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The Journal of Neuroscience, April 1, 2000, 20(7):2470-2479
Mechanisms of Cannabinoid Inhibition of GABAA
Synaptic Transmission in the Hippocampus
Alexander F.
Hoffman and
Carl R.
Lupica
Cellular Neurobiology Branch, National Institute on Drug Abuse,
Intramural Research Program, National Institutes of Health, Baltimore,
Maryland 21224
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ABSTRACT |
The localization of cannabinoid (CB) receptors to GABAergic
interneurons in the hippocampus indicates that CBs may modulate GABAergic function and thereby mediate some of the disruptive effects
of marijuana on spatial memory and sensory processing. To investigate
the possible mechanisms through which CB receptors may modulate
GABAergic neurotransmission in the hippocampus, whole-cell voltage-clamp recordings were performed on CA1 pyramidal neurons in rat
brain slices. Stimulus-evoked GABAA receptor-mediated IPSCs were reduced in a concentration-dependent manner by the CB receptor agonist WIN 55,212-2 (EC50 of 138 nM). This
effect was blocked by the CB1 receptor antagonist SR141716A (1 µM) but not by the opioid antagonist naloxone. In
contrast, evoked GABAB-mediated IPSCs were insensitive to
the CB agonist. WIN 55,212-2 also reduced the frequency of
spontaneous, action potential-dependent IPSCs (sIPSCs), without
altering action potential-independent miniature IPSCs (mIPSCs),
measured while sodium channels were blocked by tetrodotoxin (TTX).
Blockade of voltage-dependent calcium channels (VDCCs) by cadmium also
eliminated the effect of WIN 55,212-2 on sIPSCs. Depolarization of
inhibitory terminals with elevated extracellular potassium caused a
large increase in the frequency of mIPSCs that was inhibited by both
cadmium and WIN 55,212-2. The presynaptic effect of WIN 55,212-2 was
also investigated using the potassium channel blockers barium and
4-aminopyridine. Neither of these agents significantly altered the
effect of WIN 55,212-2 on evoked IPSCs. Together, these data suggest
that presynaptic CB1 receptors reduce GABAA- but not
GABAB-mediated synaptic inhibition of CA1 pyramidal neurons
by inhibiting VDCCs located on inhibitory nerve terminals.
Key words:
brain slice; calcium channels; cannabis; electrophysiology; GABAA receptors; GABAB
receptors; hippocampal; marijuana; potassium channels; presynaptic; ruthenium red
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INTRODUCTION |
The pharmacological actions of
marijuana within the mammalian CNS are attributable to specific
interactions between the active constituents of the drug, collectively
known as cannabinoids (CBs) and their receptors. Two subtypes of CB
receptor, known as CB1 and CB2, have been identified. The CB1 receptor
is expressed in high concentrations throughout the CNS, whereas the CB2
receptor is expressed primarily in immune cells (Pertwee, 1997 ; Axelrod and Felder, 1998). Cannabinoid receptors interact with G-proteins to
alter the activities of enzymes, such as adenylyl cyclase, and to
modulate ion channels (Matsuda, 1997; Pertwee, 1997). Studies of CB1
receptor localization within the CNS have revealed moderate to high
densities throughout several cortical areas, including the hippocampus
(Herkenham et al., 1990; Howlett et al., 1990; Pettit et al., 1998;
Tsou et al., 1998; Katona et al., 1999). Given the well established
role of the hippocampus in learning and memory processes, it is likely
that the adverse effects of marijuana on spatial learning tasks,
short-term memory, and attention are attributable to its actions within
this brain region (Miller and Branconnier, 1983; Murray, 1986;
Deadwyler et al., 1990; Hampson and Deadwyler, 1998).
Pyramidal neurons in area CA1 of the hippocampus receive both
excitatory and inhibitory inputs from intrinsic and extrinsic sources,
and they communicate with various cortical and limbic regions (Knowles,
1992). Several recent studies have addressed the role of CB1 receptors
in modulating excitatory synaptic transmission in the hippocampus.
Thus, presynaptic inhibition of glutamate release onto CA1 pyramidal
neurons by CBs has been described previously (Misner and Sullivan,
1999), and it has been suggested that this occurs through the
inhibition of voltage-dependent Ca2+
channels (VDCCs) of the N and P/Q classes (Twitchell et al., 1997; Shen
and Thayer, 1998; Sullivan, 1999). In contrast, although CB1-mediated
inhibition of GABAergic synaptic transmission has been demonstrated in
the basal ganglia (Chan et al., 1998; Szabo et al., 1998) and medulla
(Vaughan et al., 1999), similar studies have not been performed in the
hippocampus. The largest GABAergic input to CA1 pyramidal neurons is
derived from a diverse network of intrinsic interneurons (Freund and
Buzsáki, 1996; Buzsáki, 1997). Although these interneurons
represent only a small fraction (~10%) of the total hippocampal
neuronal population, each interneuron forms multiple synapses onto its
cellular targets. In this way, the release of GABA by interneurons
provides a means to coordinate pyramidal cell activity and hippocampal
output (Cobb et al., 1995; Buzsáki, 1997). The transmitter
released from the interneurons onto pyramidal cells can interact with
either GABAA or GABAB
receptors, generating fast IPSCs mediated by the activation of
Cl channels or slow IPSCs mediated by
the activation of K+ channels,
respectively (Alger and Nicoll, 1982; Solis and Nicoll, 1992; Ling and
Benardo, 1994). Recently, Katona and colleagues (1999) demonstrated
that CB1 receptors were located on the axon terminals of a specific
subpopulation of cholecystokinin-immunoreactive interneurons and
that CB1 receptor activation reduced
[3H]GABA release. However, this study
did not determine whether CB1 receptors inhibited synaptic GABA
release, nor did it identify the mechanism(s) involved in this
modulation. Several potential mechanisms may mediate CB modulation of
GABAergic transmission. For example, the inhibition of VDCCs (Shen and
Thayer, 1998; Sullivan, 1999), the activation of voltage-dependent
K+ channels (VDKCs) and
voltage-independent K+ channels (Deadwyler
et al., 1995; Mackie et al., 1995), the inhibition of GABA uptake
(Maneuf et al., 1996), or the activation of endogenous opioid pathways
(Chen et al., 1990) have all been proposed (Tanda et al., 1997). In the
present study, we compare the effects of CB1 receptor activation on
GABAA- and GABAB-mediated
synaptic transmission in the hippocampus, and we examine the potential mechanisms involved in this modulation. We demonstrate that CB1 receptor activation inhibits GABAA- but not
GABAB-mediated IPSCs through a presynaptic
mechanism that likely involves the inhibition of VDCCs.
