 1998; Li et al., 1998; Crozier et al.,1999). This contrasts with the situation in the adult hippocampusin which exogenous BDNF can evoke lasting changes in synapticefficacy. In a series of studies using bath perfusion of BDNFonto hippocampal slices, Schuman and colleagues demonstrated long-lastingenhancement of transmission at Schaffer collateral-CA1 synapses(Kang and Schuman, 1995, 1996; Kang et al., 1997). For reasonsthat are still unresolved, possibly related to synaptic accessof BDNF, these in vitro findings have not been replicated (Kanget al., 1996; Patterson et al., 1996; Frerking et al., 1998).However, using intrahippocampal infusion of BDNF in the intactrat, we observed robust long-lasting potentiation at perforantpath-granule cell synapses in the dentate gyrus (Messaoudi etal., 1998).

This effect, termed BDNF-induced LTP (or BDNF-LTP), provides a tool for elucidating BDNF mechanisms in synaptic plasticity.If BDNF participates in triggering late LTP, it should somehowregulate new protein synthesis. New proteins could derive fromtranslation of existing mRNA and/or from new transcription. Schumanand colleagues have provided evidence that BDNF stimulates proteinsynthesis in dendrites from existing mRNA (Kang and Schuman, 1996;Aakalu et al., 2001). However, long-term cellular responses toneurotrophins such as differentiation and survival require transcription.Current models of late HFS-LTP suggest a mechanism requiring activationof the extracellular signal-regulated protein kinase (ERK), ERK-dependentphosphorylation of the nuclear transcription factor calcium- andcAMP-response element binding protein (CREB), and the subsequenttranscription of CRE-driven genes (Impey et al., 1996, 1998; Daviset al., 2000). Two calcium-regulated immediate early genes, activity-regulatedcytoskeleton-associated protein (Arc, also known as Arg3.1) andZif268, were demonstrated recently to be required in late LTPand long-term memory (Guzowski et al., 2000; Jones et al., 2001).These genes are likely to have very distinct functions in lateLTP; Arc mRNA is rapidly transported to dendrites and translated,whereas Zif268 regulates the transcription of late responsegenes.

Here we explored the mechanism of BDNF-LTP in the dentate gyrus in vivo. Using local microinfusion of selective inhibitorsof ERK activation and immunoblotting for phosphorylated ERK, wedemonstrate a requirement for ERK activation in the induction,but not the expression, of BDNF-LTP. We further show ERK-dependentactivation of CREB and robust upregulation of Arc mRNA and protein.Interestingly, Zif268 was not affected. The results support amodel in which BDNF triggers long-lasting synaptic strengtheningthrough MEK [MAP (mitogen-activated protein) kinase kinase]-ERKand selective induction of the dendritic mRNA species Arc.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects. Data was obtained from 94 male Mol:SD rats (M&B A/S, Ry, Denmark), weighing 250-320 gm. Animals were housed in atemperature- and light-controlled vivarium (23 ± 0.5°C; lightson at 7:00 A.M., lights off at 7:00 P.M.) and supplied with food(12-14 pellets per rat per day) and water for at least 1 weekbeforesurgery.

Drugs. Human recombinant met-BDNF (a gift from Amgen-Regeneron Partners, Thousand Oaks, CA) was obtained as a concentratedstock solution (1.0 mg/ml) in PBS (150 mM NaCl, 10 mM sodium phosphatebuffer, pH 7.0, and 0.004% Tween 20), aliquoted in small volumes,and stored at $-$ 80°C until use. Recombinant cytochrome c from yeastwas obtained from Sigma (St. Louis, MO). PD98059 was obtainedfrom Calbiochem-Novabiochem (La Jolla, CA), and U0126 (1,4-diamino-2,3-dicyano-1-4-bis [2-aminophynylthio] butadiene) was generouslyprovided by Dr. James Trzaskos (DuPont Pharmaceuticals, Wilmington,DE). The MEK inhibitors were dissolved in DMSO and diluted inPBS to a final concentration of 30 µM inhibitor containing 0.3%DMSO.

Electrophysiology and intrahippocampal infusion. The procedure for combined recording of medial perforant path-evoked responsesand intrahippocampal infusion was identical to that of Messaoudiet al. (1998) with minor modifications. Rats were anesthetizedwith urethane (1.4-1.8 gm/kg, i.p.), positioned in a stereotaxicframe with the upper incisor bar 2 mm below the interaural line(skull flat position) and given supplemental doses of urethaneas required to maintain a surgical level of anesthesia. Rectaltemperature was maintained at 36°C with a thermostatically controlledelectric heating pad. Stimulating electrodes were bipolar, concentric,stainless steel with a vertical tip separation of 500 µm (SNEX100; Rhodes Medical Instruments, Woodland Hills, CA). A Teflon-coatedstainless steel wire (outer diameter of 112 µm) was used for recording.Stereotaxic coordinates for stimulation of the medial perforantpath in the dorsomedial aspect of the angular bundle were as follows(in mm): 8.0 posterior to bregma, 4.3-4.4 lateral to the midline,and 1.8-2.4 below the dura. Coordinates for recording in the dentatehilus were as follows (in mm): 3.8-4.0 posterior to bregma, 2.2-2.4lateral, and 3.0-3.1 below thedura.

