Activation of Presynaptic P2X7-Like Receptors Depresses Mossy Fiber-CA3 Synaptic Transmission through p38 Mitogen-Activated Protein Kinase

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The Journal of Neuroscience, July 15, 2002, 22(14):5938-5945

Activation of Presynaptic P2X₇-Like Receptors Depresses Mossy Fiber-CA3 Synaptic Transmission through p38 Mitogen-Activated Protein Kinase
John N. Armstrong, Tyson B. Brust, Randall G. Lewis, and Brian A. MacVicar
Neuroscience Research Group, Department of Physiology and Biophysics, Faculty of Medicine, University of Calgary, Calgary, Alberta, T2N 4N1 Canada

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

P2X₇ receptor subunits form homomeric ATP-gated, calcium-permeable cation channels. In this study, we used Western blots andimmunocytochemistry to demonstrate that P2X₇ receptors are abundanton presynaptic terminals of mossy fiber synapses in the rat hippocampus.P2X₇-immunoreactive protein was detected using a specific P2X₇antibody in Western blots of protein isolated from whole hippocampusand from a subcellular fraction containing mossy fiber synaptosomes.P2X₇ immunoreactivity was colocalized with syntaxin 1A/B-immunoreactivityin mossy fiber terminals in the dentate hilus and stratum lucidumof CA3. Extracellular and whole-cell voltage-clamp recordingsin CA3 revealed that bath application of the potent P2X₇ agonist2',3'-O-(4-benzoylbenzoyl)-ATP (Bz-ATP) caused a long-lastinginhibition of neurotransmission at mossy fiber-CA3 synapses. Consistentwith a presynaptic action at mossy fiber synapses, Bz-ATP hadno significant effect on neurotransmission at associational-commissuralsynapses in CA3 but increased paired-pulse facilitation duringdepression of mossy fiber evoked currents. In addition, Bz-ATPhad no postsynaptic effect on holding current or conductance ofCA3 neurons. Bz-ATP-induced mossy fiber synaptic depression wasblocked by the P2X₇ antagonist oxidized ATP but not by the P2X_1-3,5,6antagonist pyridoxalphosphate-6-azophenyl-2',4'-disulfonic acidor the P2Y antagonist reactive blue 2. Finally, an antagonistof p38 MAP kinase activation [4-(4-fluorophenyl)2-(4-methylsulfinylphenyl)5-(4-pyridyl)imidazole]but not extracellular signal-regulated kinase 1/2 MAP kinase (2'-amino-3'-methoxyflavone)blocked the synaptic depression mediated by Bz-ATP, suggestingthat this presynaptic inhibition was mediated by activation ofp38 MAP kinase. The results of the present study demonstrate thatactivation of presynaptic P2X₇ receptors depresses mossy fiber-CA3synaptic transmission through activation of p38 MAPkinase.

Key words: plasticity; glutamate; hippocampus; ATP; purinergic receptor; synaptic depression; hippocampus

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

ATP is released from synapses throughout the peripheral nervous system and CNS (White, 1977, 1978; Jahr and Jessell, 1983;Edwards et al., 1992; Edwards and Gibb, 1993), where it can acton P2X receptors to modulate neurotransmission. P2X receptorsare ligand-gated, calcium-permeable cation channels (Khakh, 2001)that are activated by extracellular ATP. There are seven knownP2X receptor subunits, P2X_1-7. Of the seven subunits, onlyP2X₇ subunits are thought to function exclusively as homomericreceptors (North and Surprenant, 2000). Activation of P2X₇ receptorscan lead to the initiation of signaling cascades through secondmessengers, such as phospholipase D (Kusner and Adams, 2000),p38 MAP kinase (Hu et al., 1998; Hide et al., 2000; Panenka etal., 2001), or the transcription factor nuclear factor- $kappa$ B (Ferrariet al., 1997). Recent data suggest that the initiation of thesesignaling cascades could be mediated through putative proteininteractions with the long cytoplasmic C terminus of the P2X₇subunit (Denlinger et al., 2001; Kim et al., 2001). In some circumstances,the pore formed by the P2X₇ receptor may allow permeation of largecations (North and Barnard, 1997; North and Surprenant, 2000)that may eventually lead to cytolysis (Di Virgilio, 1995; Baricordiet al., 1999; Mutini et al., 1999).