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MATERIALS AND METHODS |
Slice preparation. All protocols were performed under
National Institutes of Health Guidelines and were approved by the
Institutional Animal Care and Use Committee (National Institute on Drug
Abuse, Intramural Research Program, Baltimore, MD). Male Sprague Dawley rats (Charles River Laboratories, Raleigh, NC), 14- to 30-d-old, were
killed by decapitation, and their brains rapidly removed and placed in
ice-cold oxygenated artificial CSF (aCSF) (see below). The brain
was then blocked in a coronal plane ~2 mm anterior and 5 mm posterior
to bregma using a razor blade. The posterior end of the tissue block
was then glued to the stage of a vibrating tissue slicer (Technical
Products International, St. Louis, MO) using cyanoacrylate. A
midsagittal cut was then made with a scalpel blade to separate the two
hemispheres, and brain slices were cut at 300 µm nominal thickness.
The slices were then transferred to a beaker containing aCSF and
aerated with 95% O2-5%
CO2 at room temperature in which they were stored
for at least 90 min before they were transferred to the recording
chamber. During recordings, slices were continuously superfused with
aCSF at a rate of 2 ml/min. All recordings were performed at room
temperature (~ 22° C). Control aCSF consisted of (in
mM): NaCl 126, KCl 3.0, MgCl2 1.5, CaCl2 2.4, NaH2PO4 1.2, glucose 11.0, and NaHCO3, 26, saturated with 95%
O2 and 5% CO2. In a few
experiments, Ca2+ and
Mg2+ were omitted from the buffer and were
instead applied at selected concentrations by superfusion using a
calibrated syringe pump (Razel Scientific Instruments Inc., Stamford, CT).
Pyramidal neuron recording. Whole-cell patch-clamp
recordings of spontaneous IPSCs (sIPSCs) and tetrodotoxin
(TTX)-resistant miniature IPSCs (mIPSCs) from pyramidal cells were
obtained using methods described previously (Lupica, 1995; Miller et
al., 1997). Briefly, recordings were performed using an Axoclamp-2A or
an Axopatch 200A amplifier (Axon Instruments, Burlingame, CA) and electrodes pulled from borosilicate thick-walled capillary tubing (inner diameter of 0.75 mm, outer diameter of 1.5 mm; Sutter Instrument Co., Novato, CA). Cells were voltage clamped at  60 to 90 mV using
whole-cell electrodes containing (in mM): CsCl
125.0, HEPES 10.0, EGTA 1.0, CaCl2 0.1, Mg2+-ATP 2.0, Na+-GTP 0.2, and the quaternary lidocaine
derivative QX-314 2, pH 7.2-7.4. Series resistance was monitored
continuously using small (10 mV), hyperpolarizing voltage steps (200 msec). Only cells demonstrating <20 M series resistance were used
in these experiments. In most cases, the series resistance did not
change appreciably during the recording period. However, in cases in
which the series resistance increased, there was a noticeable decrease
in whole-cell conductance and a sudden and sustained decrease in the
holding current. When this occurred, the cell was not used in further analyses. The glutamate receptor antagonists
6,7-dinitroquinoxaline-2,3-dione (DNQX) (10 µM)
and D-()-2-amino-5-phosphonopentanoic acid
(APV) (40 µM) were continuously present in the
aCSF to block EPSPs and to isolate the presynaptic interneurons
from excitatory afferent input. Spontaneous and mIPSCs were amplified
fivefold to 100-fold, filtered at 1-3 kHz, and recorded to videotape
for later analysis. Epochs of 1-3 min of data were digitized at 4-10
kHz using a National Instruments (Austin, TX) Lab PC 1200 analog-to-digital converter and the Strathclyde electrophysiology
software package (courtesy of Dr. John Dempster, Strathclyde
University, Glasgow, UK) and then analyzed using a personal
computer-based program (Mini Analysis 4.3; Synaptosoft, Leonia, NJ).
Averaged mIPSCs were generated by aligning individual events by rise
time, and a peak to decay single exponential fit was applied (before
and during drug application) using the formula y = A1 * exp(x/ ) + Baseline, where A1
is the peak amplitude, and is the time constant for decay.
Evoked GABAA-receptor-mediated IPSCs (evIPSCs)
were generated in the presence of DNQX and APV using a bipolar tungsten
stimulating electrode placed near (<100 µm) the recording electrode,
within stratum radiatum. Evoked GABAB-mediated
IPSCs were isolated by including picrotoxin (100 µM) in
the superfusion buffer and by using stimulation intensities that were
twofold to 2.5-fold greater than those necessary to evoke
GABAA-mediated IPSCs (see below). To monitor
whole-cell access, a constant hyperpolarizing step pulse (10-20 mV,
200 msec) was delivered after each stimulus using a Master-8 pulse
generator (A.M.P.I., Jerusalem, Israel). Stimulation (0.1 msec
duration) was delivered at 30 sec intervals using a constant current
unit (A.M.P.I.) and the pulse generator. Current output was adjusted to
evoke a submaximal response in each experiment (<200 µA). In those
cells in which sIPSCs or mIPSCs were not analyzed and in all cases in
which GABAB-receptor mediated responses were measured, recordings of evIPSCs were performed using K-gluconate-filled electrodes. These whole-cell electrodes had resistances of 7-10 M
when filled with the following solution (in mM):
K+-gluconate 125.0, KCl 10.0, HEPES 10.0, EGTA 1.0, CaCl2 0.1, Mg2+-ATP 2.0, and
Na+-GTP 0.2, adjusted to pH 7.2-7.4 with
1 M KOH and brought to 270-280 mOsm with deionized water.
Analyses of predrug and postdrug effects on evIPSCs were performed
using personal computer-based software (Neuropro SCOPE; R.C.
Electronics, Goleta, CA).
Chemicals. Drugs were obtained from the following sources.
TTX, DNQX, picrotoxin, ruthenium red, bicuculline methiodide, DAMGO [Tyr-D-Ala2,N-CH3-Phe4,Gly-ol-enkephalin],
CdCl2, 4-aminopyridine, naloxone, and
BaCl2 were from Sigma (St. Louis, MO). APV and
WIN 55,212-2 were from Tocris Cookson (Ballwin, MO). SR141716A was
obtained from the National Institute on Drug Abuse drug supply system.
CGP 35348 was a generous gift from Drs. D. Scholer and H. Kaufmann
(CIBA-Geigy Ltd., Basel, Switzerland). WIN 55,212-2 and SR141716A were
prepared as concentrated (10-100 mM) stock
solutions in DMSO. Final (bath) concentrations were <0.01% DMSO. All
drugs were made up at either 50 or 100 times the desired final
concentration in deionized water and then added to the flow of the
superfusion medium using a calibrated syringe pump (Razel Scientific
Instruments Inc.).