Intrahippocampal infusions were made using a stainless steel cannula system (Plastics One, Roanoke, VA) consisting of an outerguide tube (24 gauge) and an inner infusion tube (31 gauge). Theguide cannula was beveled sharp at the tip to facilitate braininsertion. The recording electrode was glued (cyanoacrylate, Mega-Gbase; Mega Metal, Oslo, Norway) to the shaft of the outer cannulaand cut so that the electrode tip extended 900 µm below the cannulatip. After making a small slit in the dura, this guide cannula-electrodeassembly was slowly lowered until a positive-going field EPSP(fEPSP) of maximum slope was obtained in the dentate hilus. Thefinal depth of the recording electrode ranged between 300 and400 µm below the level of the maximum negative-going fEPSP sinkrecorded in the middle-third of the dentate molecular layer. Theinfusion cannula was then inserted so that the tip protruded 300µm below the end of the guide cannula. The infusion site was located~100 µm above the dentate gyrus (corresponding to deep CA1 stratumlacunosum-moleculare), 300 µm above the medial perforant path-granulecell synapses. Responses were allowed to stabilize for at least1 hr before starting collection of baselineresponses.

Biphasic rectangular pulses of 150 µsec duration were applied every 30 sec throughout the experiment. The stimulation intensityfor test pulses was set to elicit population spike amplitude of30% of the maximal response. The infusion cannula was connectedvia PE50 polyethylene tubing to a 5 µl Hamilton syringe. Solutionswere delivered by an infusion pump at a rate of 80 nl/min. BDNFwas infused over 25 min giving a total dose of 2 µg. This dosecorresponds to the lowest dose giving maximal BDNF-LTP (Messaoudiet al., 1998). The MEK inhibitors were applied at a concentration(30 µM) that blocks ERK activation in response to HFS-LTP in hippocampalslices.

Tissue microdissection and sample preparation. At the end of electrophysiological recording, rats were decapitated, and thebrain was rapidly removed and rinsed with oxygenated ice-coldartificial CSF (in mM: 124.0 NaCl, 25.0 NaHOC₃, 10.0 D-glucose,3.4 KCl, 1.2 KH₂PO₄, 1.0 MgSO₄, and 2.5 CaCL₂, pH 7.4). The dentategyrus and hippocampal CA1 and CA3 regions were rapidly dissectedon ice. Tissues were hand-homogenized with 15 strokes in 300 µlof freshly made SDS sample buffer containing 10% glycerol, 2.3%SDS, 0.01% bromophenol blue, and 0.5% $beta$ -mercaptoethanol in 62.5mM Tris-HCl, pH 6.8 at room temperature. Homogenates were boiledfor 5 min, aliquoted into Eppendorf tubes, and stored at $-$ 80°Cuntiluse.

SDS-PAGE and Western blotting. Aliquots in SDS sample buffer were subjected to SDS-PAGE and Western blot analysis. Proteinlevels were determined using the Lowry method, and all gels wereloaded with equal amounts of protein. Western blots were performedusing 10% tricine gels (1 mm) and Novex (Wadsworth, OH) apparatus.SDS-PAGE gels (10%) were run for ~1 hr at a constant voltage of125 V. After the run, proteins were transferred to nitrocelluloseat a constant voltage of 50 V. Blots were blocked in 5% BSA ona gyro-rocker at 4°C overnight or for 1 hr at room temperature.Primary antibodies recognized either the active, phosphorylatedform (p) or total protein and were anti-dual p-ERK (detects ERK1/2MAPKs phosphorylated at Thr²⁰² and Tyr²⁰⁴; 1:2000; New England Biolabs, Beverly, MA), p-JNK (c-Jun N-terminalprotein kinase)/SAPK1 (stress-activated protein kinase), p-p38/SAPK2,p-CREB (detects phosphorylation at Ser¹³³; 1:500; New England Biolabs), ERK1/2, JNK/SAPK1, p38/SAPK2, CREB(1:1000; New England Biolabs), Arc (1:500; Santa Cruz Biotechnology,Santa Cruz, CA), and Zif268 (1:1000). The primary antibody wasdiluted in Tris-buffered saline solution containing 0.1% Tween20 (TBST) and 5% BSA as specified above, and the blots incubatedfor 2 hr or 4°C overnight with constant shaking. After three washeswith TBST, blots were incubated with HRP-labeled protein A (1:25000in TBST; Zymed, San Francisco, CA) or HRP-labeled donkey anti-goatIgG (1:20000 in TBST; Jackson ImmunoResearch, West Grove, PA).Blots were developed using enhanced chemiluminescence after washingin TBST. Blots were first treated with anti-phospho-specific antibody,stripped with 100 mM 2-mercaptoethanol, 2% SDS, and 62.5 mM Tris-HCl,pH 6.7, 50°C for 30 min, and reprobed with an antibody recognizingtotal protein. Autoradiographs was scanned on a laser densitometerand quantitated using ImageQuant software (Amersham Biosciences,Sunnyvale, CA). Western blots were developed to be linear in therange used fordensitometry.