P2X₇ receptors are only activated by high extracellular concentrations of ATP. Low concentrations (nanomolar) of ATP thatare ineffective at activating P2X₇ receptors are known to increaseneuronal excitation and synaptic activity in the nervous system.For example, ATP-induced activation of P2X receptors can evokesingle-channel cation currents from chick ciliary ganglion nerveterminals (Sun and Stanley, 1996) and enhance the frequency ofminiature endplate currents at the frog neuromuscular junction(Fu and Poo, 1991). Activation of P2X receptors has also beenshown to increase the frequency of miniature postsynaptic currentsin dorsal root ganglion dorsal horn neuronal cocultures (Gu andMacDermott, 1997; MacDermott et al., 1999) and increase excitationin the hippocampus (Wieraszko and Seyfried, 1989; Inoue et al.,1992, 1995). However, high concentrations of ATP (micromolar)are known to induce a long-lasting form of synaptic depressionthat cannot be explained by the degradation of ATP into adenosine(Wieraszko and Seyfried, 1989). The synaptic depression mediatedby high concentrations of ATP could be explained by the activationof presynaptic P2X₇ receptors. Recently, Deuchars et al. (2001)reported the presynaptic localization of P2X₇ receptors in thespinal cord and brainstem of the rat. We subsequently investigatedthe anatomical distribution of P2X₇ receptors in the rat hippocampus.When we discovered that P2X₇ receptors were abundant on hippocampalmossy fiber terminals, we used whole-cell and extracellular fieldrecordings to determine the actions of P2X₇ receptor activationon neurotransmission at this synapse. In the following study,we provide physiological and pharmacological evidence that activationof these presynaptic P2X₇ receptors results in rapid and long-lastingsynaptic depression that is mediated through a p38 MAP kinasesignalingcascade.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

SDS-PAGE and Western blotting. Hippocampal proteins were isolated from Sprague Dawley rats (3-4 weeks old) and homogenizedin 0.32 M sucrose. Small (P₂) and large (P₃) mossy fiber synaptosomalfractions were then isolated according to previously publishedmethods (Terrian et al., 1988, 1989). Proteins were subjectedto SDS-PAGE on 10% gels and probed with the following antibodies:rabbit anti-P2X₇ polyclonal (1:18,000; Alomone Laboratories, Jerusalem,Israel), rabbit anti-NMDA receptor subunit 1 (NMDAR1) (1:3000;Chemicon, Temecula, CA), mouse anti- $beta$ -tubulin (1:6000; Sigma,St. Louis, MO), and rabbit anti-synaptoporin (1:30,000; SynapticSystems, Gottingen, Germany). Immunoreactive signals were visualizedusing peroxidase-labeled goat secondary antibodies (1:10,000;Jackson ImmunoResearch, West Grove, PA) and enhanced chemiluminescence(Lumi-Light^plus; Roche Diagnostics, Mannheim,Germany).

Immunocytochemistry. For immunocytochemistry, rats were anesthetized and transcardially perfused with 4% paraformaldehydein 0.1 M phosphate buffer, pH 7.4. Brains were sectioned in thecoronal plane (50 µm) on a vibrating microtome (VT100; Leica,Willowdale, Ontario, Canada) and processed for immunocytochemistryusing standard procedures (Sloviter et al., 1996). The followingprimary antibodies were used: rabbit anti-P2X₇ (1:3000; AlomoneLaboratories), mouse anti-MAP-2 (1:20,000; Sigma), or anti-syntaxin1A/B (1:5000; Stressgen, Victoria, British Columbia, Canada).The following secondary antibodies were used: biotinylated donkeyanti-mouse or rabbit IgG, Cy2-conjugated donkey anti-mouse IgGand Cy3-conjugated donkey anti-rabbit IgG, or Cy5-conjugated donkeyanti-rabbit IgG (1:1000;all from Jackson ImmunoResearch). Sectionswere imaged on an Axioskop LSM510 laser scanning microscope (CarlZeiss Microscopy, Jena,Germany).

Electrophysiology. Hippocampal slices (300 µm thick) were obtained from 10- to 30-d-old rats, immersed in ice-cold artificialCSF (aCSF; see below), and incubated in a submersion chamber for $>=$ 1 hr at room temperature. For recordings, individual slices weretransferred to either an interface chamber (Fine Science Tools,Foster City, CA) for extracellular recordings or a submersionchamber for whole-cell voltage-clamp recordings. All recordingswere done at room temperature. In either chamber, slices weresuperfused (2 ml/min) with aCSF consisting of (in mM): 119 NaCl,2.5 KCl, 1.3 MgSO₄, 26 NaHCO₃, 1 NaH₂PO_4, 2.5 CaCl₂, and 10 glucose,aerated with 95% O₂/5% CO₂. Extracellular recordings were obtainedwith glass micropipettes filled with HEPES-buffered aCSF (resistance,1-3 M $Omega$ ). Extracellular recordings were filtered at 5 kHz, digitizedat 10 kHz using a Digidata1200 interface (Axon Instruments, FosterCity, CA), and stored on a Pentium III computer for later analysisusing Clampfit (Axon Instruments). A bipolar tungsten-stimulatingelectrode was used to stimulate dentate granule cells, therebyactivating mossy fibers. Mossy fiber-CA3 synaptic responses weremeasured in the stratum lucidum of the CA3 region and distinguishedby their characteristic short latency, rapid rise time, largepaired-pulse facilitation (PPF), and >70% inhibition by the metabotropicglutamate receptor (mGluR) agonist (2s,1's,2's)-2(carboxycyclopropyl)glycine(L-CCG-1).