Statistical analysis. Group data are presented as the
mean ± SEM in all cases. Drug-induced changes in cumulative sIPSC
and mIPSC amplitude and interevent interval distributions were
analyzed for statistical significance using the Kolmogorov-Smirnov
(K-S) test (Mini Analysis 4.3) and a conservative critical
probability level of p < 0.01. All other statistical
tests were performed using a critical probability of p < 0.05 (Prism version 2.01; GraphPad Software, San Diego CA).
Post hoc analysis was performed only when an ANOVA yielded a
significant (p < 0.05) main effect.
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RESULTS |
Effect of WIN 55,212-2 on evoked GABAA IPSCs in
pyramidal neurons
In cells clamped at 80 mV, using a CsCl-based internal solution,
a single stimulus evoked a fast inward current that was abolished by
application of either the GABAA receptor
antagonist bicuculline methiodide (20 µM) or the
Cl channel blocker picrotoxin (100 µM). After a 3-5 min period to allow for stabilization
of the baseline response, the CB receptor agonist WIN 55,212-2 was
applied via the aCSF. As shown in Figure 1, application of WIN 55,212-2 (5 µM) resulted in a slow, time-dependent decrease in the
evoked GABAA receptor-mediated IPSC. Maximal
inhibition of the response generally occurred within 5-7 min of drug
application, and the peak inhibition of the response was 47 ± 4%
(n = 12) with 5 µM WIN
55,212-2. Because of the lipid soluble nature of WIN 55,212-2,
reversal of the drug effect by washout was not possible within the
temporal parameters of the recording session. Therefore, we attempted
to block the effect using the selective CB1 antagonist SR141716A
(Rinaldi-Carmona et al., 1994). Because the antagonist is also highly
lipid soluble, we found it necessary to preincubate the slices with it
for 10-15 min before application of WIN 55,212-2. Alone, SR141716A (1 µM) had no significant effect on the evIPSC (115 ± 17% of control; n = 9) (Fig.
1A). However, as shown in Figure 1, SR141716A
significantly antagonized the effect of WIN 55,212-2 on the evIPSC
(120 ± 11% of control; n = 9).
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Figure 1.
Effect of WIN 55,212-2 on stimulus-evoked
GABAA receptor-mediated IPSCs in CA1 pyramidal neurons.
Whole-cell recordings were performed using CsCl-based electrode
solution at a holding potential of 80 mV. Current
traces represent an average of 5-10 sweeps.
A, In the top series of
traces, application of 5 µM WIN 55,212-2
reduced the GABAA IPSC. Control and drug
traces are superimposed for clarity. In a different cell
shown in the bottom series of traces,
application of SR141716A (1 µM; 10 min) did not alter the
IPSC. In the continued presence of SR141716A, WIN 55,212-2 had no
effect on the IPSC. B, Summary of the effect of WIN
55-212, plotted as a percentage change (mean ± SEM) from
control. Closed circles represent the effect of WIN
55,212-2 alone (n = 12), and open
circles represent the effect of WIN 55,212-2 after
pretreatment with SR141716A (n = 9).
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We also performed a concentration-response analysis using the
sequential cumulative administration of increasing concentrations (2-4
concentrations per slice) of WIN 55,212-2. For these experiments, IPSCs were measured using K+-
gluconate-filled electrodes because of the increased stability of these
recordings over long periods of time. As shown in Figure 2, WIN 55,212-2 inhibited the evoked
IPSCs in a concentration-dependent manner, with an estimated
EC50 of 138 nM. In these experiments, stable, peak effects of the lower concentrations of WIN 55,212-2 occurred more slowly (10-15 min) than at higher concentrations of the
drug (5-7 min). However, we ensured response stability by measuring
3-5 similar consecutive responses at a given drug concentration.
Also, when the effect of the 1 µM concentration of WIN
55,212-2 (n = 3), observed at the end of the
cumulative administration paradigm, was compared with the effect at the
same concentration in WIN 55,212-2-naïve neurons
(n = 3), no significant differences were observed
(p < 0.05; two-tailed Student's t
test). This suggests that the effects of WIN 55,212-2 were
concentration-dependent and that CB1 receptor desensitization did not
occur during the cumulative administration of the drug.
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Figure 2.
Concentration-dependent effect of WIN 55,212-2 on
evoked GABAA IPSCs in CA1 pyramidal neurons.
A, Recording from a single neuron using a
K+-gluconate-based electrode solution at a holding
potential of 55 mV. Control and WIN 55,212-2 concentrations are
labeled for each trace. Traces represents
an average of 5-10 sweeps taken at the peak of a stable drug response.
B, Concentration-response curve for WIN 55,212-2. Each
data point represents the mean ± SEM of the maximal inhibition of
the evoked IPSC (n = 3-12 cells). The
EC50 estimated from the fitted curve is 138 nM.
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Several studies have demonstrated that CB-mediated actions in the CNS
could be explained by the stimulation of opioid receptors (Chen et al.,
1990; Tanda et al., 1997). Because of these observations and because
opioid receptors are known to inhibit GABA release in the hippocampus
(Siggins and Zieglgansberger, 1981; Cohen et al., 1992; Lupica, 1995),
we examined the possibility that the effects of WIN 55,212-2 might be
mediated via activation of an endogenous opioid pathway. Slices were
pretreated with the opioid antagonist naloxone (5 µM),
and the effects of WIN 55,212-2 (1 µM) were tested on
GABAA evIPSCs in the presence of naloxone. The
reduction in evIPSC amplitude in the presence of naloxone (64 ± 3% of control; n = 10) was not significantly different
than the reduction of evIPSCs by 1 µM WIN
55,212-2 alone (56 ± 7% of control; n = 6;
p = 0.29; unpaired t test). This suggests
that the inhibition of GABAA-mediated IPSCs by
WIN 55,212-2 was not attributable to activation of opioid receptors by
either the agonist itself or endogenous opioid peptides.
Effect of WIN 55,212-2 on GABAB IPSCs
The results described above demonstrate that CB1 receptor
activation reduces fast, GABAA-mediated IPSCs in
CA1 pyramidal neurons. However, CA1 neurons also demonstrate a slow
IPSC, mediated by activation of GABAB receptors
and the opening of inwardly rectifying G-protein-coupled
K+ channels (GIRK) (Alger and
Nicoll, 1982; Solis and Nicoll, 1992; Ling and Benardo, 1994). In
addition, it has been proposed that GABAB-mediated IPSCs occur in response to GABA
release from afferent fibers that are distinct from those mediating
GABAA IPSCs (Nurse and Lacaille, 1997).
