Phosphatidylinositol 3-Kinase Regulates the Induction of Long-Term Potentiation through Extracellular Signal-Related Kinase-Independent Mechanisms

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The Journal of Neuroscience, May 1, 2003, 23(9):3679

Phosphatidylinositol 3-Kinase Regulates the Induction of Long-Term Potentiation through Extracellular Signal-Related Kinase-Independent Mechanisms
Patricio Opazo¹, Ayako M. Watabe¹, Seth G. N. Grant², and Thomas J. O'Dell¹
¹ Department of Physiology, David Geffen School of Medicine at University of California at Los Angeles, Los Angeles, California 90095, and ² Department of Neuroscience, University of Edinburgh, Edinburgh EH8 9JZ, United Kingdom

  ABSTRACT

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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Inhibitors of both phosphatidylinositol-3-kinase (PI3-kinase) and MAPK/ERK (mitogen-activate protein kinase/extracellularsignal-related kinase) activation inhibit NMDA receptor-dependentlong-term potentiation (LTP). PI3-kinase inhibitors also blockactivation of ERK by NMDA receptor stimulation, suggesting thatPI3-kinase inhibitors block LTP because PI3-kinase is an essentialupstream regulator of ERK activation. To examine this hypothesis,we investigated the effects of PI3-kinase inhibitors on ERK activationand LTP induction in the CA1 region of mouse hippocampal slices.Consistent with the notion that ERK activation by NMDA receptorstimulation is PI3-kinase dependent, the PI3-kinase inhibitorwortmannin partially inhibited ERK2 activation induced by bathapplication of NMDA and strongly suppressed ERK2 activation byhigh-frequency synaptic stimulation. PI3-kinase and MEK (MAP kinasekinase) inhibitors had very different effects on LTP, however.Both types of inhibitors suppressed LTP induced by theta-frequencytrains of synaptic stimulation, but only PI3-kinase inhibitorssuppressed the induction of LTP by high-frequency stimulationor low-frequency stimulation paired with postsynaptic depolarization.Concentrations of PI3-kinase inhibitors that inhibited LTP whenpresent during high-frequency stimulation had no effect on potentiatedsynapses when applied after high-frequency stimulation, suggestingthat PI3-kinase is specifically involved in the induction of LTP.Finally, we found that LTP induced by theta-frequency stimulationwas MEK inhibitor insensitive but still PI3-kinase dependent inhippocampal slices from PSD-95 (postsynaptic density-95) mutantmice. Together, our results indicate that the role of PI3-kinasein LTP is not limited to its role as an upstream regulator ofMAPK signaling but also includes signaling through ERK-independentpathways that regulate LTPinduction.

Key words: long-term potentiation; hippocampus; phosphatidylinositol 3-kinase; extracellular signal-related kinase II; NMDA receptor; $beta$ -adrenergic receptor

  Introduction

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ABSTRACT
Introduction
Materials and Methods
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Discussion
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The small GTPase Ras as well as Ras regulators and effectors are associated with NMDA-type glutamate receptors in the postsynapticdensity of excitatory synapses (Chen et al., 1998; Kim et al.,1998; Hisatsune et al., 1999; Husi et al., 2000). Although therole of Ras in NMDA receptor-mediated signaling has not been wellcharacterized, several findings indicate that Ras signaling pathwayshave an important role in NMDA receptor-dependent forms of synapticplasticity, such as long-term potentiation (LTP). For instance,mice with mutations affecting H-Ras (Manabe et al., 2000) or theRas GTPase-activating proteins NF1 (neurofibromin) (Costa et al.,2002) and SynGAP (a synaptic Ras-GTPase activating protein) (Komiyamaet al., 2002) have alterations in hippocampal LTP. Moreover, pharmacologicalinhibition of the Ras effectors phosphatidylinositol 3-kinase(PI3-kinase) (Kelly and Lynch, 2000; Lin et al., 2001; Raymondet al., 2002; Sanna et al., 2002) and the p44/42 MAPK (mitogen-activatedprotein kinase) pathway (for review, see Sweatt, 2001; Adams andSweatt, 2002) disruptsLTP.

Although Ras-activated signaling pathways are clearly involved in LTP, the molecular details of how these pathways contributeto an enhancement of synaptic strength remain unclear and, insome cases, controversial. For example, whereas the enhancementof LTP in H-Ras mutant mice suggests that Ras activation normallysuppresses LTP induction (Manabe et al., 2000), the inhibitionof LTP in hippocampal pyramidal cells expressing a dominant-negativeform of Ras (Zhu et al., 2002) suggests just the opposite, i.e.,Ras activation is required for LTP induction. The role of PI3-kinasein LTP is also poorly understood. Activation of the MAPK ERK2(extracellular signal-related kinase 2) by NMDA receptor stimulationis completely dependent on PI3-kinase activity in cultured neurons(Chandler et al., 2001; Perkinton et al., 2002), suggesting thatPI3-kinase inhibitors suppress LTP because PI3-kinase activityis required for NMDA receptor-mediated ERK activation. However,in non-neuronal cells, the requirement for PI3-kinase activityin ERK activation is very dependent on experimental conditions(Duckworth and Cantley, 1997; Wennström and Downward, 1999; Moellinget al., 2002), and, in some cases, PI3-kinase activation can inhibit,rather than facilitate, ERK activation (Rommel et al., 1999; Zimmermannand Moelling, 1999). These complex interactions between PI3-kinaseand ERK signaling pathways have not been examined in neurons.Thus, it is not clear whether PI3-kinase inhibitors suppress LTPsolely because PI3-kinase activation is required for NMDA receptor-dependentERK activation or because LTP is also dependent on PI3-kinasesignaling through ERK-independentmechanisms.

In the experiments described here, we examined the role of PI3-kinase and ERK in LTP at excitatory synapses in the CA1 regionof the mouse hippocampus. Consistent with the notion that PI3-kinaselinks NMDA receptors to the ERK pathway, PI3-kinase inhibitorssignificantly reduced both NMDA and high-frequency stimulation(HFS)-induced increases in ERK2 phosphorylation. We found, however,that PI3-kinase inhibitors suppress LTP under conditions in whichblocking ERK activation with MEK (MAP kinase kinase) inhibitorshas no effect. Thus, although PI3-kinase contributes to NMDA receptor-mediatedERK activation, our results demonstrate that the induction ofLTP is also dependent on PI3-kinase signaling through ERK-independentpathways.

  Materials and Methods

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Materials and Methods
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Slice preparation and electrophysiology. Standard techniques were used to prepare slices (400 µm thick) from the hippocampusof halothane-anesthetized C57BL/6 mice (male, 5-8 weeks old).Slices were maintained in interface-type chambers (Fine ScienceTools, Foster City, CA) that were continuously perfused (at 2-3ml/min) with a warm (30°C), oxygenated (95% O₂-5% CO₂) artificialCSF (ACSF) containing the following (in mM): 124 NaCl, 4.4 KCl,25 Na₂HCO₃, 1 NaH₂PO₄, 1.2 MgSO₄, 2 CaCl₂, and 10 glucose. Inour initial experiments, field EPSPs (fEPSPs) were recorded inslices maintained in an interface-type recording chamber, whereasin later experiments, extracellular recordings were done usingslices completely submerged in ACSF. The type of recording configuration,which is noted in the figure legends, had no apparent affect onourobservations.