Whole-cell recordings were obtained using patch pipettes filled with (in mM): 100 cesium methanesulfonate, 10 cesium-BAPTA,40 HEPES, and 5 N-(2,6-dimethylphenyl carbamoylmethyl)triethylammoniumbromide, adjusted to a pH of 7.3 with cesium hydroxide (resistance,1-3 M $Omega$ ). CaCl₂ and MgSO₄ were increased to 4 mM in the aCSF forall whole-cell recordings. During paired-pulse facilitation experiments,picrotoxin (10 µM) was included in the patch pipette to blockGABA_A receptors (Nelson et al., 1994; Xiang and Brown, 1998).Series resistance in all recordings was <20 M $Omega$ , and data wereexcluded if series resistance varied by >15%. All recordings weredigitized at 5-10 kHz and filtered at 2kHz.

Statistics. All statistics were performed using a paired (correlated groups) t test except for the comparison between theeffect of 2',3'-O-(4-benzoylbenzoyl)-ATP (Bz-ATP) and adenosineon slices incubated with 4-(4-fluorophenyl)2-(4-methylsulfinylphenyl)5-(4-pyridyl)imidazole(SB203580). In this case, a simple one-way ANOVA wasused.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

P2X₇ receptors were found on mossy fiber terminals

Western blotting and immunocytochemistry revealed that P2X₇ receptors were abundant on presynaptic terminals of the rat hippocampus.We used a P2X₇ antibody that was raised against amino acid residues576-595 of the rat P2X₇ receptor subunit. This antibody recognizeda single 70 kDa band in Western blots of proteins isolated fromthe hippocampus (Fig. 1A,B), small (P₂) hippocampal synaptosomes,and large, mossy fiber (P₃) synaptosomes (Fig. 1B). Inclusionof the P2X₇ antigenic peptide (1:1) with the antibody blockeddetection of the 70 kDa P2X₇-immunoreactive band. We did not detectany signal in the P₃ fraction with an antibody against iba-1,a protein selectively expressed in microglia (Ito et al., 1998).This indicates that microglia did not contaminate our P₃ synaptosomepreparation (data not shown). Immunocytochemistry with this P2X₇-selectiveantibody revealed dense immunoreactive terminals throughout mossyfiber termination zones in the dentate hilus and stratum lucidumof CA3 (Fig. 1C, arrows). Fainter staining was also observed throughoutthe hippocampus and may represent immunoreactivity of other presynapticterminals, or glial cells, such as microglia (Ferrari et al.,1996; Chessell et al., 1997; Di Virgilio et al., 1999) or astrocytes(Kukley et al., 2001; Panenka et al., 2001). Confocal microscopyconfirmed that the P2X₇-immunoreactive boutons were presynapticmossy fiber terminals, because P2X₇ immunoreactivity was colocalizedwith presynaptic syntaxin 1A/B immunoreactivity (Bennett et al.,1992; Ruiz-Montasell et al., 1996) (Fig. 1G-I) but not with dendriticMAP-2 immunoreactivity (Fig. 1D-F).

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Figure 1. P2X₇ receptors are located on presynaptic terminals of mossy fiber synapses. A, A Western blot of proteins isolated from the rat hippocampus showed that the P2X₇ antibody recognized a single band of protein at an approximate molecular weight of 70 kDa. Lane 1, Amido Black-stained proteins that were first immunoblotted in lane 2. B, P2X₇-immunoreactive bands of protein were present in proteins isolated from whole hippocampus (H), as well as small (P₂) synaptosomal and large (P₃) mossy fiber synaptosomal preparations. The presence of synaptoporin and relatively low abundance of NMDAR1 and $beta$ -tubulin indicates that P2X₇ receptors were highly enriched in the fraction containing mossy fiber terminals (P₃). C, Immunocytochemistry with this P2X₇-selective antibody revealed dense immunoreactivity throughout mossy fiber termination zones in the dentate hilus (h) and stratum lucidum (luc) of CA3 (arrows). Fainter staining was also observed throughout the hippocampus and may represent immunoreactivity of other presynaptic terminals. rad, Stratum radiatum; l-m, stratum lacunosum-moleculare; m, molecular layer; dgc, dentate granule cell layer. D-L, Colocalization studies demonstrated that P2X₇ immunoreactivity was located in the presynaptic terminals of mossy fiber synapses. D-F, P2X₇ immunoreactivity (blue) was found throughout stratum lucidum; however, dendritic MAP2 immunoreactivity (green) did not colocalize with the punctate P2X₇ immunoreactivity. Cell bodies were counterstained with ethidium bromide (red). G-I, In contrast, presynaptic syntaxin 1A/B immunoreactivity (green) was colocalized with the punctate P2X₇ immunoreactivity (red), demonstrating that the mossy fiber terminals contained P2X₇ receptors. Scale bars: C, 2 mm; D, 70 µm; E, 50 µm; F, 30 µm; G-I, 100 µm.