Therefore, to determine whether GABAB IPSCs were
also sensitive to modulation by CB1 receptors and whether this subset
of GABAergic fibers was sensitive to presynaptic inhibition by CB1
receptors, we measured GABAB IPSCs in CA1
pyramidal neurons. Stimulus-evoked GABAB IPSCs
were isolated in neurons voltage clamped at 55 to 65 mV in the
presence of DNQX (10 µM), APV (40 µM), and
picrotoxin (100 µM). The IPSCs observed under these
conditions were significantly reduced (p < 0.01; n = 6) by application of the
GABAB receptor antagonist CGP 35348 (100 µM) (Fig. 3), and they reversed polarity at membrane potentials between 90 and 110
mV, suggesting that they were mediated by
K+ currents
(Ek of 96 mV with
[K+]o of 3.0 mM and
[K+]i of 135.0 at
20° C, using the Nernst equation). In contrast to its effect on the
GABAA-mediated IPSC, WIN 55,212-2 (1 µM) did not significantly alter the amplitude
of the GABAB-mediated response
(p > 0.05; n = 7; one-way
ANOVA) (Fig. 3). However, in agreement with a previous study (Lupica et
al., 1992), these GABAB responses were
significantly inhibited presynaptically by the µ-opioid agonist DAMGO
(1 µM; p < 0.05;
n = 4) (Fig. 3B).
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Figure 3.
Effect of WIN 55,212-2 on GABAB
receptor-mediated IPSCs. A, Recording from a single
neuron clamped at 55 mV using K+-gluconate-based
internal solution. APV (40 µM), DNQX (10 µM), and picrotoxin (100 µM) were included
in the superfusion medium. Traces represent an average
of 8-10 sweeps. Application of the GABAB antagonist CGP
35348 (100 µM) reduced the IPSC amplitude, and this
effect reversed within ~10 min. Subsequent application of WIN
55,212-2 (1 µM; 15 min) did not decrease the IPSC.
B, Summary of the effects of WIN 55,212-2 (1 µM; n = 7)
(WIN), CGP 35348 (100 µM;
n = 6) (CGP), and the µ-opioid
agonist DAMGO (1 µM; n = 4) on the
GABAB response (*p < 0.05, **p < 0.01 vs control; one-way ANOVA, followed by
Tukey-Kramer post hoc analysis). For comparison, the
effect of 1 µM WIN 55,212-2 on the GABAA
receptor-mediated IPSC is shown (solid bar)
(n = 6; **p < 0.01 vs WIN
effect on GABAB IPSC; unpaired Student's t
test).
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Effect of WIN 55,212-2 on spontaneous GABAA IPSCs
The inhibition of GABAA-mediated evoked
IPSCs by WIN 55,212-2 could involve either presynaptic or postsynaptic
mechanisms. To distinguish between these possibilities, we conducted
studies examining the effects of WIN 55,212-2 on spontaneously
occurring IPSCs. Action potential-dependent sIPSCs were measured in
pyramidal neurons under voltage clamp at 80 mV (n = 6). Treatment with WIN 55,212-2 (5 µM)
significantly reduced the mean amplitude of the sIPSCs from 16.7 ± 3.7 to 11.9 ± 1.4 pA (p < 0.05;
Wilcoxon signed rank test). In addition, the mean frequency of sIPSCs
was significantly reduced by WIN 55,212-2 from 2.0 ± 0.3 Hz in
control to 1.2 ± 0.1 Hz (p < 0.05;
Wilcoxon signed rank test). The effects of WIN 55,212-2 on sIPSC
amplitude and frequency are shown in Figure
4. Significant differences in both the
cumulative amplitude and cumulative interevent interval distributions
(p < 0.001; Kolmogorov-Smirnov test) were
observed in five of six cells tested during WIN 55,212-2 application.
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Figure 4.
Effect of WIN 55,212-2 on spontaneous, action
potential-dependent IPSCs in a CA1 pyramidal neuron. Recording was
performed using a CsCl-based electrode solution at a holding potential
of 80 mV. A, Traces represent portions
of 2 min epochs recorded before (Control) and
during the peak drug effect (~7 min after 5 µM WIN
55,212-2 application). B, Cumulative interevent
interval distribution shown for the same cell, revealing a significant
increase in the interevent interval (i.e., decreased frequency;
p < 0.001; K-S test) during WIN 55,212-2
application. C, Cumulative amplitude distribution
obtained from the same cell reveals a significant decrease in sIPSC
amplitude (p < 0.001; K-S test) in the
presence of WIN 55,212-2. The mean sIPSC amplitude in this cell was
decreased from 29.5 pA (n = 392 events) to 18.4
pA (n = 145 events). D, Summary of
the effect of 5 µM WIN 55,212-2
(WIN) on the amplitude and frequency of sIPSCs
(mean ± SEM; n = 5). Significant reductions
were observed in both amplitude and frequency (*p < 0.05; Wilcoxon signed rank test). Calibration: 50 pA, 500 msec.
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Effects of WIN 55,212-2 on miniature IPSCs
To further confirm a presynaptic mechanism for the actions of WIN
55,212-2 on GABA release and to assess the role of voltage-dependent ion channels in this effect, we measured action potential-independent mIPSCs in the presence of the voltage-dependent
Na+ channel blocker TTX (1 µM). We reasoned that any action of WIN 55,212-2 on
postsynaptic sensitivity to GABA or on GABA uptake processes should be
manifested as a change in mIPSC amplitude or mIPSC kinetics. In all
cells, the efficacy of the TTX block of
Na+ channels was monitored by observing
the disappearance of the evIPSC during maximal electrical stimulation.
A complete elimination of the evoked response usually occurred within 2 min after beginning the TTX application. As shown in Figure
5, application of TTX alone reduced both
the frequency and amplitude of sIPSCs. However, the mIPSCs remaining
after TTX application were completely insensitive to WIN 55,212-2
(1-5 µM). Thus, WIN 55,212-2 did not produce a shift in
either the cumulative amplitude or cumulative interevent interval mIPSC
distributions in any of these cells (p > 0.05; Kolmogorov-Smirnov test; n = 6). Mean mIPSC amplitudes
were 9.2 ± 3.3 pA in TTX (control) versus 9.5 ± 0.5 pA
during WIN 55,212-2 application (p > 0.05;
Wilcoxon signed rank test). The average frequency of mIPSCs was
0.68 ± 0.18 Hz in TTX versus 0.61 ± 0.15 Hz during WIN
55,212-2 (p > 0.05; Wilcoxon signed rank
test).
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Figure 5.
Effect of WIN 55,212-2 on action
potential-independent (TTX-insensitive) mIPSCs in a single CA1
pyramidal neuron. Holding potential, 80 mV. A,
Traces represent portions of 2 min epochs recorded
before TTX application (Control), 10 min into the
TTX (500 nM) application, and 10 min into the WIN 55,212-2
(5 µM) application. B, Cumulative
interevent interval distributions for each treatment condition in the
same cell. A significant decrease in the frequency of events was
observed during TTX (p < 0.001; K-S test).