In situ hybridization histochemistry. Antisense oligonucleotides (45mers) were synthesized (Oswel DNA Service) complementaryto Arc (nucleotides 961-1005) (Lyford et al., 1995) and Zif268(nucleotides 355-399) (Milbrandt, 1987). Oligonucleotides were3' end-labeled with [-³⁵S]dATP (1200Ci/mmol; NEN, Boston, MA) in a 30:1 ratio of radiolabeledATP/oligonucleotide using terminal deoxynucleotidyl transferase(Promega, Madison, WI). Specific activity of the ³⁵S-labeled probe was between 100,000 and 300,000 cpm/µl probe.Hybridizations were performed essentially as described by Wisdenet al. (1990). Cryostat sections (15 µm) were mounted on polylysine-coatedslides, dehydrated, and stored in 95% ethanol. Sections to undergoin situ hybridization were air dried for 1-2 hr. ³⁵S-radiolabeled oligonucleotide probes were hybridized to the sectionsin a sealed humid chamber at 42°C for 14-18 hr. The sections thenunderwent three washes of decreasing stringency (two washes of1× SSC at 55°C for 30 min; one wash of 0.1× SSC at room temperaturefor 1 min). Sections were dehydrated, air-dried, and then opposedto Kodak (Eastman Kodak, Rochester, NY) Biomax MR x-ray film for1-2 weeks. To define nonspecific hybridization, adjacent slide-mountedsections were incubated with radiolabeled oligonucleotide in thepresence of an excess (100×) concentration of unlabeled oligonucleotideprobe.

Data processing and statistical analysis. Signals from the dentate hilus were amplified, filtered (1 Hz to 3 kHz), digitized(25 kHz for field potentials), and stored to computer disk. Acquisitionand analysis of field potentials were accomplished using DataWaveTechnologies (Longmont, CO) WorkBench software. The maximum slopeof the fEPSP and the amplitude of the population spike was measuredfrom its negative-going apex to the tangent line joining the firsttwo positive peaks. Statistical analysis of electrophysiologicaldata are based comparison of the last 10 min of baseline recordingwith 10 min recording sessions obtained after BDNF treatment asindicated.

For Western blot analysis, optical density values obtained from the treated hippocampus were normalized relative to valuesin the nontreated hippocampus for each microdissected region.Statistics were performed using a paired t test for dependentsamples for the immunoblot data and a one-way repeated-measuresANOVA for the electrophysiology data. Differences were consideredsignificant when p < 0.05.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

MEK inhibitors block induction of BDNF-LTP in vivo

TrkB receptors are coupled to three main signaling pathways, including the Ras-ERK protein kinase cascade, phosphoinositide-3kinase, and phospholipase C. The Ras-ERK pathway is critical forlong-term responses requiring gene expression, such as neuronaldifferentiation and growth (Kaplan and Miller, 2000). ERK is activatedby MEK (MAPK, or ERK, kinase), a dual specificity kinase thatphosphorylates ERK on Thr²⁰² and Tyr²⁰⁴. We first explored the role of ERK activation in BDNF-LTP pharmacologically,using intrahippocampal infusion of the MEK inhibitors PD98059and U0126. Both compounds are selective for MEK relative to relatedkinases, as assessed in cell-free assays, cell cultures, and intacthippocampal tissue (Alessi et al., 1995; English and Sweatt, 1997;Favata et al., 1998). MEK inhibitors were applied at a concentration(30 µM) that inhibits ERK activation in the hippocampalslice.