P2X₇ receptor activation depressed mossy fiber-CA3 synaptic transmission

Next, we investigated the effect of P2X₇ receptor activation on synaptic transmission at mossy fiber synapses. First, we recordedevoked postsynaptic field potentials (fEPSPs) in the stratum lucidumof CA3 after stimulation of the dentate granule cells (Fig. 2).To ensure that we were recording from mossy fiber-CA3 synapses,we first applied L-CCG-I (20 µM), an mGluR agonist that selectivelydepresses mossy fiber inputs onto CA3 pyramidal cells (Manzoniet al., 1995; Schmitz et al., 2000). Bath application of L-CCG-Ireversibly depressed the amplitude of the fEPSP (Fig. 2A). Subsequentbath application of the P2X₇ receptor agonist Bz-ATP (30 µM) alsodepressed the fEPSP (Fig. 2A). However, application of L-CCG-Iduring the peak of the Bz-ATP response did not result in any additionaldepression of the synaptic response (fEPSP amplitude after Bz-ATPwas 0.22 ± 0.12 of controls vs 0.17 ± 0.09 of controls in Bz-ATPplus L-CCG-I; mean ± SEM; n = 3), indicating that P2X₇ receptoractivation depressed the same population of synaptic inputs asL-CCG-I. Bz-ATP was also applied alone to monitor the time courseof the P2X₇-mediated synaptic depression without previous L-CCG-Iapplication (Fig. 2B). This prevented any potential interactionsbetween progressive drug applications. As shown in Figure 2B,Bz-ATP caused a rapid and long-lasting (>2 hr) statistically significant(t₍₅₎ = 10.37; p < 0.01) decrease in the fEPSP (fEPSP amplitudeafter Bz-ATP was 0.3 ± 0.05 of control amplitude; mean ± SEM;n = 6).

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Figure 2. The P2X₇ agonist Bz-ATP depressed mossy fiber fEPSPs but had no detectable effect on the presynaptic fiber volley. A, Averaged sample traces and plots of mossy fiber-CA3 synaptic responses recorded extracellularly from the stratum lucidum during one experiment at the indicated time points. L-CCG-I (20 µM) reversibly depressed the postsynaptic component of the field potential (indicated by * in the first trace). Bz-ATP (30 µM) depressed the L-CCG-I-sensitive component of the fEPSP, and coapplication of L-CCG-I did not cause additional depression. B, Summary of separate experiments in which Bz-ATP was applied without preapplication of L-CCG-I. Averaged sample traces are shown before and after Bz-ATP application. Plot shows the mean values obtained from six slices. Bz-ATP depressed the mossy fiber fEPSP amplitude for >2 hr. C, Single plot and mean sample traces from a single experiment in which the field response was recorded in the presence of NBQX (20 µM) to monitor the presynaptic fiber volley. Bz-ATP had no effect on the presynaptic fiber volley. D, Summary of the effects of Bz-ATP on the fEPSP (n = 6) and the presynaptic fiber volley (n = 5). C, Control. *Statistical significance using a paired t test; p < 0.01. Calibration: A, 0.2 mV, 20 msec; B, 0.5 mV, 10 msec; C, 0.3 mV, 20 msec.

In separate experiments, the postsynaptic response was blocked by 2,3-dihydroxy-6-nitro-7-sulfonyl-benzo[f]quinoxaline (NBQX),and the presynaptic fiber volley was monitored after Bz-ATP application(Fig. 2C). There were no significant (t₍₄₎ = $-$ 1.13; p > 0.05)alterations in the presynaptic fiber volley as a result of Bz-ATPapplication (n = 5; summarized in Fig. 2D). Furthermore, we visualizedmossy fiber terminals using a laser scanning microscope to seewhether Bz-ATP induced the uptake of YO-PRO-1 via pore dilationand cell lysis (Virginio et al., 1999). We did not observe anyuptake of YO-PRO-1 after Bz-ATP application (data not shown; n= 2). These data suggest that activation of P2X₇ receptors withBz-ATP does not induce cytolysis of mossy fiberterminals.