During WIN 55,212-2 application, no further change
(p > 0.05; K-S test) in the distribution
was observed. C, Cumulative amplitude distribution for
the same cell demonstrating a decrease in amplitude during TTX
(p < 0.001; K-S test). The mean amplitude
decreased from 12.6 pA (n = 518 events) to 8.8
pA (n = 43 events) in TTX. However, no further
change in the mean amplitude (9.3 pA; n = 56 events) was observed during WIN 55,212-2 treatment. D,
Summary of mIPSC amplitude and frequency (mean ± SEM;
n = 6) before TTX (Con, open
bars), during TTX (filled bars)
(*p < 0.05 vs control; Wilcoxon signed rank test),
and during WIN 55,212-2 (5 µM) (hatched
bars). Calibration: 25 pA, 500 msec.
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In a further attempt to identify any postsynaptic effects of WIN
55,212-2 on the sensitivity to GABA or on GABA uptake, mIPSCs were
averaged before and during WIN 55,212-2 application, and single
exponential decay time constants () were fit to these waveforms (see
Materials and Methods). During TTX alone, was 28.8 ± 2.2 msec, whereas during WIN 55,212-2 application, was 28.9 ± 3.1 msec. These values were not significantly different (n = 6; p = 0.98; paired Student's
t test). Similarly, the 10-90% rise times of mIPSCs were
not significantly affected by WIN 55,212-2 (control, 2.9 ± 0.2 msec; WIN, 2.3 ± 0.3 msec; p = 0.07; paired Student's t test; n = 6). Thus, because WIN
55,212-2 did not alter the amplitudes or kinetics of mIPSCs , it is unlikely that postsynaptic sensitivity to GABA was altered or
that GABA uptake was disrupted in these neurons.
Because the frequency of mIPSCs was significantly slower than sIPSC
frequency, we considered the possibility that our inability to observe
modulation of mIPSCs might be because of the small number of events
available to analyze in the presence of TTX. Therefore, to increase the
relative frequency of mIPSCs in the presence of TTX, we used the
polyvalent cation ruthenium red, which blocks VDCCs and enhances mIPSC
frequency via a Ca2+-independent mechanism
(Trudeau et al., 1996; Sciancalepore et al., 1998; Cibulsky and Sather,
1999). Ruthenium red (200 µM) increased mIPSC frequency
threefold to fivefold in every cell tested, which, on average, was
similar to the frequency of action potential-dependent sIPSCs (sIPSCs,
2.0 ± 0.3 Hz; TTX, 0.60 ± 0.11 Hz; ruthenium red, 2.3 ± 0.78 Hz; n = 9; data not shown). However, ruthenium
red had no effect on mIPSC amplitude (TTX, 8.6 ± 0.6 pA;
ruthenium red, 8.8 ± 0.9 pA; n = 9). Similar to the lack of effects of WIN 55,212-2 on mIPSCs, a 1 µM concentration of this agonist had no effect
on mIPSC frequency (WIN 55,212-2, 2.3 ± 0.8 Hz) or amplitude
(WIN 55,212-2, 8.5 ± 1.1 pA) in the presence of ruthenium red.
Together, the above data suggest that WIN 55,212-2 altered neither the
postsynaptic sensitivity to GABA nor its rate of clearance and that the
effects of the CB1 agonist on sIPSCs were presynaptic. Also, the
absence of CB1 receptor-mediated effects on mIPSCs was not attributable
to the smaller number of synaptic currents available for the analysis.
Effects of WIN 55,212-2 on sIPSCs in the presence of cadmium
The experiments involving TTX demonstrated that, when
voltage-dependent Na+ channels were
blocked, the effects of WIN 55,212-2 on GABA release were eliminated.
This could indicate that the presynaptic actions of WIN 55,212-2 were
attributable to either a direct action on voltage-dependent
Na+ channels or on another
voltage-dependent current activated by Na+
channel-induced depolarization. To distinguish between these possibilities, we examined the actions of WIN 55,212-2 on spontaneous IPSCs during the blockade of VDCCs by CdCl2. Bath
application of CdCl2 (200 µM)
completely eliminated the evIPSC and reduced the amplitude and the
frequency of sIPSCs (Fig. 6). However, as shown in Figure 6, application of WIN 55,212-2 (1-5 µM;
n = 6) in the presence of CdCl2
did not produce an additional shift in either the cumulative amplitude
sIPSC distribution or the interevent interval distribution in any cell
(p > 0.05; Kolmogorov-Smirnov test). The mean
sIPSC amplitudes in these experiments were 11.8 ± 1.0 pA in
CdCl2 and 11.5 ± 1.5 pA during WIN
55,212-2 (p > 0.05; Wilcoxon signed rank
test). A slight increase in the mean frequency was observed during WIN
55,212-2 treatment in these experiments (CdCl2,
0.49 ± 0.08 Hz; WIN 55,212-2, 0.63 ± 0.13 Hz), but it was
not statistically significant (p > 0.05;
Wilcoxon signed rank test). These data demonstrate that the blockade of VDCCs, like the blockade of VD Na+
channels, eliminated the CB1 receptor-mediated inhibition of GABA
release.
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Figure 6.
Effect of WIN 55,212-2 on spontaneous IPSCs in a
CA1 pyramidal neuron during CdCl2 application. Holding
potential, 80 mV. A, Traces represent
portions of 2 min epochs obtained before treatment
(Control), 10 min into CdCl2 (200 µM) application, and 13 min into WIN 55,212-2 (1 µM) application. B, Cumulative interevent
interval distribution for the same cell. CdCl2 produced a
significant increase in the interevent interval
(p < 0.001; K-S test). During WIN
55,212-2 treatment in the presence of CdCl2, there
was no further change in the distribution (p > 0.05; K-S test). C, Cumulative amplitude
distribution for the same cell reveals that CdCl2 treatment
significantly (p < 0.001; K-S test)
reduced the amplitude from control. The mean amplitude decreased from
17.9 pA (n = 241 events) in control to 13.0 pA
(n = 126 events) during CdCl2. A
significant change in the amplitude distribution was not observed
during WIN 55,212-2 application in the presence of CdCl2
(p > 0.05; K-S test; mean amplitude,
10.7 pA; n = 92 events). D,
Summary of mean ± SEM amplitude and frequency changes of sIPSCs
(n = 6) during CdCl2
(Cd) (*p < 0.05 vs control;
Wilcoxon signed rank test) and WIN 55,212-2 in the presence of
CdCl2 (WIN). Calibration: 25 pA, 500 msec.