Standard extracellular recording techniques were used to record fEPSPs in the CA1 region of hippocampal slices (for review,see Thomas et al., 1998; Watabe et al., 2000). Presynaptic fiberstimulation pulses were delivered at 0.02 Hz using a stimulationstrength that evoked fEPSPs that were approximately half of themaximal fEPSP amplitude that could be evoked by strong intensitystimulation. LTP was induced using short-duration trains of thetapulse stimulation (TPS) (150 pulses of presynaptic stimulationdelivered at 5 Hz), long-duration trains of TPS (900 pulses) deliveredin the presence of the $beta$ -adrenergic receptor agonist isoproterenol(ISO) (1 µM), or two trains of HFS (100 pulses of 100 Hz stimulation;intertrain interval of 10 sec). The average of fEPSP slopes recordedbetween 40 and 45 min after TPS or between 55 and 60 min afterHFS were used for statisticalcomparisons.

Whole-cell current-clamp recordings were used to examine the effects of various inhibitors on LTP induced by pairing low-frequencypresynaptic fiber stimulation with postsynaptic depolarization.In these experiments, slices were bathed in a modified ACSF inwhich the concentrations of CaCl₂ and MgSO₄ were increased to4 mM each, the concentration of KCl was reduced to 2.2 mM, andpicrotoxin (100 µM) was added to block GABA_A-mediated inhibitorypostsynaptic potentials. The CA3 region of the slices was removedto prevent spontaneous bursting. Low-resistance (5-10 M $Omega$ ) patch-clampelectrodes filled with a solution containing 122.5 mM Cs-gluconate,17.5 mM CsCl, 10 mM tetraethylammonium (TEA)-Cl, 0.2 mM EGTA,10 mM HEPES, 2 mM Mg-ATP, and 0.3 mM GTP, pH 7.2, were used torecord EPSPs evoked by 0.05 Hz presynaptic fiber stimulation.Current was injected into the cells throughout the experimentto hyperpolarize membrane potentials to between $-$ 80 and $-$ 90 mVand thus minimize action potential generation by potentiated EPSPs.An additional 50-msec-long, 0.1 nA pulse of hyperpolarizing currentwas injected 150 msec after each evoked EPSP to monitor inputand access resistance. At the start of each experiment, the intensityof presynaptic fiber stimulation was adjusted to evoke EPSPs between5 and 10 mV in amplitude. After a 10 min period of baseline recording,current injected through the recording electrode was used to depolarizethe postsynaptic cell to near 0 mV, and LTP was induced by pairingthis tonic depolarization with 100 presynaptic fiber stimulationpulses delivered at 2 Hz. Pairing was done within 20 min of obtainingwhole-cell recordings to minimize the "wash-out" of LTP that canoccur during whole-cell recordings. Statistical significance ofresults from electrophysiological experiments was assessed usingANOVAs (followed by Bonferroni t tests) or paired and unpairedt tests (two-tailed).

Western immunoblotting. Hippocampal slices were prepared as described above and allowed to recover for at least 2 hr beforean experiment. For each experiment, slices obtained from the sameanimal were placed into four separate interface type chambers(typically three slices were loaded per chamber) and constantlyperfused at 2 ml/min with warm (30°C) ACSF. The slices in onechamber were exposed to ACSF alone and served as untreated controls,whereas the slices in the other three chambers were exposed ACSFcontaining various combinations of agonists and antagonists. Toexamine the effects of NMDA receptor activation on ERK2 activation,we first conducted a series of preliminary experiments in whichwe measured phospho-ERK2 levels in slices exposed to differentconcentrations of NMDA (1-100 µM) for various periods of time(2.5-10 min). A concentration (20 µM) and incubation time (5 min)of NMDA that reliably induced a robust, but submaximal, increasein phospho-ERK2 levels was then used for all subsequent experiments.Similar preliminary experiments were also performed to find anappropriate dose (1.0 µM) and incubation time (5 min) for activationof ERK2 by the $beta$ -adrenergic receptor agonist ISO. After drug treatments,the slices were rapidly frozen on dry ice and stored for up to1 week at $-$ 80°C.

CA1 "mini-slices" containing just the CA1 region of the hippocampus were used to examine changes in ERK activation inducedby high-frequency synaptic stimulation. In these experiments,the CA3, dentate gyrus, and subiculuar regions of freshly cuthippocampal slices were removed to produce isolated CA1 regions.After a 2 hr recovery period, we determined the health of eachmini-slice by examining postsynaptic responses evoked by low-frequencypresynaptic stimulation pulses delivered by a stimulating electrodeplaced in stratum radiatum. Slices that showed evidence of epileptiformactivity (evoked and/or spontaneous bursting) were discarded.Three mini-slices were then each stimulated with two trains ofHFS (100 pulses delivered at 100 Hz; intertrain interval of 10sec) using a stimulation intensity sufficient to evoke a 2-6 mVpopulation spike. These mini-slices were pooled (times after HFSranged from 2.5 to 5 min) and rapidly frozen on dry ice. CA1 mini-slicesthat received low-frequency stimulation alone served ascontrols.

For Western analysis, the slices were homogenized in ice-cold buffer containing 50 mM Tris-HCl, 50 mM NaCl, 10 mM EGTA, 10mM EDTA, 80 µM sodium molybdate, 5 mM sodium pyrophosphate, 1mM sodium orthovanadate, 1 mM phenylmethylsulfonyl fluoride, 0.01%Triton X-100, 4 mM para-nitrophenylphosphate, and Protease InhibitorsComplete (Roche Molecular Biochemicals, Indianapolis, IN). A smallaliquot (2 µl) was removed from each sample for protein determinationusing the Bradford method, and 2× loading buffer was added tothe rest of the sample. Samples were boiled for 3 min and thenloaded (20-40 µg of protein per lane) onto 12% SDS-PAGE gels.After electrophoresis, proteins were transferred onto either nitrocellulose(Protran; Schleicher and Schuell, Keene, NH) or polyvinylidenedifluoride (Immun-Blot; Bio-Rad, Hercules, CA) membranes. Blotswere incubated in a blocking buffer consisting of Tris-bufferedsaline containing 0.05% Tween 20 (TBST) plus either 4% nonfatdry milk or 5% bovine serum albumin for 1 hr and then incubatedovernight (at 4°C) with primary antibodies diluted in blockingbuffer. After this, the blots were washed three times with TBSTand then incubated with the appropriate horseradish peroxidase-conjugatedsecondary antibody (usually at a dilution of 1:2000 in blockingbuffer) for 1-2 hr. Proteins were visualized using enhanced chemiluminescence[ECL Western Blotting Analysis System (Amersham, Arlington Heights,IL) or Immun-Star HRP detection kit (Bio-Rad)]. Images of theblots were acquired using a cooled CCD camera-based image acquisitionsystem (Chemi-Doc; Bio-Rad), and densitometric analysis was performedusing the Quantity One software package (Bio-Rad). Primary antibodiesto phospho-p44/p42 MAPK (Thr202/Tyr204, 1:2000), total p44/p42MAPK (1:1000), phospho-glutamate receptor type 1 (GluR1) (S845,1:1000), phospho-Akt (Thr308, 1:500), and total Akt (1:1000) wereobtained from Cell Signaling Technology (Beverly, MA). A primaryantibody to a neuronal-specific isoform ( $beta$ III) of tubulin (1:5000)was obtained from Upstate Biotechnology (Lake Placid, NY). Tocontrol for potential variations in loading, the optical densityof bands for each protein of interest were first normalized tothe optical density values obtained for tubulin bands in eachlane. These normalized values were then expressed as a percentageof the levels seen in untreated control slices. In some experiments,signals were normalized to actin levels determined using an anti-actinantibody (10 µg/ml) obtained from Chemicon (Temecula, CA). One-wayANOVAs or, when appropriate, Kruskal-Wallis one-way ANOVA on rankswere used to assess statistical significance of Western blot data.In both cases, Student-Newman-Keuls tests were used for multiplepairwisecomparisons.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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PI3-kinase inhibitors suppress NMDA receptor-dependent activation of the MAPK pathway