Next, we obtained whole-cell voltage-clamp recordings from CA3 pyramidal neurons to determine whether Bz-ATP selectively depressedmossy fiber-CA3 synaptic transmission or had a postsynaptic effecton AMPA receptors. As shown in Figure 3, Bz-ATP significantly(t₍₅₎ = 22.36; p < 0.01) depressed the amplitude of voltage-clampedmossy fiber EPSCs (mossy fiber EPSC amplitude after Bz-ATP was0.33 ± 0.04 of controls; mean ± SEM; n = 6) but had no statisticallysignificant (t₍₄₎ = 2.02; p > 0.05) effect on associational-commissuralEPSCs (associational-commissural EPSC amplitude after Bz-ATP was0.81 ± 0.1 of controls; mean ± SEM; n = 5). Associational-commissuralresponses were evoked by stimulation of the stratum radiatum inthe presence of L-CCG-I to block mossy fiber synapses. Bz-ATPalso had no significant effect on the CA3 whole-cell conductance(308 ± 34 pS before vs 288 ± 60 pS after Bz-ATP) or holding current(65.8 ± 8.2 pA before Bz-ATP application vs 71.6 ± 7.9 pA afterBz-ATP). Therefore, P2X₇ receptor activation selectively depressedmossy fiber synapses and had no direct postsynaptic effect onCA3 neurons.

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Figure 3. Activation of presynaptic P2X₇ receptors with Bz-ATP selectively depressed synaptically evoked mossy fiber currents in CA3. A, Plots of mean whole-cell voltage-clamp recordings in CA3 pyramidal neurons after stimulation of the mossy fiber (MF) pathway (n = 6 slices) or the associational-commissural (A/C) pathway (n = 5 slices). Bz-ATP significantly depressed the amplitude of voltage-clamped mossy fiber EPSCs but had no significant effect on associational-commissural EPSCs. B, Summary of the data presented in A. *Statistical significance using a paired t test; p < 0.01. C, Average sample traces from evoked responses after stimulation of the mossy fiber pathway or the associational-commissural pathway. Con, Control. Calibration: C, 200 pA, 50 msec; 250 pA, 50 msec.

Bz-ATP-induced synaptic depression was blocked by oxidized periodate-ATP

To further delineate P2X₇ receptor involvement in this Bz-ATP-induced effect, we assessed the ability of Bz-ATP to inducesynaptic depression of mossy fiber-CA3 fEPSPs in the presenceof the nonselective P2Y antagonist reactive blue 2 (RB2; 30 µM)(Fig. 4A) or the P2X_1-3,5,6 receptor antagonist pyridoxalphosphate-6-azophenyl-2',4'-disulfonicacid (PPADS; 10 µM) (Fig. 4B). As shown in Figure 4, both RB2(n = 5) and PPADS (n = 4) failed to block the effect of Bz-ATPon mossy fiber fEPSPs (t₍₄₎ = 13.81, p < 0.01; and t₍₃₎ = 26.5,p < 0.01, respectively). These data suggest that Bz-ATP-inducedsynaptic depression was not mediated by the nonselective activationof P2Y receptors or postsynaptically located P2X_1-3,5,6receptors.

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Figure 4. The selective P2X₇ antagonist o-ATP blocked Bz-ATP-induced depression of the mossy fiber-CA3 synaptic responses. A, Plots and average sample traces of mossy fiber-CA3 synaptic responses recorded extracellularly from the stratum lucidum of CA3 in the presence of the nonselective P2Y antagonist RB2 (30 µM; n = 5 slices). RB2 failed to block the effect of Bz-ATP on mossy fiber fEPSPs. B, Similarly, the P2X_1-3,5,6 receptor antagonist PPADS failed to block the effect of Bz-ATP on mossy fiber fEPSPs (n = 4 slices). C, However, preincubation of the slices with the P2X₇ receptor antagonist o-ATP (100 µM; n = 5 slices) significantly reduced the magnitude of the Bz-ATP-induced depression compared with controls (n = 5 slices). D, Summary of data presented in A-C. Con, Control. *Significance using a paired t test; p < 0.01. Calibration: A, 0.5 mV, 10 msec.

To determine whether Bz-ATP-induced synaptic depression was mediated by activation of P2X₇ receptors, we applied Bz-ATP inthe presence of the P2X₇ receptor antagonist oxidized periodate-ATP(o-ATP; 100 µM) (Murgia et al., 1993; Visentin et al., 1999).Consistent with Bz-ATP acting at presynaptic P2X₇ receptors, Bz-ATP-inducedsynaptic depression was potently inhibited by 2 hr of preincubationwith the P2X₇ antagonist o-ATP (in matched slices, fEPSP amplitudeafter Bz-ATP was 0.3 ± 0.05 of controls vs 0.81 ± 0.12 of controlsin slices preincubated with o-ATP; mean ± SEM; n = 5 for both)(Fig. 4C). This P2X₇-like pharmacological profile combined withour inability to detect a postsynaptic current in CA3 pyramidalcells suggests that Bz-ATP acted presynaptically at P2X₇ receptorsto mediate mossy fiber synapticdepression.