BDNF was infused immediately above the dentate gyrus, ~300 µm dorsal to the synaptic zone of medial perforant path fibers.As shown in Figure 1A, BDNF infusion (2 µg/2 µl, 25 min) led toa robust increase in the slope of the fEPSP and in the amplitudeof the population spike. fEPSP values were significantly elevatedabove baseline at 15 min (p < 0.05; n = 16) (Fig. 1A), climbedgradually to a stable plateau at 3-4 hr after BDNF infusion (Fig.2), and persisted without decrement for as long as we recorded(maximum of 15 hr; data not shown). Infusion of PD98059 (30 µM;n = 8) for 10 min before and during infusion of BDNF completelyabolished this potentiation (Fig. 1A). U0126 (30 µM; n = 8), astructurally and mechanistically distinct MEK inhibitor, alsocompletely blocked development of BDNF-LTP (Fig. 1B). Cytochromec, a protein similar to BDNF in molecular weight and charge, wasused to control for possible nonspecific effects of protein infusion.Figure 1C shows that synaptic transmission remained stable aftercytochrome c infusion (n = 8; p > 0.05). Infusion of PD98059 (n= 6) or U0126 (n = 4) alone also had no significant effect onbaseline transmission (Fig. 1D). The complete block of BDNF-LTPdevelopment by two different MEK inhibitors indicates a requirementfor ERK activation in BDNF-LTP. Furthermore, the results suggestthat maintenance of baseline synaptic efficacy is not dependenton constitutive activation of ERK through MEK.

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Figure 1. MEK inhibitors block BDNF-LTP. Time course plots of medial perforant path-evoked fEPSP and population (Pop) spike responses. Test pulses were applied at a rate of 1 every 30 sec. BDNF (2 µg/2 µl) was infused 300 µm above the medial perforant-granule cell synapses, during the period indicated by the white bar. n = 16. a, Effect of PD98059 on BDNF-LTP. Infusion of 1 µl of PD98059 (30 µM) was followed immediately by infusion of 2 µg of BDNF in 2 µl of PD98059. The period of MEK inhibitor (black bar) and BDNF plus MEK inhibitor (hatched bar) application are indicated. Values are means ± SEM expressed in percentage of baseline. n = 8. Inset above shows traces of averaged field responses (5 sweeps) recorded at the time points indicated. b, Effect of U0126 (30 µM) on BDNF-LTP in a separate groups of animals. n = 8. BDNF-LTP development is abolished by both MEK inhibitors. The group receiving BDNF alone is the same in a and b. c, Cytochrome c (2 µg/2 µl; n = 8) had no significant effect on baseline transmission. d, PD98059 (30 µM; n = 6) and U0126 (30 µM; n = 4) applied alone had no effect on baseline synaptic transmission. fEPSP slope data are shown. Insets are averaged traces as done in c. Infusion of PBS-DMSO vehicle also had no effect on baseline transmission (n = 4; data not shown). Calibration: 3 mV, 4 msec.

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Figure 2. Effect of the MEK inhibitor U0126 on established BDNF-LTP. a, U0126 (30 µM, 2 µl) was infused 110 min after BDNF infusion, during established BDNF-LTP. MEK inhibitor treatment had no significant effect on medial perforant path-evoked responses during infusion or during the subsequent 2 hr recording period. n = 6. b, Effect of vehicle (DMSO-PBS) infusion on established BDNF-LTP. n = 6. c, Summary bar graph of fEPSP slope increases obtained in groups receiving BDNF alone or BDNF and post-treatment with U0126 or PBS. Values are group means + SEM) based on 20 responses collected at the end of recording, 245-255 min after BDNF infusion. n = 6 in all groups. There was no significant difference between groups in the magnitude of BDNF-LTP (p > 0.05).

MEK activation is not required for the expression of BDNF-LTP

The kinetics of BDNF inactivation is not well known, but BDNF is a sticky protein, and tissue clearance is relatively slow.If BDNF is retained in the extracellular space, the observed increasein synaptic efficacy might be attributable to repetitive activationof TrkB rather than induction of a plastic change. To addressthis issue, U0126 was applied during established BDNF-LTP, 2 hrafter BDNF infusion. U0126, applied at a concentration that eliminatesBDNF-LTP development, had no effect when applied after BDNF-LTPwas established (Fig. 2A). Statistical analysis was performedon fEPSP slope values obtained immediately before, immediatelyafter, and 2 hr after U0126 infusion (p < 0.05; n = 6). Treatmentwith the MEK inhibitor vehicle PBS-DMSO also had no significanteffect on established BDNF-LTP (n = 4) (Fig. 2B). The magnitudeof the fEPSP slope increase in rats receiving U0126 or vehicleafter treatment was not significantly different from time-matchedcontrols receiving BDNF alone (p > 0.05) (Fig. 2C). We concludethat (1) BDNF acts rapidly through ERK to induce a long-term increasein synaptic efficacy and (2) ERK activation through MEK is notrequired for expression of the potentiatedstate.