As shown in Figure 1, phospho-ERK2 levels were increased more than threefold in hippocampal slices exposed to 20 µM NMDA for5 min. Although the increase in phospho-ERK2 levels induced byNMDA was significantly (p < 0.01) smaller in slices pretreatedwith the PI3-kinase inhibitor wortmannin, this increase was surprisinglyrobust (more than twofold) and statistically significant comparedwith basal phospho-ERK2 levels in untreated control slices (p< 0.001). Thus, although PI3-kinase inhibitors completely blockNMDA-induced ERK activation in cultured neurons (Chandler et al.,2001; Perkinton et al., 2002), our results suggest that activationof the ERK pathway by NMDA receptor stimulation is only partiallyPI3-kinase dependent in hippocampal slices from young adult animals.

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Figure 1. NMDA-induced increases in phosphorylated ERK2 are only partially PI3-kinase dependent. A, Average ± SEM results from nine experiments in which slices from the same animal were either left untreated (open bar) or exposed to 20 µM NMDA (5 min), 200 nM wortmannin (Wort) ( $>=$ 40 min), or NMDA plus wortmannin. Phospho-ERK2 levels were significantly increased by NMDA in both control and wortmannin-treated slices (*p < 0.01 compared with untreated controls). The increase in phospho-ERK2 levels induced by NMDA in wortmannin-treated slices (250 ± 25.2% of untreated control slices) was significantly less than that induced by NMDA in slices bathed in ACSF (341 ± 30.4% of untreated control slices; #p < 0.05). Wortmannin did not have a significant effect on basal levels of phospho-ERK2. Total levels of ERK2 were unchanged in slices exposed to wortmannin alone, NMDA alone, or wortmannin plus NMDA (levels were 108 ± 5.5, 116 ± 6.4, and 108.3 ± 8.1% of that seen in untreated control slices, respectively). B, Results from individual experiments summarized in A. The plot shows the NMDA-induced increase in phospho-ERK2 levels in slices bathed in ACSF (control) versus ACSF plus 200 nM wortmannin (filled symbols) or 5 µM wortmannin (open symbols). C, Wortmannin inhibits NMDA-induced increases in phospho-Akt in hippocampal slices. Average ± SEM results from nine experiments. In the absence of wortmannin, NMDA (20 µM, 5 min) increased phospho-Akt levels to 214 ± 58% of baseline (*p < 0.05 compared with untreated control). Wortmannin reduced basal levels of phospho-Akt to 15.4 ± 6.2% of control (p < 0.05 compared with untreated controls) and completely blocked NMDA-induced increases in phospho-Akt (phospho-Akt levels were 9.3 ± 2% of control in wortmannin-treated slices exposed to NMDA). D, Representative immunoblots showing the effects of wortmannin on levels of phospho-ERK1/2 and phospho-Akt (Thr308) in untreated (UT) and NMDA treated (N) slices.

One possible explanation for the modest effect of wortmannin on NMDA-induced ERK activation observed in our experiments isthat PI3-kinase activity was not adequately inhibited by the wortmanninconcentration and/or incubation time ( $>=$ 40 min) used in our experiments.To address this possibility, we performed two additional, controlexperiments. Activation and phosphorylation of the protein kinaseAkt is typically PI3-kinase dependent (Toker, 2000), and changesin levels of Akt phosphorylated at S473 or Thr308 can been usedas a convenient assay of PI3-kinase activity (Lin et al., 2001;Sanna et al., 2002). We thus used an antibody that specificallyrecognizes Thr308 phosphorylated Akt to measure levels of activatedAkt in slices treated with NMDA and/or wortmannin. As shown inFigure 1, C and D, phospho-Akt was readily detected in untreatedcontrol slices, and levels were increased approximately twofoldin NMDA-treated slices. Wortmannin (200 nM, 40 min) strongly reducedbasal levels of phospho-Akt and completely prevented the increasein Akt phosphorylation induced by NMDA. This indicates that 200nM wortmannin effectively inhibits PI3-kinase in hippocampal slices.As an additional control, we also examined whether incubatingslices in ACSF containing a 25-fold higher concentration of wortmannin(5 µM) might produce a more robust inhibition of NMDA-inducedERK2 activation. As shown by the open symbols in Figure 1B, increasingthe wortmannin concentration to 5 µM did not produce a strongerinhibition of NMDA-induced MAPK activation. In these experiments,phospho-ERK2 levels were increased to 350 ± 36% of control inslices exposed to NMDA alone and were increased to 227 ± 43% ofcontrol in slices exposed to NMDA in the presence of 5 µM wortmannin(n =3).

Although these results indicate that activation of ERK2 by NMDA receptor stimulation is partially PI3-kinase dependent inhippocampal slices from adult animals, bath-applied NMDA willactivate both synaptic and extrasynaptic receptors. Because thesetwo pools of NMDA receptors can couple to distinct signaling pathways(Hardingham et al., 2002), we also examined whether PI3-kinaseinhibitors suppress activation of ERK2 by patterns of synapticstimulation that activate synaptic NMDA receptors and induce NMDAreceptor-dependent LTP. In addition, we used isolated CA1 mini-slicesin these experiments to lessen the possibility that our biochemicalresults might be confounded by regional differences in the typesof signaling pathways that couple NMDA receptors to the ERK pathway.In control experiments (normal ACSF), HFS reliably induced a statisticallysignificant (p < 0.05) increase in levels of phospho-ERK2 withno effect on total ERK2 levels (Fig. 2). In contrast, HFS in wortmannin-treatedslices failed to induce a statistically significant increase inphospho-ERK2 levels compared with unstimulated control slices(Fig. 2). These results indicate that activation of ERK pathwayby LTP-inducing patterns of synaptic stimulation in the hippocampalCA1 region is strongly dependent on PI3-kinase activity.