P2X₇ receptor activation increased paired-pulse facilitation

If Bz-ATP depresses mossy fiber synaptic transmission by activating presynaptic P2X₇ receptors, then Bz-ATP-induced depressionshould be associated with an increase in PPF (Regehr et al., 1994;Salin et al., 1996). We monitored PPF while recording whole-cellsynaptic-evoked currents in CA3 neurons. Consistent with Bz-ATPactivating presynaptic P2X₇ receptors, we observed a significant(t₍₄₎ = $-$ 4.65; p < 0.01) increase in the ratio of the second EPSCamplitude to the first EPSC amplitude immediately after applicationof Bz-ATP (ratio before Bz-ATP was 1.74 ± 0.05; ratio after was2.14 ± 0.09; mean ± SEM; n = 5 slices) (Fig. 5). These data indicatethat Bz-ATP decreased the probability of release at mossy fibersynapses.

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Figure 5. Activation of presynaptic P2X₇ receptors increased mossy fiber PPF (50 msec). PPF was monitored by recording whole-cell synaptic currents evoked in CA3 neurons (n = 5 slices). A, Mean PPF ratio before and after application of Bz-ATP. *Statistical significance using a paired t test; p < 0.01. We observed a significant increase in the PPF ratio after Bz-ATP application, which is consistent with Bz-ATP acting on presynaptic P2X₇ receptors. B, Average sample traces before and after Bz-ATP application. The lower trace on the right was rescaled so that the first current was the same size after Bz-ATP as it was in controls. Con, Control. Calibration: B, 200 pA, 50 msec; rescaled traces, 70 pA.

P2X₇ receptor-mediated synaptic depression required activation of p38 MAP kinase

Recent evidence suggests that MAP kinase activity is potently activated by synaptic activity and is essential for some formsof synaptic plasticity (Impey et al., 1999). For example, extracellularsignal-regulated kinase 1 (ERK1)/ERK2 MAP kinase activation isessential for the induction of long-term potentiation, and p38MAP kinase activity is essential for the induction of long-termdepression in CA1 of the hippocampus (Bolshakov et al., 2000).We have shown recently that activation of P2X₇ receptors in culturedastrocytes leads to activation of p38 and ERK1/ERK2 MAP kinase(Panenka et al., 2001). To determine whether MAP kinase activitywas necessary for the synaptic depression induced by Bz-ATP wepreincubated the slices (2 hr) with the p38 MAP kinase inhibitorSB203580 (25 µM) or the ERK1/ERK2 MAP kinase inhibitor 2'-amino-3'-methoxyflavone(PD98059; 50 µM). Bz-ATP-induced synaptic depression of the L-CCG-I-sensitivemossy fiber-CA3 postsynaptic response was significantly (t₍₃₎= 0.19; p > 0.05) blocked by inhibition of p38 MAP kinase activitywith SB203580 (fEPSP amplitude after Bz-ATP was 0.93 ± 0.12 ofcontrol amplitude in slices preincubated with SB203580; n = 4)(Fig. 6A). In contrast, preincubation of the slices with the ERK1/ERK2MAP kinase activity inhibitor PD98059 failed to block (t₍₃₎ =8.27; p < 0.01) Bz-ATP-induced mossy fiber synaptic depression(fEPSP amplitude after Bz-ATP was 0.24 ± 0.11 of controls in slicespreincubated with PD98059; n = 4) (Fig. 6B). These data demonstratethat activation of p38 MAP kinase was necessary for P2X₇ receptor-mediateddepression of mossy fiber-CA3 synaptic transmission.

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Figure 6. P2X₇ receptor-mediated mossy fiber synaptic depression required p38 MAP kinase activity. A, B, Plots of mean mossy fiber-CA3 synaptic responses recorded extracellularly from the stratum lucidum of CA3. A, Preincubation of the slices in the p38 MAP kinase inhibitor SB203580 (25 µM) completely blocked Bz-ATP-induced synaptic depression but had no effect on the L-CCG-I-induced depression of the mossy fiber fEPSP (n = 4 slices). B, Preincubation of the slices with the ERK1/ERK2 MAP kinase inhibitor PD98059 (50 µM) failed to have any effect on Bz-ATP-induced synaptic depression (n = 4 slices). C, Summary of data presented in A and B. Con, Control. *Significance using a paired t test; p < 0.01. Calibration: A, 0.5 mV, 10 msec.