BDNF-LTP triggers rapid activation of ERK and p38 but not JNK

Next we sought to determine the time course of ERK phosphorylation. We also examined two additional MAPK family members, p38kinase (or SAPK2) and JNK (or SAPK1). Homogenates from microdissecteddentate gyrus and hippocampal regions CA1 and CA3 were preparedat 15 min and 3 hr after BDNF infusion and subjected to Westernblotting. Densitometric analysis of phospho-ERK2 showed significantlyelevated levels at 15 min (n = 8) and 3 hr (n = 7) in the infuseddentate gyrus (Fig. 3A,B). No changes in ERK2 phosphorylationwere detected in the CA1 and CA3 fields. Treatment with U0126blocked both the increase in ERK2 phosphorylation (Fig. 3A,B)and the development of BDNF-LTP at 15 min and 3 hr (n = 4 at bothtime points) (Fig. 3C). The results confirm a rapid activationof ERK in response to BDNF and verify the efficacy of MEK inhibitorsin blocking ERK activation. Figure 4 shows the effect of BDNFon p38 and JNK phosphorylation. Interestingly, ERK2 activationwas paralleled by activation of p38 at 15 min and 3 hr in theinfused dentate gyrus, whereas JNK phosphorylation was unaffected.Control infusions with cytochrome c had no effect on ERK, p38,or JNK activity (Figs. 3A, 4A). Total protein levels for thesekinases were monitored throughout and were found to be unchangedacross treatments and hippocampal regions. A representative blotin Figure 3B shows the lack of effect of BDNF on total ERK1/2protein levels in all hippocampal regions.

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Figure 3. BDNF-LTP is coupled to enhanced ERK phosphorylation in the dentate gyrus. Western blot assays of phosphorylated, active ERK (p-ERK1/2) were run on aliquoted samples from microdissected dentate gyrus (DG) and hippocampal regions CA1 and CA3 after in vivo electrophysiological experiments. a, Group mean + SEM changes in p-ERK2 immunoreactivity levels based on densitometric analysis. Optical density values are expressed as a ratio between the treated and nontreated (control) side for each hippocampal subfield. BDNF infusion increased activation of ERK2 at 15 min (n = 8) and 3 hr (n = 7) in the infused dentate gyrus. BDNF had no effect on ERK2 phosphorylation in hippocampal region CA1 or CA3. Delivery of the MEK inhibitor U0126 abolished the increase in ERK2 phosphorylation at both 15 min and 3 hr. n = 4 at both time points. Cytochrome c (Cyt C) infusion had no effect on p-ERK2 immunoreactivity levels. *p < 0.05, significant difference from control. b, Representative p-ERK immunoblots for the group data shown in a. Total ERK2 protein levels were unchanged. c, Bar graph of the fEPSP slope changes obtained at 15 min and 3 hr after infusion. *p < 0.05, significant difference from baseline.

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Figure 4. BDNF-LTP is associated with enhanced activation of p38 MAPK but not JNK. a, Group mean + SEM changes in phosphorylated kinase immunoreactivity levels based on densitometric analysis. Optical density values are expressed as a ratio between the treated and nontreated (control) dentate gyrus. BDNF infusion increased phospho-p38 immunoreactivity at 15 min (n = 8) and 3 hr (n = 7) in the infused dentate gyrus. BDNF infusion had no effect on JNK phosphorylation. Cytochrome c (Cyt C) infusion had no effect on p-p38 or p-JNK immunoreactivity levels. There were no changes in phosphorylation of these kinases in region CA1 or CA3 (data not shown). Total protein levels of p38 and JNK were unchanged in all hippocampal regions across treatments. *p < 0.05, significant difference from control. b, Representative Western blots for group data shown in a.

ERK-dependent CREB activation

ERK activation leading to phosphorylation of CREB at Ser-133 and the expression of CRE-driven genes is implicated in the formationof late phase LTP (Impey et al., 1998; Davis et al., 2000), andBDNF acts through CREB in the regulation of early gene expressionin hippocampal cell cultures (Finkbeiner et al., 1997). We thereforeasked whether BDNF-induced LTP is associated with CREB activation.As shown in Figure 5, CREB Ser¹³³ phosphorylation in the infused dentate gyrus was enhanced 15min after BDNF infusion and returned to control levels at 3 hr.This rapid activation of CREB was abolished by the MEK inhibitorU0126. Thus, BDNF signaling through ERK is required for CREB phosphorylationand induction of BDNF-LTP in vivo.