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Figure 2. Blocking PI3-kinase with wortmannin inhibits HFS-induced ERK2 activation. A, Western immunoblots showing the effect of HFS delivered in the presence and absence of wortmannin (Wort) on phospho-ERK1/2 and total ERK1/2 levels in CA1 mini-slices. Lane 1, Untreated control (ACSF alone, no HFS); lane 2, HFS in ACSF; lane 3, 200 nM wortmannin alone; lane 4, HFS in wortmannin. Note that, although HFS delivered to slices bathed in normal ACSF induced a robust increase in phospho-ERK2 levels, it had little effect on phospho-ERK2 levels in wortmannin-treated slices. B, C, Average ± SEM results from seven experiments showing basal and stimulated (2.5-5 min after HFS) levels of phospho-ERK2 (B) and total ERK2 (C) in slices bathed in normal ACSF or ACSF containing 200 nM wortmannin. High-frequency stimulation delivered to slices bathed in ACSF increased phospho-ERK2 levels to 182 ± 19% of unstimulated controls (*p < 0.05 compared with unstimulated controls). High-frequency stimulation-induced ERK activation was significantly reduced in wortmannin-treated slices (levels were 125 ± 16% of unstimulated controls; #p < 0.05 compared with HFS in ACSF) and not significantly different from levels of phospho-ERK2 in unstimulated slices bathed in ACSF alone or ACSF plus wortmannin. None of the treatments had any effect on total ERK2 levels.

PI3-kinase inhibitors suppress ERK-dependent forms of LTP

To examine whether PI3-kinase and ERK signaling might have distinct roles in NMDA receptor-dependent forms of synaptic plasticity,we compared the effects of MEK and PI3-kinase inhibitors on LTPinduced by different patterns of synaptic stimulation. In theCA1 region of mouse hippocampal slices, the induction of LTP bya short train (150 pulses) of TPS alone or by a longer train (900pulses) of TPS delivered in the presence of the $beta$ -adrenergic receptoragonist ISO is especially sensitive to inhibitors of ERK activation(Winder et al., 1999; Watabe et al., 2000). Thus, to examine whetherPI3-kinase is required for the induction and/or maintenance ofERK-dependent forms of LTP, we first investigated whether PI3-kinaseinhibitors suppressed the amount of potentiation induced by theseTPSprotocols.

As shown in Figure 3A, the PI3-kinase inhibitor LY294002 strongly suppressed LTP induced by a 150 pulse train of TPS. In controlexperiments, fEPSPs were potentiated to 167.9 ± 9.5% of baselineafter TPS (n = 6), whereas fEPSPs were just 109.1 ± 5.9% of baselineafter TPS in slices continuously bathed in ACSF containing 20µM LY294002 (n = 6). The inhibition of LTP by LY294002 is mostlikely not attributable to direct effects on NMDA receptors becauseprevious studies have found that LY294002 and wortmannin do notinhibit NMDA receptor-mediated responses in hippocampal neurons(Shanley et al., 2001; Sanna et al., 2002). Moreover, at thisconcentration, LY294002 had no obvious effect on basal synaptictransmission (data not shown) or on synaptic transmission duringthe TPS train (Fig. 3B). LY294002 also had no effect on the numberof EPSP-evoked complex spike bursts that were evoked during theTPS train [complex spike bursts were elicited by 77.3 ± 2.7% ofthe EPSPs during the TPS train in control slices (n = 6) and by77.2 ± 1.6% of the EPSPs during the TPS train in LY294002-treatedslices (n = 6)]. This indicates that LY294002 does not inhibitLTP induction through indirect effects on postsynaptic excitability(Thomas et al., 1998). As described below (see Fig. 9), TPS-inducedLTP was also inhibited by wortmannin (200 nM).

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Figure 3. The PI3-kinase inhibitor LY294002 suppresses TPS-induced LTP. A, A 150 pulse train of TPS delivered at time 0 induced LTP in vehicle control experiments (0.1% DMSO; open symbols; n = 6) but had little lasting effect on synaptic transmission in slices treated with 20 µM LY294002 for at least 40 min before TPS (filled symbols; n = 6). LY294002 was present throughout the experiment. Inset shows fEPSPs recorded during baseline and 45 min after TPS in a control slice (left set of traces) and in a slice bathed in LY294002 (right set of traces). Calibration: 2 mV, 5 msec. B, LY294002 has no effect on synaptic responses evoked during TPS. Note that both the facilitation at the start of TPS and the depression of synaptic transmission at the end of the TPS train are similar in control (open symbols) and LY294002-treated slices (filled symbols). On average, fEPSPs elicited by pulse 2 to pulse 6 of the TPS train facilitated to 147.6 ± 6.1% of baseline in control experiments and were facilitated to 145.8 ± 4.8% of baseline in LY294002-treated slices (not significantly different; p = 0.82). In control experiments, fEPSPs were depressed to 37.1 ± 6.2% of baseline at the end of the TPS train (average of the last 5 stimulation pulses) and were depressed to 45.2 ± 5.8% of baseline in LY294002-treated slices (not significantly different; p = 0.363). Recordings were done using slices maintained in an interface chamber.

Although the induction of LTP by a short, 150-pulse-long train of TPS by itself induces LTP, longer trains of TPS (300-900pulses) only induce significant levels of potentiation when combinedwith $beta$ -adrenergic receptor activation (Thomas et al., 1996; Winderet al., 1999). Because the induction of LTP by TPS paired with $beta$ -adrenergic receptor activation is also ERK dependent (Winderet al., 1999), we examined whether PI3-kinase inhibitors inhibitLTP induced by this pattern of synaptic stimulation as well. Asshown in Figure 4, in control experiments (n = 15), fEPSPs werepotentiated to 189.7 ± 7.9% of baseline 45 min after 900 pulsesof TPS delivered at the end of a 10 min application of the $beta$ -adrenergicreceptor agonist ISO. In contrast, TPS in the presence of ISOinduced a significantly smaller potentiation of synaptic transmissionin wortmannin-treated slices (fEPSPs were potentiated to 165.7± 6.8% of baseline; n = 14; p < 0.05 compared with control). Wortmanninalso significantly reduced ISO-induced increases in phospho-ERK2levels in hippocampal slices (Fig. 4B), a finding consistent witha recent report showing that cAMP-induced activation of ERK isPI3-kinase dependent in neurons (Lin et al., 2001). Although bothof these findings are consistent with the hypothesis that PI3-kinaseactivity is required for ERK-dependent forms of plasticity, bothTPS-induced LTP (Thomas et al., 1996) and ISO-induced ERK activationare protein kinase A (PKA) dependent (Roberson et al., 1999).Thus, the inhibition of both ISO-induced ERK2 activation and LTPinduced by TPS in the presence of ISO might be attributable tononselective effects of wortmannin on PKA. We thus examined whether200 nM wortmannin interfered with $beta$ -adrenergic receptor activation-inducedincreases in phosphorylation of the GluR1 subunit of AMPA receptorsat a site phosphorylated by PKA (Ser845). As shown in Figure 4C,the increase in phospho-GluR1 levels induced by ISO was not alteredin wortmannin-treated slices, suggesting that wortmannin doesnot appreciably affect PKA under our experimental conditions.