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Effect of WIN 55,212-2 on Ca2+-dependent mIPSCs
during depolarization with KCl
The experiments described above indicated that the presynaptic
modulation of GABA release by CB1 receptors could be occluded by
blockade of either Na+ channels by TTX or
VDCCs by CdCl2. Because the activation of VDCCs
and the release of GABA are dependent on the depolarization initiated
by Na+ action potentials, we hypothesized
that TTX acted indirectly to inhibit VDCC activity and thus occlude the
effect of the CB1 agonist, whereas CdCl2 acted
directly on VDCCs to occlude this effect. However, although these
experiments supported the hypothesis that CBs inhibit GABA release by
modulating VDCC activity, they did not permit us to dismiss the
possibility of direct modulation of VD Na+
channels by WIN 55,212-2. In an effort to dissociate VDCC from VD
Na+ channel activity, we increased the
contribution of presynaptic VDCCs by directly depolarizing the
inhibitory terminals with elevated [K+]o in the
presence of TTX.
In the presence of TTX, the elevation of extracellular
K+ from 3 to 15 mM produced a
significant increase in both the amplitude (TTX, 11.8 ± 3.6 pA;
high K+, 21.6 ± 8.2 pA;
n = 6) and the frequency (TTX, 0.5 ± 0.7 Hz; high
K+, 13.7 ± 5.6 Hz; n = 6) of mIPSCs in every cell tested (p < 0.01; K-S test; n = 6), although the absolute magnitude of
the increase varied considerably from cell to cell. To confirm that
larger and more frequent mIPSCs observed in high
[K+]o were caused
by increased VDCC activity, we applied CdCl2 (200 µM). In each neuron,
CdCl2 reduced the frequency (mean, 2.5 ± 0.98 Hz; n = 6) and amplitude (18.1 ± 5.3 pA)
of the mIPSCs, suggesting that the elevated
[K+]o increased
GABA release as a result of increased VDCC activity (Fig.
7). Under conditions of elevated
[K+]o, WIN
55,212-2 (1 µM) significantly reduced the
frequency of mIPSCs to 59 ± 9% of the baseline recorded during
application of TTX and high
[K+]o (Fig. 7). In
addition, mIPSC amplitude was significantly reduced by WIN 55,212-2 in
four of six neurons (p < 0.01; K-S test).
Thus, the CB1 receptor-mediated inhibition of GABA release was restored under conditions that favored VDCC activity, during the blockade of VD
Na+ channels.
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Figure 7.
Effect of WIN 55,212-2 on mIPSCs during
depolarization of inhibitory terminals with elevated
[K+]o. Holding potential, 80 mV
using a CsCl-based internal solution. A,
Traces representing portions of 2 min epochs acquired
during the sequential administration of TTX (500 nM; in
standard 3 mM
[K+]o), elevated
[K+]o (KCl) (15 mM), WIN 55,212-2 (1 µM), and
CdCl2 (200 µM). B, Cumulative
interevent interval distribution for the same cell. WIN 55,212-2
produced a significant (p < 0.001; K-S
test) increase in the interevent interval distribution during
application of high [K+]o and TTX,
indicating a decrease in frequency. Subsequent application of
CdCl2 also resulted in a significant
(p < 0.001; K-S test) shift in the
interevent interval distribution, indicating that the direct activation
of VDCCs contributed to the enhancement of mIPSC frequency in elevated
[K+]o. C, Cumulative
amplitude distribution for the same cell. Both WIN 55,212-2 and the
subsequent application of CdCl2 produced a significant
(p < 0.001; K-S test) decrease in the
cumulative amplitude distribution relative to high
[K+]o. The mean amplitudes were as
follows: high [K+], 10.6 pA
(n = 637 events); WIN 55,212-2, 8.4 pA
(n = 367 events); and CdCl2,
7.9 pA (n = 264 events). D,
Summary of the effects of WIN 55,212-2 (WIN) (1 µM; n = 6) and CdCl2
(Cd) (200 µM; n = 6)
on the mean frequency and amplitude. Data represent the mean ± SEM and are shown as a percentage of the baseline obtained in high
[K+]o (*p < 0.05 vs baseline; Student's two-tailed t test). Although the
mean amplitude was not significantly affected, a significant
(p < 0.001; K-S test) shift in the
cumulative amplitude distribution was observed in four of six cells.
Calibration: 25 pA, 500 msec.
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Effects of K+ channel blockade on the inhibition
of evIPSCs by WIN 55,212-2
The experiments described above demonstrated that CB1 receptor
activation presynaptically reduced GABA release onto CA1 pyramidal neurons and suggested that the inhibition of VDCCs was involved. However, because CBs have also been shown to modulate voltage-dependent K+ channels
(IA) in hippocampal pyramidal neurons
(Deadwyler et al., 1995) and voltage-independent
K+ channels in cellular expression systems
(Mackie et al., 1995; Jin et al., 1999), we sought to assess the
potential role of presynaptic K+ channels
in the CB1 receptor-mediated inhibition of GABA release. Recordings
were performed on neurons voltage clamped at 45 to 55 mV using a
K+-gluconate-based internal solution (see
Materials and Methods), and K+ channels
were blocked by either BaCl2 (300 µM) or 4-AP (100 µM). Evoked IPSC amplitudes and durations were increased by both
BaCl2 (amplitudes, 138 ± 10% of control;
n = 9) and 4-AP (amplitudes, 148 ± 15% of
control; n = 9) (Fig. 8).
Application of WIN 55,212-2 (1 µM) failed to
reduce the evIPSC in the presence of either of the
K+ channel blockers (Fig. 8). However,
because the blockade of presynaptic K+
channels is known to delay repolarization of the synaptic terminal and
thereby prolong the presynaptic action potential (for discussion, see
Lupica and Dunwiddie, 1993), it was likely that
Ca2+ influx into the terminal was
increased and that the GABA release process was saturated. Because this
shift in the Ca2+ dependence of GABA
release might confound our ability to observe modulation by the CB1
receptor agonist, we sought to "normalize" this action by lowering
[Ca2+]o to
generate evIPSCs that were similar in amplitude to those observed
before K+ channel blockade. Thus, after
BaCl2 (n = 3) or 4-AP
(n = 4) application, the
Ca2+ concentration was adjusted to between
1.5 and 2.0 mM (from 2.4 mM, with corresponding
Mg2+ levels increased to maintain
osmolarity). This manipulation reduced the evIPSC to 70-100% of
control levels. As shown in Figure 8, in the presence of
BaCl2 or 4-AP and under conditions of lowered Ca2+, the ability of WIN 55,212-2 (1 µM) to reduce evIPSCs was not changed compared
with its effect in the absence of these manipulations (p > 0.05 vs 1 µM WIN
55,212-2 alone; one-way ANOVA). This suggests that CB1 receptor
activation did not inhibit IPSCs through the modulation of 4-AP- and
BaCl2-sensitive K+
channels.
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Figure 8.