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Figure 5. BDNF-LTP is coupled to rapid CREB phosphorylation. a, Group mean + SEM changes in p-CREB immunoreactivity levels based on densitometric analysis. CREB-Ser¹³³ was rapidly phosphorylated at 15 min (n = 8), returning to control levels at 3 hr (n = 7) after BDNF infusion. Infusion of the U0126 blocked CREB activation. *p < 0.05, significant difference from control. b, p-CREB Western blots for group data in a.

ERK-dependent upregulation of Arc expression

HFS-LTP is associated with the induction of calcium-regulated immediate early genes encoding Arc and Zif268 (Cole et al.,1989; Wisden et al., 1990; Link et al., 1995; Lyford et al., 1995).Both genes are required for the full development of late LTP andlong-term memory consolidation (Guzowski et al., 2000; Jones etal., 2001). If exogenous BDNF stimulates the generation of lateLTP, one or both of these critical genes should be induced. Wefirst used immunoblotting to determine the effect of BDNF-LTPon Arc and Zif268 protein expression. As illustrated in Figure6, A and B, BDNF led to a threefold elevation in Arc protein levelsat 3 hr in the infused dentate gyrus. Blockade of BDNF-LTP withU0126 completely abolished the increase in Arc protein expression.In contrast, BDNF had no effect on Zif268 levels in the dentategyrus or other hippocampal regions at the same time point (3 hr).The possibility that we missed a time window of Zif268 regulationis unlikely, because Arc and Zif268 show similar activation kineticsafter HFS-LTP, with strong upregulation of Zif268 protein between30 min and at least 4 hr after HFS (Richardson et al., 1992).

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Figure 6. BDNF-LTP is coupled to upregulation of Arc mRNA and protein. a, Group mean + SEM changes in Arc and Zif268 protein immunoreactivity levels. Arc protein expression was increased at 3 hr (n = 7), but not 15 min (n = 8), after BDNF infusion. These increases were confined to the infused dentate gyrus. U0126 blocked the increases in Arc expression. BDNF infusion had no effect on Zif268 protein expression. *p < 0.05, significant difference from control. b, Representative Western blots for group data in a. c, Autoradiographs showing in situ hybridization signals for Arc and Zif268 in the hippocampus 2 hr after BDNF or cytochrome c infusion into the left dentate gyrus. Note the robust increase in the hybridization signal for Arc mRNA in the treated dentate gyrus. d, High-magnification autoradiographic image of the Arc mRNA signal in the dentate gyrus. Model granule cells with apical dendrites extending throughout the molecular layer are depicted in the top and bottom blades of the dentate gyrus. Arc mRNA is strongly upregulated in granule cell bodies and extensively distributed in granule cells dendrites.

Next we performed in situ hybridization histochemistry to assess the expected transcriptional activation of Arc and to gaininsight into the cellular localization of Arc regulation in thedentate gyrus. Brains for in situ hybridization were obtained2 hr after infusion with BDNF or cytochrome c. Arc mRNA levelswere powerfully upregulated in the granule cell layer and thethroughout the molecular layer of the dentate gyrus, indicatingextensive dendritic delivery of Arc transcripts from granule cellsomata into dendrites (Fig. 6C,D). Consistent with the proteinexpression data, BDNF infusion had no effect on Zif268 mRNA levelsin the dentate gyrus. These results link BDNF-LTP to ERK-dependentinduction of Arc gene expression and protein synthesis in granulecells.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Current evidence suggests that BDNF released during or shortly after HFS plays an obligatory role in the generation of lateLTP in the CA1 region of the hippocampal slice. Maintenance ofLTP beyond 1-2 hr is relatively selectively impaired by treatmentwith the BDNF scavenger TrkB-Fc, treatment with function blockingantibodies to BDNF or TrkB, constitutive deletion of a BDNF allele,or conditional deletion of the TrkB gene (Figurov et al., 1996;Patterson et al., 1996; Kang et al., 1997; Korte et al., 1998;Chen et al., 1999; Minichiello et al., 1999).

The present study is the first to explore BDNF mechanisms in long-term synaptic plasticity in vivo. We show that locally appliedBDNF triggers a long-term potentiation (BDNF-LTP) at medial perforantpath-granule synapses, the induction of which (but not the maintenance)requires MEK-ERK activation. We also found that BDNF-LTP is associatedwith ERK-dependent activation of CREB and upregulation of theimmediate early gene Arc. ERK and CREB have emerged as criticalpoints of convergence in the signaling pathways regulating genetranscription in late LTP and long-term memory (Atkins et al.,1998; Impey et al., 1998; Davis et al., 2000). Inhibition of ArcmRNA translation after injection of antisense oligonucleotidesimpairs late LTP and long-term memory consolidation, leaving LTPinduction and memory acquisition intact (Guzowski et al., 2000).The present data show that BDNF triggers synaptic strengtheningand activates a set of cellular events obligatory to developmentof late LTP and long-termmemory.