Inhibitory effects of adenosine were not mediated through p38 MAP kinase

ATP and some of its analogs can be rapidly degraded into adenosine by the actions of ectonucleotidase (Dunwiddie et al., 1997;Cunha et al., 1998). Thus, ATP application can inhibit synaptictransmission indirectly through adenosine formation and the activationof presynaptic A1 receptors (Dunwiddie et al., 1997; Cunha etal., 1998; Cunha and Ribeiro, 2000; Dunwiddie and Masino, 2001).We could not use an A1 antagonist, such as 1,3-dipropylcyclopentylxanthine,because blocking A1 receptors results in persistent seizure activityin the CA3 region, making it impossible to record stable mossyfiber responses as reported previously (Thummler and Dunwiddie,2000). Therefore, to determine indirectly whether Bz-ATP-inducedmossy fiber-CA3 synaptic depression was mediated through degradationof Bz-ATP into adenosine, we tested whether adenosine inhibitssynaptic transmission through p38 MAP kinase activity. As shownin Figure 7, preincubation of the slices with SB203580 (25 µM)blocked Bz-ATP-induced mossy fiber synaptic depression (n = 4)but failed to have any effect on adenosine-mediated (30 µM) mossyfiber synaptic depression (n = 4). In slices preincubated withSB203580, the fEPSP amplitude after Bz-ATP was 0.95 ± 0.15 ofcontrols, versus 0.15 ± 0.09 of controls in adenosine (F_(1,6)= 21.58, p < 0.01). Therefore, adenosine does not exert its inhibitoryactions through p38 MAP kinase, and the presynaptic actions ofBz-ATP cannot be explained by the degradation of Bz-ATP into adenosine.

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Figure 7. The p38 antagonist SB203580 blocked the actions of Bz-ATP but not the inhibition by adenosine (30 µM). A, Plot of an extracellular recording in which the p38 MAP kinase inhibitor SB203580 blocked the Bz-ATP-induced mossy fiber synaptic depression but failed to block the adenosine-induced inhibition of the mossy fiber fEPSP. B, SB203580 differentially affected the depression induced by Bz-ATP and adenosine. Therefore, adenosine does not exert its inhibitory actions through p38 MAP kinase, and the presynaptic actions of Bz-ATP cannot be explained by the degradation of Bz-ATP into adenosine by ectonucleotidase activity. *Statistical significance using a one-way ANOVA; p < 0.01.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results of the present study demonstrate that activation of presynaptic P2X₇ receptors results in the inhibition of neurotransmissionat mossy fiber-CA3 synapses through a p38 MAP kinase-signalingpathway. First, we have used immunocytochemistry to demonstratethat P2X₇ receptors are abundant on presynaptic terminals of mossyfiber synapses in the rat hippocampus. Immunocytochemistry witha specific P2X₇ antibody resulted in the labeling of small terminal-likepuncta throughout the hippocampus. P2X₇ immunoreactivity was particularlydense throughout the termination zones of hippocampal mossy fibers,where it was completely colocalized with the presynaptic markersyntaxin 1A/B but not the dendritic marker MAP-2 (Fig. 1). Syntaxin1A is known to be present in the presynaptic mossy fiber terminals,and syntaxin 1B is present in the mossy fiber axons (Ruiz-Montasellet al., 1996). As demonstrated in Figure 1, all of the observedP2X₇ immunoreactivity in the stratum lucidum was colocalized withthe syntaxin 1A labeling of the presynaptic terminal. These datademonstrate that P2X₇ receptors are located presynaptically inthe stratum lucidum of the rat hippocampus. The specific presynapticP2X₇ receptor localization shown here is in contrast to the postsynapticlocation of other known P2X receptors in the hippocampus of therat (e.g., P2X₂, P2X₄, and P2X₆) (Le et al., 1998; Rubio and Soto,2001). These postsynaptically located receptors are likely tocontribute to the increase in excitation that is observed in thehippocampus after application of low doses of ATP (Wieraszko andSeyfried, 1989).

Consistent with their presynaptic localization, activation of P2X₇ receptors with Bz-ATP completely depressed the L-CCG-I-sensitivemossy fiber-CA3 synaptic response in extracellular field recordings.However, no direct effects of Bz-ATP on postsynaptic CA3 pyramidalneurons were observed when the conductance and holding currentwere monitored during whole-cell voltage-clamp recordings. Furthermore,we found no significant effect of Bz-ATP on AMPA receptor-mediatedassociationalcommissural synaptic transmission in CA3. This observationis consistent with our conclusion that Bz-ATP selectively activatespresynaptic P2X₇ receptors and suggests that at this concentration(30 µM), Bz-ATP did not activate other known postsynaptic P2Xreceptors (e.g., P2X₂, P2X₄, and P2X₆). Although our conclusionssupport the involvement of P2X₇ receptors in presynaptic depression,the possible contribution of P2X₄ cannot be totally eliminated.The enhancement of PPF during the Bz-ATP-induced synaptic depressionis also consistent with a presynaptic site of action (Regehr etal., 1994; Salin et al., 1996) similar to what has been observedduring mGluR-mediated depression in CA1 (Fitzjohn et al., 2001).Bz-ATP-induced synaptic depression was not blocked by the P2Yreceptor antagonist RB2 (30 µM) or the P2X_1-3,5,6 antagonistPPADS (10 µM). Other P2X receptors are antagonized by PPADS atthis concentration, whereas P2X₇ receptors are not (Surprenantet al., 1996). However, Bz-ATP-mediated synaptic depression requiredP2X₇ receptor activation, because little or no synaptic depressionwas observed when the slices were preincubated with the irreversibleP2X₇ receptor antagonist o-ATP (Fig. 4) (Murgia et al., 1993;Visentin et al., 1999). Bz-ATP-induced synaptic depression alsocannot be explained by the degradation of Bz-ATP into adenosineby local ectonucleotidases, because adenosine-mediated synapticinhibition was not blocked by p38 MAP kinase inhibition, whereasthe actions of Bz-ATP were blocked (seebelow).