Effect of K+ channel blockade
on WIN 55,212-2-mediated inhibition of evoked
GABAA-mediated IPSCs in CA1 pyramidal neurons. Recordings
were performed using a K+-gluconate-based electrode
solution at a holding potential of 45 to 55 mV. A,
Under standard conditions (2.4 mM
CaCl2), BaCl2 (300 µM)
(top traces) and 4-AP (100 µM)
(bottom traces) produced a large increase in the IPSC.
Application of WIN 55,212-2 (1 µM) in the presence of
BaCl2 or 4-AP failed to cause a significant reduction in
the IPSC. B, Under conditions in which the extracellular
Ca2+ was reduced to 1.2-2.0 mM after
BaCl2 (top trace) or 4-AP (bottom
trace) application, WIN 55,212-2 reduced the IPSC.
C, Summary of the effects of WIN 55,212-2 (1 µM) in the presence of BaCl2 (300 µM) or 4-AP (100 µM) under either standard
(open bars) or low Ca2+
(hatched bars) aCSF. Data represent the mean ± SEM
of the number of cells given in parentheses. The horizontal
dashed lines represent the effect of 1 µM WIN
55,212-2 on GABAA IPSCs in standard aCSF without
BaCl2 or 4-AP (mean ± SEM; n = 4).
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DISCUSSION |
The present study demonstrates that the CB1 agonist WIN 55,212-2
acted presynaptically to inhibit GABA release onto
GABAA receptors in the CA1 region of the
hippocampus. This was in contrast to the actions of this CB1 agonist on
GABAB-mediated synaptic transmission, which was
not affected at a concentration of WIN 55,212-2 that maximally
inhibited GABAA-mediated IPSCs. In addition, this
electrophysiological analysis permitted the exclusion of possible
postsynaptic effects of WIN 55,212-2 on the postsynaptic sensitivity
to GABA, GABA uptake (Maneuf et al., 1996), and the indirect modulation
of GABA release via the activation of opioid receptors (Tanda et al.,
1997). We also provide evidence that the CB1 receptor inhibition of
GABAA-mediated synaptic transmission likely
occurs through the inhibition of VDCCs and probably not through
alterations in Na+ or
K+ channel activity. These results thereby
extend those demonstrating that CB1 receptors were located on the
inhibitory terminals of hippocampal interneurons and that
K+-stimulated
[3H]GABA release was modulated by WIN
55,212-2 (Katona et al., 1999).
Although the adverse affects of marijuana on memory and cognitive
function have long been ascribed to its actions in the hippocampus (Drew and Miller, 1974; Miller and Branconnier, 1983; Essman, 1984;
Hampson and Deadwyler, 1998), the description of CB binding sites in
this brain region has provided strong corroborative evidence in favor
of this hypothesis (Herkenham et al., 1990; Howlett et al., 1990;
Breivogel and Childers, 1998). Furthermore, the development of potent
ligands for the CB1 receptor has provided a means to directly assess
the effects of CBs in the CNS (Pertwee, 1997). One of the hallmarks of
CNS CB function that has emerged from these studies is that activation
of CB1 receptors can presynaptically inhibit fast synaptic transmission
in a variety of brain regions. Thus, CB1 agonists can inhibit
glutamatergic transmission in the cerebellum (Levenes et al., 1998) and
the hippocampus (Shen et al., 1996; Misner and Sullivan, 1999;
Sullivan, 1999), whereas GABAergic synaptic transmission is inhibited
by CBs in the substantia nigra (Chan et al., 1998), the striatum (Szabo
et al., 1998), the medulla (Vaughan et al., 1999), and the hippocampus
(present study).
CB1 receptors modulate GABAA- but not
GABAB-mediated synaptic responses
The present study demonstrated that WIN 55,212-2 inhibited evoked
GABAA receptor-mediated IPSCs in a
concentration-dependent manner, without affecting
GABAB-mediated IPSCs. The differential modulation
of GABAA and GABAB synapses
by monoamine receptor agonists has been shown previously in midbrain
dopamine neurons (Johnson et al., 1992; Cameron and Williams, 1993;
Shoji et al., 1999). However, it is not clear whether
GABAA and GABAB synaptic
responses arise from different populations of inhibitory terminals in
the hippocampus (Nurse and Lacaille, 1997). Our results support the hypothesis that the innervation of GABAA and
GABAB receptors arises from distinct inhibitory
terminals and are consistent with the idea that CB1 receptors are found
on inhibitory basket cell terminals (Katona et al., 1999) that
constitute a major source of GABAA-mediated synaptic input onto CA1 pyramidal neuron somata (Buhl et al., 1995).
This differential targeting of inhibitory terminals by CB1 receptors is
in contrast to µ-opioid receptors, which inhibit both
GABAA- and GABAB-mediated
synaptic transmission in the hippocampus (Lupica et al., 1992).
Our estimated EC50 value for WIN
55,212-2-mediated inhibition of GABAA IPSCs (138 nM) is in reasonable agreement with the values of 41 nM for inhibition of
[3H]GABA release (Katona et al., 1999)
and 30 nM for inhibition of
[3H]acetylcholine release in hippocampal
slices (Gifford and Ashby, 1996). In agreement with previous data
(Collins et al., 1995; Katona et al., 1999), the effect of WIN
55,212-2 was completely blocked by the CB1 antagonist SR141716A.
However, the lack of an effect of SR141716A alone on evoked IPSCs
suggests that endogenous CBs do not modulate ongoing GABAergic synaptic
transmission under basal conditions in hippocampal slices (Katona et
al., 1999). In addition, the inability of naloxone to significantly
alter the effect of WIN 55,212-2 indicates that CB1 receptors did not reduce GABA release through either the direct activation of opioid receptors or the stimulation of endogenous opioid release in the hippocampus. This is in contrast to studies showing that such a
mechanism exists for the CB-induced increase in dopamine release in the
nucleus accumbens (Chen et al., 1990; Tanda et al., 1997).
The effects of CB1 receptors on GABAergic transmission
are presynaptic
Several experiments were performed to determine whether the effect
of WIN 55,212-2 on GABAergic neurotransmission was presynaptic. First,
we compared the effects of WIN 55,212-2 on action potential-dependent sIPSCs with its effects on action potential-independent mIPSCs. These
results showed that sIPSCs were inhibited by WIN 55,212-2, and that
mIPSCs were completely unaffected. Thus, postsynaptic changes in the
sensitivity to GABA or a change in mIPSC kinetics caused by a slowing
of the rate of uptake of GABA were not observed (Maneuf et al., 1996).
Second, the elimination of the effects of WIN 55,212-2 on spontaneous
IPSCs by the VDCC blocker CdCl2 also indicated
that the effects of the agonist were presynaptic. Changes in mIPSC
frequency are often used to demonstrate the modulation of transmitter
release through direct actions on nerve terminals (Cohen et al., 1992;
Thompson et al., 1993; Lupica, 1995; Manzoni and Williams, 1999).