HFS-LTP experiments have shown that Arc induction is NMDA receptor dependent, but the signal transduction pathways underlyingArc induction are unknown (Link et al., 1995; Lyford et al., 1995;Steward et al., 1998). The possibility that BDNF induces LTP indirectlyby stimulating glutamate release and NMDA receptor activationcan be ruled out because NMDA receptor blockers have no effecton BDNF-LTP in the CA1 region in vitro or dentate gyrus in vivo(Kang and Schuman, 1995; Messaoudi et al., 2000). Our resultsimplicate BDNF as an important regulator of Arc induction in long-termsynaptic plasticity in vivo and demonstrate a requirement forMEK-ERK in the process. Very little information is available onArc function at present, although roles in cytoskeletal reorganizationand regulation of calcium/calmodulin-dependent kinase II localizationin dendrites have been proposed (Guzowski et al., 2000). Previousin vitro work has identified CREB as a major mediator of BDNFresponses (Finkbeiner et al., 1997; Pizzorusso et al., 2000; Iidaet al., 2001). Our results extend this observation to BDNF regulationof synaptic plasticity in vivo. A causal role for CREB and Arcremains to be established, although the parallels to late LTPmechanisms arestriking.

A recent study in Zif268 knock-out mice showed that this gene is required for late LTP (as measured 2 and 3 d after HFS) andhippocampal-dependent long-term memory (Jones et al., 2001). IfBDNF launches late LTP, why does it not activate Zif268? The simplestexplanation is that Arc and Zif268 mediate separable componentsof mRNA synthesis-dependent LTP (Fig. 7). This is consistent withthe different kinetics of Arc and Zif268 function; Arc mRNA isdelivered to dendrites and translated within minutes after HFS,followed by delayed, if overlapping, expression of Zif268-regulatedlate response genes. Arc antisense experiments support an earlyrole for Arc, because treated animals show impaired LTP as earlyas 4 hr after HFS. In seeking to dissect the components of lateLTP, exogenous BDNF-LTP should provide a useful tool for exploringthe Arc effector pathway.

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Figure 7. Model of BDNF signaling pathways underlying BDNF-LTP in the dentate gyrus in vivo. Exogenous application of BDNF triggers LTP through activation of MEK-ERK. ERK activation is required for both CREB phosphorylation and induction of the immediate early gene Arc in dentate granule cells. Arc and Zif268 are both required in late HFS-LTP (Guzowski et al., 2000; Jones et al., 2001), yet they are likely to mediate distinct components of the process; Arc is rapidly delivered to dendrites and translated, whereas Zif268 regulates expression of delayed response genes. Our data suggests the hypothesis that BDNF triggers late LTP through ERK-dependent induction of Arc. HFS must recruit additional pathways to induce Zif268 expression, leading to transcription of late effector genes and full expression of late LTP.

The phenomenon of BDNF-LTP is controversial in the CA1 region in hippocampal slices in which high rates of BDNF perfusionare necessary (Kang et al., 1996). In the present in vivo study,BDNF was applied as a concentrated bolus. The question may beasked whether exogenous application is physiologically relevant.Two lines of evidence support a functional role. First, in triggeringmechanisms critical to late LTP, exogenous BDNF mimics the predictedactions of endogenous BDNF. Second, BDNF-LTP occludes with lateLTP in the CA1 region in vitro and in the dentate gyrus in vivo,indicating common mechanisms of expression (Kang et al., 1997;Messaoudi et al., 2000). The difficulty in obtaining BDNF-LTPin slices may be related to the difficulty in accessing (and rapidlyactivating) signal transducing TrkB receptors at excitatory synapses.Access to the synaptic cleft is strongly inhibited by truncated(noncatalytic) TrkB receptors on glial cells and dendritic shafts,and expression of truncated TrkB is strongly upregulated in adulthood(Biffo et al., 1995; Eide et al., 1996; Drake et al., 1999). Wesuggest that acute, local delivery of a BDNF saturates the truncatedTrkB system, allowing activation of synapticTrkB.