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Figure 4. PI3-kinase inhibitors suppress the induction of LTP by long trains of TPS paired with $beta$ -adrenergic receptor activation and inhibit ISO-induced ERK2 activation. A, Nine hundred pulses of TPS (delivered at time 0) paired with a 10 min application of 1 µM ISO (indicated by the bar) induced significantly less potentiation in slices continuously bathed in 200 nM wortmannin (filled symbols; n = 14) compared with slices bathed in normal ACSF plus vehicle (0.1% DMSO; open symbols; n = 15). A long train of TPS delivered in the absence of ISO had little lasting effect on synaptic transmission in control and wortmannin-treated slices (data not shown). B, Wortmannin (Wort) inhibits ISO-induced ERK2 activation. Average ± SEM results from five separate experiments in which slices from the same animal were either left untreated (UT; open bar) or exposed to 1 µM ISO (5 min), 200 nM wortmannin ( $>=$ 40 min), or ISO plus wortmannin. In vehicle control experiments (0.01-0.1% DMSO), phospho-ERK2 levels were increased to 250 ± 40.2% of control in ISO-treated slices (*p < 0.05 compared with untreated controls). A significantly smaller increase in phospho-ERK2 levels was induced by ISO in wortmannin-treated slices (phospho-ERK2 levels were increased to 164.1 ± 17.8% of control; #p < 0.05 compared with levels in slices treated with ISO alone). Total levels of ERK2 were unchanged in slices exposed to wortmannin alone, ISO alone, or wortmannin plus ISO (data not shown). The inset shows a representative immunoblot showing basal and ISO-stimulated levels of phospho-ERK2 in slices bathed in ACSF alone and ACSF plus 200 nM wortmannin. C, Wortmannin has no effect on the increase in phospho-S845 GluR1 levels induced by ISO. In slices bathed in ACSF, a 5 min application of 1.0 µM ISO increased phospho-GluR1 levels to 512 ± 69% of control (n = 5). In wortmannin-treated slices, phospho-GluR1 levels were 547.7 ± 90.4% of control. The inset shows a representative immunoblot showing basal and ISO-stimulated levels of phospho-S845 GluR1 in slices bathed in ACSF and ACSF plus wortmannin.

PI3-kinase inhibitors suppress ERK-independent forms of LTP

Previously, we found that the MEK inhibitor SL327 has no effect on the induction of LTP by low-frequency presynaptic fiberstimulation paired with postsynaptic depolarization, suggestingthat the induction of LTP by this stimulation protocol is MAPKindependent (Watabe et al., 2000). If PI3-kinase inhibitors blockLTP solely because they prevent NMDA receptor-mediated ERK activation,then PI3-kinase inhibitors should have no effect on pairing-inducedLTP. We thus examined whether PI3-kinase inhibitors affect pairing-inducedLTP to determine whether ERK-independent forms of LTP are alsoPI3-kinase dependent. To confirm that this stimulation protocolinduces an ERK-independent form of potentiation, we first examinedwhether a different MEK inhibitor, U0126, affects pairing-inducedLTP. As shown in Figure 5B, the amount of potentiation observed30 min after pairing postsynaptic depolarization with low-frequencypresynaptic fiber stimulation in cells recorded from slices bathedin ACSF containing 20 µM U0126 was not significantly differentfrom the potentiation seen in cells recorded from slices bathedin ACSF plus 0.2% DMSO. To confirm that 20 µM U0126 effectivelyblocked NMDA receptor-mediated ERK2 activation under our experimentalconditions, we examined the effects of U0126 on NMDA-induced increasesin ERK2 phosphorylation in hippocampal slices. As shown in Figure5A, U0126 strongly reduced basal levels of phospho-ERK2 and blockedincreases in ERK2 phosphorylation induced by a 5 min bath applicationof 20 µM NMDA. Thus, it seems unlikely that the inability of U0126to block pairing-induced LTP can be attributed to an insufficientlevel of MEK inhibition. In contrast to U0126, pairing-inducedLTP was strongly suppressed in cells in which the PI3-kinase inhibitorLY294002 was present in the recording electrode solution (Fig.5B) (p < 0.001 compared with the potentiation induced in controlcells). The differential sensitivity of pairing-induced LTP toMEK and PI3-kinase inhibitors indicates that the effects of PI3-kinaseinhibitors on LTP are not simply attributable to alterations inERK signaling. Moreover, because LY294002 was selectively deliveredinto the postsynaptic CA1 pyramidal cells, our results suggestthat postsynaptic PI3-kinase activity is especially importantfor LTP.

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Figure 5. Low-frequency presynaptic fiber stimulation paired with postsynaptic depolarization induces an ERK-independent but PI3-kinase inhibitor-sensitive form of LTP. A, The MEK inhibitor U0126 (20 µM) blocks NMDA-induced ERK2 activation. Western immunoblot showing phospho-ERK2 levels (top) and total ERK levels (bottom) in a representative experiment. Lane 1, Untreated control (slices exposed to ACSF alone); lane 2, NMDA (20 µM, 5 min) in ACSF; lane 3, 20 µM U0126 alone ( $>=$ 40 min); lane 4, U0126 plus NMDA. Note that U0126 strongly reduces basal levels of phospho-ERK2 and blocks the increase in ERK2 phosphorylation induced by NMDA. None of the treatments had an affect on total ERK2 levels. The same results were obtained in three separate experiments. B, Pairing-induced LTP is not blocked by U0126 but is inhibited by LY294002. Presynaptic stimulation pulses paired with postsynaptic depolarization to near 0 mV (at time 0) induced nearly identical levels of potentiation in vehicle control experiments (0.1-0.2% DMSO; open circles; EPSPs were potentiated to 267 ± 13% of baseline; n = 13) and in cells recorded from slices continuously bathed in ACSF containing 20 µM U0126 (triangles; EPSPs were potentiated to 275 ± 13% of baseline; n = 9). Significantly less LTP was induced, however, in cells in which LY294002 (100 µM) was included in the electrode filling solution to block postsynaptic PI3-kinase (filled circles; EPSPs were potentiated to 159 ± 22% of baseline; n = 8; p < 0.001 compared with vehicle control cells). The inset shows EPSPs (average of 3 responses) recorded during baseline (smaller responses) and 30 min after pairing. Calibration: 5 mV, 20 msec.