However, dissociation of the effects of neuromodulators on sIPSCs and
mIPSCs can also provide evidence for a presynaptic mechanism of action,
because the loss of a drug effect in the presence of TTX may indicate
that some action potential-dependent process in the presynaptic neuron
was required to observe the modulation (Miller et al., 1997).
Mechanism of presynaptic inhibition of GABA release by
CB1 receptors
Despite providing evidence in support of a presynaptic mechanism
for WIN 55,212-2, the analysis of sIPSCs and mIPSCs did not distinguish among the several possible ion channel targets of CB1
receptors. Because somatic VDCCs (Shen and Thayer, 1998; Sullivan, 1999) and VDKCs (Deadwyler et al., 1995) have been implicated in the
effects of the CBs, we hypothesized that at least one of these classes
of ion channels was modulated by WIN 55,212-2. We reasoned that the
block of the effect of WIN 55,212-2 by TTX indicated that CB1
receptors inhibited Na+ channels directly
or that CB1 receptors inhibited VDCCs or VDKCs that were activated by
the Na+ channel-dependent depolarization.
Our hypothesis that the inhibition of GABA release occurred as a result
of the inhibition of VDCCs was derived from the observations that (1)
the inhibitory effect of WIN 55,212-2 on sIPSCs was also eliminated
when VDCCs "downstream" of Na+
channels were blocked by CdCl2, and (2) the
effect of WIN 55,212-2 on sIPSCs was restored when inhibitory
terminals were depolarized and VDCCs activated directly by elevated
[K+]o during
Na+ channel blockade with TTX. However,
because distinct classes of VDCCs are known to differentially
inactivate according to the level of sustained depolarization, the
VDCCs that were recruited by elevated
[K+]o may
represent only a subset of the VDCCs activated by a brief depolarization, such as that initiated by an action potential (Doze et
al., 1995). Nevertheless, our results clearly demonstrate that
elevating [K+]o
recruited VDCCs that could support GABA release and that these channels
were sensitive to inhibition by both CdCl2 and
WIN 55,212-2. Thus, although these data do not conclusively establish
which VDCCs were involved in this process, they do support the
hypothesis that GABA release is inhibited by CB1 receptor modulation of
VDCCs. In this way, the modulation of presynaptic VDCCs in the
inhibition of GABA release is similar to that described for the
CB1-mediated inhibition of glutamate release in hippocampal cultures
(Twitchell et al., 1997; Sullivan, 1999).
Although the inhibition of VDCCs represents a likely mechanism for the
CB1-mediated inhibition of synaptic GABA release, these experiments did
not eliminate the possibility that WIN 55,212-2 may also act on
presynaptic K+ channels. This mechanism
was important to evaluate because K+
channels have been implicated as targets in the actions of other presynaptic modulators of neurotransmitter release (Simmons and Chavkin, 1996; Vaughan et al., 1997). Furthermore, the CB1 receptor is
known to activate voltage-dependent K+
channels (IA) in hippocampal neurons
(Deadwyler et al., 1993, 1995) and voltage-independent, GIRKs in
cellular expression systems (Mackie et al., 1995; Matsuda, 1997; Garcia
et al., 1998; Jin et al., 1999). Therefore, we assessed the effect of
blockade of the IA-like channel with
4-AP and the GIRK channel with BaCl2 on the
modulation of evIPSCs by WIN 55,212-2. Although both
BaCl2 and 4-AP appeared to block the inhibition
of evIPSCs by WIN 55,212-2 at physiological concentrations of
Ca2+ (2.4 mM), an
important caveat must be considered. Because blockade of presynaptic
K+ channels prolongs the depolarization of
the nerve terminal, Ca2+ influx is
enhanced (Fig. 8). This increase in intraterminal
Ca2+ can then "saturate" the
neurotransmitter release process (Lupica and Dunwiddie, 1993),
confounding the observation of the inhibition of evoked IPSCs,
particularly if VDCCs are indeed modulated. In support of this
hypothesis, the inhibitory effect of WIN 55,212-2 on evIPSCs was
restored when
[Ca2+]o was
lowered (1.5-2.0 mM) during
BaCl2 or 4-AP treatment. Thus, we conclude that
neither 4-AP nor BaCl2 blocked the modulation of
evIPSCs by WIN 55,212-2. In this respect, our data are similar to
previous studies demonstrating that the ability of 4-AP to reduce
presynaptic inhibition by adenosine could be reversed by decreasing
[Ca2+]o (Klapstein
and Colmers, 1992) or by increasing
[Mg2+]o (Lupica
and Dunwiddie, 1993).
Conclusions
The GABAergic interneurons of the hippocampus play a critical role
in the synchronization of pyramidal cell activity and thereby contribute to oscillatory patterns, such as theta rhythm, that are
important in the encoding of spatial and sensory information (O'Keefe,
1993; Cobb et al., 1995; Buzsáki, 1997; Paulsen and Moser, 1998).
Presynaptic inhibition of GABA release by CBs would therefore be
expected to interfere with this synchronization, perhaps explaining the
disruptive effects of marijuana on spatial memory and learning tasks
(Heyser et al., 1993; Ameri, 1999). Our observation that CBs
differentially modulate GABAergic synapses, together with the fact that
CBs also inhibit glutamatergic transmission in the hippocampus (Shen et
al., 1996; Misner and Sullivan, 1999), suggests that the activation of
CB1 receptors is likely to have complex effects on hippocampal
circuitry. It remains to be determined whether inhibitory or excitatory
synapses display differential sensitivity to CBs or whether the
specific Ca2+ channels differ between
these populations of synapses. Despite these unresolved issues, it is
apparent that the adverse effects of marijuana on cognitive processes
are attributable in part to actions on fast synaptic transmission in
the hippocampus.
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FOOTNOTES |
Received Nov. 30, 1999; revised Jan. 14, 2000; accepted Jan. 18, 2000.
This work was supported by the Intramural Research Program of the
National Institute on Drug Abuse, National Institutes of Health. We
thank Dr. James A. Bell for his assistance in analyzing the data and in
helpful discussions on this manuscript.
Correspondence should be addressed to Dr. Carl R. Lupica, National
Institute on Drug Abuse, Intramural Research Program, Building C, Room
267, 5500 Nathan Shock Drive, Baltimore, MD 21224. E-mail: clupica{at}intra.nida.nih.gov.
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T. Ohno-Shosaku, H. Tsubokawa, I. Mizushima, N. Yoneda, A. Zimmer, and M. Kano
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R. I. Wilson and R. A. Nicoll
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Q. Li, S. Clark, D. V. Lewis, and W. A. Wilson
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T. Yoshida, K. Hashimoto, A. Zimmer, T. Maejima, K. Araishi, and M. Kano
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M. A. Diana, C. Levenes, K. Mackie, and A. Marty
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TOP
ABSTRACT
INTRODUCTION