The MEK inhibitor experiments identify a time window of rapid ERK activation critical for BDNF-LTP induction. U0126 blockedBDNF-LTP when applied together with BDNF but had no effect ifapplied 2 hr later. Interestingly, the time course of ERK phosphorylationwas both rapid and sustained. What is the function of the sustainedincrease in ERK activity? One possibility is that it mediatesdelayed gene expression responses that come into play at a laterstage, beyond the recording period used here. In PC12 cells, NGFinduces a sustained ERK activity that is critical for gene inductionresponses leading to neuronal differentiation (Marshall, 1995;Xing et al., 1998). In this system, ERK is persistently activatedafter the formation of a stable upstream complex between the smallG-protein Rap-1 and B-raf, an MEK activator (York et al., 1998).Alternatively, ERK may be retained in a constitutively activatedstate after its dimerization and nuclear translocation (Impeyet al., 1998; Grewal et al., 1999). ERK is rapidly activated inresponse to HFS-LTP in the CA1 region (English and Sweatt, 1996,1997; Impey et al., 1998) and dentate gyrus (Coogan et al., 1999;Maguire et al., 1999; Davis et al., 2000; Rosenblum et al., 2000).Most studies have focussed on relatively early time points, andit is not yet clear whether sustained ERK activation occurs. However,hippocampal-dependent learning is associated with a period oflong-lasting ERK activation (Atkins et al., 1998), and sustainedERK activity is coupled to structural plasticity of dendritesin cultured hippocampal neurons (Wu et al., 2001).

BDNF-LTP was coupled to a parallel activation of ERK and p38 MAPK. Recent data suggests a broad range of physiological functionsfor p38 in processes such as long-term depression, cytoskeletalreorganization, and cell proliferation (Matsumoto et al., 1999;Bolshakov et al., 2000), in addition to its common associationwith pathophysiological processes such as inflammation and neurodegeneration.The p38 activation observed here cannot be attributed to nonspecificeffects of infusion because infusion with a control protein, cytochromec, had no effect on p38 activation (or activation of any of theother kinases examined). Furthermore, BDNF and cytochrome c hadno effect on JNK, the MAPK family member most strongly implicatedin neurodegeneration and apoptosis. Xing et al. (1998) have identifieda pathway in PC12 cells that may be involved. They found thatNGF activates a bifurcated pathway from Ras leading to dual activationof ERK and p38. ERK and p38 then converge through distinct CREBkinases to activate CREB and trigger immediate early genetranscription.

The rapid onset of BDNF-LTP (it was significant 40 min after starting BDNF infusion) seems incompatible with a process dependentsolely on gene expression. ERK has many potential cytosolic substrates,however, and several rapid ERK-dependent mechanisms could be involved(Grewal et al., 1999). One intriguing scenario is that ERK andp38 stimulate protein synthesis at the post-transcriptional levelthrough activation of the Ser/Thr kinase Mnk1 and subsequent phosphorylationof eukaryotic initiation factor 4E (Sonenberg and Gingras, 1998).In the hippocampal CA1 region, BDNF is thought to enhance synapticefficacy by stimulating translation of dendritically localizedmRNA (Kang and Schuman, 1996). Translation activation in dendriteswould precede transcriptional events, going hand-in-hand withthe arrival of Arc mRNA indendrites.

Catalytic TrkB is located on axon terminals and dendritic spines of glutamate synapses and to a lesser extent on terminalsof interneurons and extrinsic modulatory inputs (Drake et al.,1999; Aoki et al., 2000). Presynaptically, BDNF can acutely enhanceglutamate release and attenuate synaptic fatigue in response toHFS (Gottschalk et al., 1998, 1999; Jovanovic et al., 2000; Schinderand Poo, 2000; Xu et al., 2000). Although BDNF clearly functionsas a presynaptic modulator, postsynaptic actions, including newmRNA and protein synthesis, are likely to underlie long-term synapticplasticity. The present data showing ERK-dependent activationof the nuclear transcription factor CREB and upregulation of ArcmRNA in granule cells clearly supports a postsynapticmechanism.

In a recent review, Schinder and Poo (2000) asked whether neurotrophins play an "instructive" role in LTP by inducing synapticpotentiation or a "permissive" role by maintaining housekeepingfunctions that are necessary for the induction and maintenanceof LTP. Our findings support an instructive role in which BDNFtriggers a consolidation process underlying stable synapticstrengthening.

  FOOTNOTES

Received Sept. 5, 2001; revised Dec. 3, 2001; accepted Dec. 5, 2001.

^* S.W.Y. and M.F. contributed equally to thiswork.

This work was supported by European Union Biotechnology Program Grant BIO4-CT98-0333. BDNF was provided by Amgen-RegeneronPartners.

Correspondence should be addressed to Dr. Clive Bramham, Department of Physiology, University of Bergen, Årstadveien 19, N-5009Bergen, Norway. E-mail: clive.bramham{at}pki.uib.no.

Dr. Ying's present address: Department of Anesthesiology A-1050, Weill Medical College of Cornell University, 525 E. 68thStreet, New York, NY10021.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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