In agreement with previous reports (Winder et al., 1999; Watabe et al., 2000), we also found that MEK inhibitors do not blockHFS-induced LTP in mouse hippocampal slices (Liu et al., 1999).As shown in Figure 6A, the MEK inhibitor SL327 (10 µM) had noeffect on the amount of potentiation present 60 min after HFS,although this concentration of SL327 completely blocked HFS-inducedincreases in levels of phospho-ERK2 in CA1 mini-slices. In contrast,blocking PI3-kinase with either LY294002 (Fig. 6B) or wortmannin(Fig. 7A) strongly inhibited HFS-induced LTP. Thus, PI3-kinaseinhibitorsnot only suppress ERK-dependent forms of LTP but also inhibitLTP induced by patterns of synaptic stimulation (pairing, HFS)that induce an ERK-independent form of LTP. This later findingis difficult to reconcile with the simple notion that PI3-kinaseactivity is required for LTP only because PI3-kinase is an essentiallink between NMDA receptors and ERK activation. Instead, theseobservations indicate that PI3-kinase and ERK signaling have distinctroles in NMDA receptor-dependent LTP.

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Figure 6. HFS-induced LTP is not blocked by MEK inhibitor SL327 but is suppressed by PI3-kinase inhibitors. A, Concentrations of the MEK inhibitor SL327 that block HFS-induced ERK2 activation have no effect on HFS-induced LTP. In experiments done in interface slice chambers, the amount of potentiation present 60 min after HFS (delivered at time 0) is the same in control and SL327-treated slices. In control experiments (open symbols; 0.1% DMSO), fEPSPs were potentiated to 173 ± 12% of baseline 60 min after HFS (n = 6) and were potentiated to 182 ± 12% of baseline in slices continuously bathed in 10 µM SL327 (filled symbols; n = 6). The inset shows example immunoblots probed with antibodies specific for phospho-ERK1/2 (top) and total ERK1/2 (bottom). Lane 1, Untreated control (ACSF alone); lane 2, HFS in ACSF; lane 3, SL327 alone ( $>=$ 40 min); lane 4, HFS in SL327. Note that SL327 strongly reduced both basal levels of phospho-ERK2 and the increase in ERK2 phosphorylation induced by HFS. None of the treatments affected total ERK2 levels. The same results were obtained in three separate experiments. B, Inhibiting PI3-kinase activity with LY294002 significantly reduces HFS-induced LTP. In vehicle control experiments (0.1% DMSO; open symbols), fEPSPs were potentiated to 185 ± 16% of baseline 60 min after HFS; n = 6). In contrast, fEPSPs were potentiated to 138 ± 6% of baseline 60 min after HFS in slices continuously bathed in 20 µM LY294002 (filled symbols; n = 6; p < 0.05 compared with control). The inset shows fEPSPs recorded during baseline and 60 min after HFS (larger responses) in a control slice (left set of traces) and in a slice bathed in ACSF containing LY294002 (right set of traces). Calibration: 2 mV, 5 msec. Experiments were done using interface slice recording chambers.

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Figure 7. PI3-kinase inhibitors suppress the induction but not the maintenance and expression of LTP. A, Wortmannin (Wort) inhibits HFS-induced LTP in submerged slices. Slices were continuously bathed in ACSF containing 0.02% DMSO (vehicle control; open symbols; n = 10) or ACSF containing 200 nM wortmannin (filled symbols; n = 10). One hour after HFS, fEPSPs were potentiated to 174 ± 11% of baseline in control slices but increased to only 132 ± 9% of baseline in wortmannin-treated slices (p < 0.01 compared with control). B, PI3-kinase (PI3K) inhibitors have no effect on established LTP. Wortmannin (200 nM; n = 3) or LY294002 (10 µM; n = 4) were applied starting 30 min after HFS (duration of inhibitors in the bath indicated by the bar). Neither wortmannin nor LY294002 inhibited potentiated synaptic transmission, and the results from all experiments were combined. All experiments were done using a submerged-slice recording chamber.

PI3-kinase inhibitors suppress LTP induction

Because continuous applications of PI3-kinase inhibitors were used in the experiments described above, the inhibition of LTPproduced by wortmannin and LY294002 could be attributable to effectson the induction, maintenance, and/or expression of LTP. To examinewhether PI3-kinase activity is specifically required for the maintenanceand/or expression of LTP, we first induced LTP by delivering HFSin the absence of PI3-kinase inhibitors and then applied eitherLY294002 (20 µM; n = 4) or wortmannin (200 nM; n = 3) for 30 minstarting 30 min after HFS. As shown in Figure 7B, blocking PI3-kinaseafter LTP induction had no effect on potentiated synaptic transmission.In three additional experiments, we extended the duration of thewortmannin application to at least 60 min and still observed noeffect on potentiated synaptic transmission (data not shown).Wortmannin and LY294002 must therefore be present during HFS toinhibit LTP. This suggests that PI3-kinase activity has an importantrole in the induction of LTP but not its maintenance or expression.In contrast, a recent report found that PI3-kinase is activatedfor up to 30 min after LTP induction and that PI3-kinase inhibitorsapplied after HFS produce a reversible inhibition of potentiatedEPSPs, suggesting that PI3-kinase activity is specifically requiredfor the expression and not the induction or maintenance of LTP(Sanna et al., 2002). Notably, the concentrations of LY294002and wortmannin used by Sanna et al. in their experiments (100and 5 µM, respectively) were much higher than those used in ourexperiments (20 µM and 200 nM). We thus reexamined the effectsof PI3-kinase inhibitors on the maintenance and expression ofLTP using these higher inhibitor concentrations. As shown in Figure8, potentiated synaptic transmission was depressed when either100 µM LY294002 or 5 µM wortmannin was applied starting 30 minafter LTP was induced with HFS. Whereas Sanna et al. (2002) reportedthat these high concentrations of LY294002 and wortmannin hadno effect on unpotentiated synaptic transmission, under our experimentalconditions, 100 µM LY294002 and 5 µM wortmannin also depressedtransmission at unpotentiated synapses (Fig. 8). Although thereason for this difference is unclear, our results suggest thatthe inhibition of potentiated synaptic transmission by high concentrationsof PI3-kinase inhibitors is not attributable to a selective disruptionof mechanisms involved in the expression or maintenance of LTP.

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Figure 8. High concentrations of PI3-kinase inhibitors depress potentiated synaptic transmission but also inhibit transmission at unpotentiated synapses. A, Potentiated synaptic transmission is inhibited by a high concentration of LY294002 (100 µM) applied for 30 min starting 30 min after LTP induction (n = 5; presence of LY294002 in the recording chamber indicated by the bar). At this concentration, LY294002 also inhibited basal synaptic transmission in a separate series of experiments (open symbols; n = 5). B, A 30 min application of a high concentration of wortmannin (5 µM; Wort) also inhibited both potentiated (filled symbols; n = 5) and basal synaptic transmission (open symbols; n = 4). The bar indicates presence of wortmannin in the recording chamber. All experiments were done using a submerged-slice recoding chamber.