Mossy fiber synapses contain vesicular ATP, and synaptosomes prepared from mossy fiber synapses release ATP in a Ca²⁺-dependent manner in response to K⁺-induced depolarization (Terrian et al., 1989). However, it isnot known whether ATP is normally released from mossy fiber synapsesor whether P2X₇ receptors are normally activated during the evokedrelease of neurotransmitters from mossy fiber terminals. It ispossible that presynaptic mossy fiber P2X₇ receptors might onlybe activated during intense periods of mossy fiber activity, suchas that observed during tetanus or seizure, when ATP release mightreach levels high enough to activate P2X₇ receptors. Therefore,P2X₇ receptors might play an important role in limiting synaptictransmission when mossy fiber synaptic transmission is unusuallyhigh.

The results of the present study demonstrate that activation of p38 MAP kinase is necessary for P2X₇ receptor-mediated depressionof mossy fiber-CA3 synaptic transmission. Maruyama et al. (2000)have demonstrated recently that p38 MAP kinase is abundant inthe terminals of mossy fiber synapses. As shown in Figure 6, Bz-ATP-inducedsynaptic depression was completely blocked by preincubation ofthe slices with the p38 MAP kinase activity inhibitor SB203580but not the ERK1/ERK2 MAP kinase activity inhibitor PD98059. Thepresynaptic mechanism by which P2X₇ receptor-dependent p38 MAPkinase activity depresses mossy fiber synaptic transmission remainsto be determined. However, recent evidence suggests that p38 MAPkinase activity is necessary for the inhibition of N-type calciumcurrents in neuroblastoma cells after bradykinin application (Wilk-Blaszczaket al., 1998). Therefore, it is possible that P2X₇ receptor-dependentp38 MAP kinase activity depresses mossy fiber synaptic transmissionthrough inhibition of calcium channels. However, mossy fiber terminalsexhibit predominantly P-type calcium channel-dependent evokedneurotransmitter release and contain few N-type channels (Castilloet al., 1994).

Recent evidence suggests that MAP kinase activity is potently activated by synaptic activity and is essential for some formsof neuronal plasticity (Impey et al., 1999; Bolshakov et al.,2000). For example, translocation of ERK1/ERK2 MAP kinase to thenucleus of the presynaptic neuron is essential for long-term facilitationin Aplysia neurons (Martin et al., 1997), and p38 MAP kinase isessential for the induction of mGluR receptor-dependent, long-termdepression in CA1 of the hippocampus (Bolshakov et al., 2000).Interleukin-1 $beta$ has also been shown to increase p38 activationand modify long-term potentiation in perforant path synapses (Verekeret al., 2000). In the present study, we have shown that the rapidand reversible depression of mossy fiber synaptic transmissionby the mGluR agonist L-CCG-I is unaffected by preincubation ofthe slices with the p38 MAP kinase inhibitor SB203580. Therefore,the mGluR-induced inhibition of mossy fiber synapses is apparentlynot mediated by p38 as it is inCA1.

In conclusion, we have provided evidence that P2X₇ receptor subunits are abundant on presynaptic terminals of mossy fibersynapses in the rat hippocampus. Activation of these presynapticP2X₇ receptors with the P2X₇ agonist Bz-ATP produced a rapid andlong-lasting synaptic inhibition at mossy fiber-CA3 synapses.This presynaptic inhibition was mediated by the activation ofp38 MAP kinase, because it was not observed when the slices werepreincubated with a p38 MAP kinase inhibitor. Therefore, the resultsof the present study demonstrate that unlike any other memberof the P2X receptor family, P2X₇ receptors can decrease neurotransmitterrelease at mossy fiber-CA3 synapses by activating p38 MAP kinasein the presynapticterminal.

  FOOTNOTES

Received Feb. 13, 2002; revised April 12, 2002; accepted May 1, 2002.

This work was supported by the Canadian Institutes for Health Research (CIHR). B.A.M. is an Alberta Heritage Foundation forHealth Research and CIHR Senior Scientist. T.B.B. was supportedby studentships from Libin Neuroscience Canada Foundation Alberta,the Natural Sciences and Engineering Research Council of Canada,and the Alberta Heritage Foundation for Medical Research. We thankDenise Feighan and Naili Liu for their technicalassistance.

Correspondence should be addressed to Brian A. MacVicar, Department of Physiology and Biophysics, Faculty of Medicine, Universityof Calgary, 3330 Hospital Drive Northwest, Calgary, Alberta, T2N4N1 Canada. E-mail: macvicar{at}ucalgary.ca.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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