TPS-induced LTP is ERK independent but PI3-kinase dependent in the hippocampus of PSD-95 mutant mice

Recent studies have shown that NMDA receptors form large multiprotein complexes that contain a number of proteins involvedin Ras signaling (Husi et al., 2000). PI3-kinase (p85 regulatorysubunit) directly binds to the NR2B subunit of NMDA receptorsvia an interaction mediated by the SH2 (Src homology 2) domainof p85 binding a tyrosine site on NR2B (Hisatsune et al., 1999).This site is phosphorylated by Fyn tyrosine kinase (Hisatsuneet al., 1999), which is required for LTP induction (Grant et al.,1992). In contrast to the direct interaction of PI3-kinase withNR2B, MEK and ERK are regulated by SynGAP, a Ras GTPase-activatingprotein that directly binds PSD-95 (postsynaptic density-95) (Chenet al., 1998; Kim et al., 1998), which in turn binds to NR2 subunits(Kornau et al., 1995). PI3-kinase and ERK are thus linked to theNMDA receptor via distinct protein interactions. Because our pharmacologicaland biochemical studies indicate that PI3-kinase and MAPK havedistinct roles in LTP, we wondered whether alterations in thecomposition of NMDA receptor complexes could differentially influencethe involvement of these signaling pathways in LTP. To begin toaddress this question, we examined the effects of MEK and PI3-kinaseinhibitors on LTP in the hippocampus of mice with a mutation thatdisrupts PSD-95 (Migaud et al., 1998). As shown in Figure 9A,the induction of LTP by 150 pulses of TPS was significantly inhibitedby both U0126 and wortmannin in slices from wild-type mice. Asexpected from previous work (Migaud et al., 1998; Komiyama etal., 2002), TPS induced a larger potentiation of synaptic transmissionin slices from PSD-95 mutant mice. Surprisingly, U0126 did notinhibit TPS-induced LTP in slices from PSD-95 mutants (Fig. 9B),suggesting that ERK activation may no longer be required for TPS-inducedLTP in the absence of PSD-95. Although the mechanistic basis responsiblefor this change in ERK dependency is unknown, this aspect of thePSD-95 mutant phenotype provides an additional way to examinethe relationship between PI3-kinase and ERK in LTP. Specifically,if a serial pathway with PI3-kinase positioned upstream of ERKactivation could account for the role of PI3-kinase in LTP, thenthe induction of LTP by TPS in slices from PSD-95 mutant miceshould also be PI3-kinase independent. We observed, however, thatwortmannin still significantly reduced TPS-induced LTP in slicesfrom PSD-95 mutant mice (Fig. 9B). Thus, whereas the absence ofPSD-95 dramatically alters the involvement of ERK in TPS-inducedLTP, the induction of LTP by this protocol remains partially dependenton PI3-kinase activity. The differential effects of PI3-kinaseand MAPK inhibitors on TPS-induced LTP in hippocampal slices fromPSD-95 mutant mice thus provides additional evidence that theeffects of PI3-kinase inhibitors on LTP cannot be solely attributedto alterations in ERK signaling.

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Figure 9. TPS-induced LTP is ERK independent but still PI3-kinase dependent in hippocampal slices from PSD-95 mutant mice. A, Both MEK and PI3-kinase inhibitors suppress the induction of LTP by a 150 pulse train of TPS in slices from wild-type animals. In vehicle control experiments (0.1- 0.2% DMSO; open circles), fEPSPs were potentiated to 205 ± 7% of baseline 45 min after TPS (n = 9). The amount of potentiation induced by TPS was significantly reduced (p < 0.001) in slices continuously bathed in ACSF containing either 200 nM wortmannin (Wort; filled circles; fEPSPs were 125 ± 11% of baseline; n = 6) or 20 µM U0126 (filled triangles; fEPSPs were 137 ± 9% of baseline; n = 11). B, The amount of LTP induced by a 150 pulse train of TPS was not reduced by U0126 in slices from PSD-95 mutant mice. In vehicle control experiments, fEPSPs were potentiated to 279 ± 15% of baseline (open circles; n = 14) and were potentiated to 270 ± 12% of baseline (n = 14) in slices continuously bathed in ACSF containing U0126 (triangles). LTP induced by TPS in PSD-95 mutant slices was inhibited by wortmannin. In slices from PSD-95 mutant mice that were continuously bathed in 200 nM wortmannin, fEPSPs were potentiated to 195 ± 13% of baseline (filled circles; n = 7; p < 0.05 compared with control levels of LTP in PSD-95 mutant slices). All experiments were done in an interface-type recording chamber.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Inhibitors of PI3-kinase not only suppress hippocampal LTP (Kelly and Lynch, 2000; Raymond et al., 2002; Sanna et al., 2002)but also inhibit NMDA receptor-mediated ERK activation (Chandleret al., 2001; Perkinton et al., 2002). This suggests that PI3-kinaseactivity is required for LTP induction because it provides anessential link between NMDA receptors and ERK. In our experiments,wortmannin significantly reduced, but did not block, NMDA-inducedERK activation, suggesting that NMDA receptor-mediated ERK activationis only partially PI3-kinase dependent in the hippocampus of youngadult animals. Activation of ERK2 by HFS was strongly suppressedby wortmannin, however, suggesting that PI3-kinase may be particularlyimportant for activation of the ERK pathway by LTP-inducing patternsof synaptic activity. Although these findings are consistent withthe hypothesis that PI3-kinase blockers inhibit LTP by antagonizingNMDA receptor-dependent ERK activation, we found that PI3-kinaseand MEK inhibitors have distinct effects on LTP. Although blockingERK activation inhibited LTP induced by two different TPS protocols,it had no effect on LTP induced by HFS or low-frequency synapticstimulation paired with postsynaptic depolarization. In contrast,PI3-kinase inhibitors suppressed the induction of LTP by all fourprotocols. In addition, the effects of MEK, but not PI3-kinase,inhibitors on TPS-induced LTP were dramatically altered in PSD-95mutant mice. The role of PI3-kinase in LTP is thus not limitedto its role as an upstream regulator of ERKsignaling.

The role of MAPK in the induction of LTP

Although our experiments primarily focused on the role of PI3-kinase in LTP, our findings have important implications regardingthe role of ERK in LTP. In our experiments, both pairing and HFS-inducedLTP were unaffected by two different MEK inhibitors, indicatingthat ERK activation is not absolutely required for LTP (Winderet al., 1999; Watabe et al., 2000). In addition, previous studieshave shown that ERK activation by itself is not sufficient forLTP induction (Winder et al., 1999; Dudek and Fields, 2001). Thus,ERK activation is not an essential signaling event required forthe early phases of NMDA receptor-dependent LTP in the hippocampalCA1 region. This does not mean that ERK activity is not importantlyinvolved in LTP. Indeed, numerous studies have shown that hippocampalLTP is inhibited by MEK inhibitors (English and Sweatt, 1997;Atkins et al., 1998; Coogan et al., 1999; Winder et al., 1999;Watabe et al., 2000; Giovannini et al., 2001). Moreover, as weshow here, the induction of LTP by 150 pulse trains of TPS isstrongly reduced by MEK inhibitors (Winder et al., 1999; Watabeet al., 2000). Thus, although ERK activation may not be requiredfor the induction of LTP by all patterns of synaptic stimulation,or under all experimental conditions, it clearly represents animportant modulator of LTP. In addition to modulating LTP induction,ERK activation is also thought to have an important role in transcriptionalevents involved in the later, mRNA synthesis and protein synthesis-dependentstages of LTP (Impey et al., 1998; Davis et al., 2000).

Recently, two different models have been proposed to account for the role of ERK signaling in the induction of LTP (Sweatt,2001; Zhu et al., 2002). In one model (Sweatt, 2001), ERK activationcontributes to LTP induction by facilitating activation of synapticNMDA receptors through a downregulation of dendritic A-type K⁺ channels (Adams et al., 2000; Watanabe et al., 2002; Yuan etal., 2002). In the second model (Zhu et al., 2002), ERK activationhas a more central role in LTP induction and is required for activity-dependentmembrane insertion of AMPA receptors. Our observations supportthe first of these models. First, we found that MEK inhibitorshave no effect on pairing-induced LTP in experiments in whichpostsynaptic K⁺ channels were blocked by the inclusion of Cs⁺ and TEA in the recording electrode solution. Thus, as would beexpected if ERK activation normally contributes to LTP inductionby downregulating K_A channels, bypassing ERK and directly inhibitingthese channels pharmacologically obviates the need for ERK activationand renders LTP insensitive to the effects of MEK inhibitors.Second, our observation that MEK inhibitors do not block HFS (orpairing-induced LTP) is incompatible with a model in which ERKactivation is an essential step in LTP. What is less clear, however,is how the first model can explain the lack of effect of MEK inhibitorson HFS-induced LTP. One possibility is that, under our experimentalconditions, the postsynaptic depolarization evoked by HFS is largeenough to strongly activate NMDA receptors and induce LTP evenin the absence of an ERK-mediated downregulation of K_Achannels.

The role of PI 3-kinase in LTP

Although LY294002 and wortmannin almost completely blocked LTP induced by a short train of TPS, HFS and presynaptic stimulationpaired with postsynaptic depolarization still induced a significant,albeit smaller, potentiation of synaptic transmission in slicespretreated with these inhibitors. One trivial explanation forthis incomplete block of LTP is that PI3-kinase activity was notsufficiently inhibited by the concentrations of wortmannin andLY294002 used in our experiments. This seems unlikely, however,because the concentrations of wortmannin (Fig. 1) and LY294002(data not shown) used in our experiments completely blocked NMDA-inducedincreases in phospho-Akt levels. Thus, the partial inhibitionof LTP by PI3-kinase inhibitors most likely indicates that PI3-kinaseactivity is not absolutely required for the early stages of LTPup to 1 hr after induction. Instead, like ERK, PI3-kinase maybe part of an important modulatory pathway that normally enhancesthe amount of potentiation induced by some patterns of synapticstimulation. Alternatively, some patterns of synaptic stimulationmay induce two distinct forms of potentiation, one that is dependenton PI3-kinase signaling and another that arises from PI3-kinase-independentmechanisms. The results from our experiments do not distinguishbetween these two possibilities. In either scenario, however,it seems likely the PI3-kinase activity contributes to the inductionof LTP rather than its maintenance or expression because PI3-kinaseinhibitors applied after LTP induction do not blockLTP.

In contrast to our findings, it has been reported that PI3-kinase inhibitors applied after LTP induction can produce a selectiveand reversible depression of transmission at potentiated synapses(Sanna et al., 2002), suggesting that the expression of LTP isdependent on persistent PI3-kinase activity. Although we foundthat potentiated synaptic transmission was depressed by the muchhigher concentrations of LY294002 and wortmannin used by Sannaet al. (2002), under our experimental conditions, these high concentrationsof the inhibitors also depressed transmission at basal, nonpotentiatedsynapses. The reason for the difference between our observationsand those of Sanna et al. (2002) with respect to the effects ofhigh PI3-kinase inhibitor concentrations on basal synaptic transmissionis unclear but might be attributable to species differences (ratvs mouse). It is important to note, however, that the lower concentrationsof PI3-kinase inhibitors used in our experiments strongly blockedPI3-kinase activity in our slices (as measured by changes in phospho-Aktlevels) yet had no effect on transmission at potentiatedsynapses.

How might PI3-kinase be involved in the induction of LTP? In many cell types, PI3-kinase activates atypical isoforms of proteinkinase C (PKC) via activation of phosphoinositide-dependent kinase-1,a protein kinase activated by the phospholipid products generatedby PI3-kinase (Chou et al., 1998; Le Good et al., 1998). The atypicalPKC isoform PKC $zeta$ is activated by LTP-inducing patterns of synapticstimulation (Sacktor et al., 1993), and inhibitors that selectivelyblock PKC $zeta$ inhibit LTP in the hippocampal CA1 region (Ling etal., 2002). Moreover, introduction of activated PKC $zeta$ into CA1pyramidal cells induces a robust potentiation of synaptic transmissionthat occludes HFS-induced LTP (Ling et al., 2002). Thus, one possibilityis that PI3-kinase contributes to the initial activation of PKC $zeta$ during LTP induction. PI3-kinase is also involved in the traffickingand insertion of some membrane proteins (Corvera and Czech, 1998;Wu et al., 1998; Rameh and Cantley, 1999; Lhuillier and Dryer,2002), including AMPA-type glutamate receptors containing GluR1subunits (Passafaro et al., 2001). Thus another possibility isthat PI3-kinase is involved in activity-dependent changes in AMPAreceptor trafficking-insertion that are thought to underlie LTP(for review, see Malinow and Malenka, 2002). With regard to thispossibility, it is interesting to note that wortmannin completelyblocks membrane insertion of GluR1-containing AMPA receptors inducedby NMDA receptor activation in cultured neurons (Passafaro etal., 2001) but only partially inhibits LTP in hippocampal slices.Finally, PI3-kinase signaling can regulate organization of theactin cytoskeleton through activation of GTP exchange factorsthat regulate members of the Rho family of GTPases (Cantrell,2001; Rodgers and Theibert, 2002). PI3-kinase signaling mightthus have an important role in changes in dendritic spine structureinduced by activation of synaptic NMDA receptors (for review,see Yuste and Bonhoeffer, 2001). Although the downstream mechanismsunderlying the role of PI3-kinase in LTP remain unknown, our resultssuggest that Ras activation engages a divergent network of multipledownstream signaling events that have distinct regulatory rolesinLTP.

  FOOTNOTES

Received Dec. 10, 2002; revised Feb. 20, 2003; accepted Feb. 24, 2003.

This work was supported by a grant from the National Institute of Mental Health (T.J.O.) and the Wellcome Trust (S.G.N.G.).We thank Jane Robinson and Lynsey Forsyth for animal husbandryand genotyping and Rex Parker and Oahn Ho for technical assistance.SL327 was a generous gift from J. M. Trzaskos (DuPont PharmaceuticalsResearch Laboratories, Wilmington,DE).

Correspondence should be addressed to Thomas J. O'Dell, Department of Physiology, David Geffen School of Medicine at Universityof California at Los Angeles, 53-231 Center for Health Science,Box 951751, Los Angeles, CA 90095. E-mail: todell{at}mednet.ucla.edu.

A. M. Watabe's present address: Division of Neuronal Network, Department of Basic Medical Sciences, The Institute of MedicalScience, The University of Tokyo, Tokyo 108-8639,Japan.

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