Modulation of Synaptic GABAA Receptor Function by PKA and PKC in Adult Hippocampal Neurons

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The Journal of Neuroscience, January 15, 1999, 19(2):674-683

Modulation of Synaptic GABA_A Receptor Function by PKA and PKC in Adult Hippocampal Neurons
Pierrick Poisbeau², Michael C. Cheney¹, Michael D. Browning³, and Istvan Mody¹
¹ Departments of Neurology and Physiology, University of California at Los Angeles, School of Medicine, Los Angeles, California 90095, ² Laboratoire de Neurophysiologie Cellulaire et Intégrée, Centre National de la Recherche Scientifique UMR 7519, Université Louis Pasteur, 67084 Strasbourg, France, and ³ Department of Pharmacology, University of Colorado Health Science Center, Denver, Colorado 80262

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Several protein kinases are known to phosphorylate Ser/Thr residues of certain GABA_A receptor subunits. Yet, the effect ofphosphorylation on GABA_A receptor function in neurons remainscontroversial, and the functional consequences of phosphorylatingsynaptic GABA_A receptors of adult CNS neurons are poorly understood.We used whole-cell patch-clamp recordings of GABA_A receptor-mediatedminiature IPSCs (mIPSCs) in CA1 pyramidal neurons and dentategyrus granule cells (GCs) of adult rat hippocampal slices to determinethe effects of cAMP-dependent protein kinase (PKA) and Ca²⁺/phospholipiddependent protein kinase (PKC) activation on thefunction of synaptic GABA_A receptors. The mIPSCs recorded in CA1pyramidal cells and in GCs were differentially affected by PKAand PKC. In pyramidal cells, PKA reduced mIPSC amplitudes andenhanced the fraction of events decaying with a double exponential,whereas PKC was without effect. In contrast, in GCs PKA was ineffective,but PKC increased the peak amplitude of mIPSCs and also favoreddouble exponential decays. Intracellular perfusion of the phosphataseinhibitor microcystin revealed that synaptic GABA_A receptors ofpyramidal cells, but not those of GCs, are continually phosphorylatedby PKA and conversely, dephosphorylated, most likely by phosphatase1 or 2A. This differential, brain region-specific phosphorylationof GABA_A receptors may produce a wide dynamic range of inhibitorysynaptic strength in these two regions of the hippocampalformation.

Key words: GABA_A; miniature IPSCs; phosphorylation; receptors; PKA; PKC

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Phosphorylation of ligand-gated ion channels is an important short- and long-term regulatory mechanism of channel functionin the CNS (Levitan, 1994; Sigel, 1995; Moss and Smart, 1996).In the process of long-term potentiation (LTP) of synaptic transmission,experimental evidence strongly supports a critical role of proteinkinases (for review, see Raymond et al., 1993; Soderling, 1995;McEachern and Shaw, 1996; Barria et al., 1997). A recent study(Barria et al., 1997) has directly demonstrated the phosphorylationof AMPA-type glutamate receptors (GluRs) by type II Ca²⁺/calmodulin kinase afterLTP.

In contrast to the familiar plasticity of excitatory amino acid receptors through phosphorylation, fewer studies implicatethis process in altering the efficacy of GABAergic synaptic transmission.In Purkinje cells, repetitive stimulation of climbing fibers inducesa rebound potentiation of GABA_A receptor (GABAR) function (Kanoet al., 1996). This potentiation has been attributed to elevatedpostsynaptic Ca²⁺ levels over 10-30 min, possibly leading to protein phosphorylation.Various cells when deprived of intracellular ATP by omitting itfrom the patch pipette commonly respond by downregulating GABARfunction (Raymond et al., 1993; Sieghart, 1995; Moss and Smart,1996). Most studies examined whole-cell currents evoked by GABAin expression systems, but a rundown of GABAR-mediated synapticcurrents has been noted in central neurons (Lewis and Faber, 1996).

Biochemical approaches demonstrated that some native and many recombinantly expressed GABARs can be phosphorylated directlyand consequently can be functionally modulated by cAMP-dependentkinase (PKA) (Heuschneider and Schwartz, 1989; Tehrani et al.,1989; Browning et al., 1990; Porter et al., 1990; Leidenheimeret al., 1991; Moss et al., 1992a,b; Angelotti et al., 1993; Browninget al., 1993), Ca²⁺/phospholipid-dependent protein kinase (PKC) (Sigel and Baur,1988; Browning et al., 1990, 1993; Sigel et al., 1991; Leidenheimeret al., 1992; Krishek et al., 1994; Lin et al., 1994; Chang etal., 1996; Weiner et al., 1997), type II Ca²⁺/calmodulin-dependent protein kinase (Machu et al., 1993; McDonaldand Moss, 1994, 1997), or protein tyrosine kinase (Moss et al.,1995; Wan et al., 1997). In general, phosphorylation of Ser/Thrresidues on GABAR subunits by PKC and PKA is believed to decreaseGABAR function (Sigel, 1995; Moss and Smart, 1996), although somereports show an increase in GABA_A receptor-mediated whole-cellcurrents by PKC (Lin et al., 1994) and PKA (Cheun and Yeh, 1992;Angelotti et al., 1993; Cheun and Yeh, 1996). Tyrosine phosphorylationseems to be involved in either potentiating or maintaining GABAR-mediatedinhibition (Moss et al., 1995; Wan et al., 1997; Huang and Dillon,1998).

Unfortunately, the precise subunit composition of synaptic GABARs as well as the local enzymatic machinery are not known.Therefore, no accurate predictions can be made about the effectof phosphorylation on the modulation of GABAR-mediated synaptictransmission. With the exception of a recent study showing alteredIPSCs in cultured neurons after inhibition of the Ca²⁺/CaM-dependent phosphatase calcineurin (Jones and Westbrook, 1997),there is no compelling evidence demonstrating the impact of phosphorylationon synaptic GABARfunction.

We have investigated the postsynaptic effects of PKA and PKC in CA1 pyramidal cells and granule cells (GCs) of adult hippocampalslices using intracellular delivery of nonpermeant peptides andcatalytic kinases. By recording mIPSCs in fully developed centralneurons, we could focus on the modulation of synaptic GABAR functionby PKA- and PKC-dependentphosphorylation.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Slice preparation and solutions. Coronal slices were prepared from Wistar rats (350-400 gm) as described previously (Staleyet al., 1992; Poisbeau et al., 1997). Briefly, after pentobarbitalanesthesia (75 mg/kg, i.p.), animals were decapitated, and thebrain was quickly removed and immersed for 1-2 min in cold (6-9°C)artificial CSF (ACSF) containing (in mM): 126 NaCl, 2.5 KCl, 2CaCl₂, 2 MgCl₂, 1.25 NaH₂PO₄, 10 D-glucose, 26 NaHCO₃, 2 kynurenicacid (Fluka) continuously bubbled with 95% O₂/5% CO₂, pH 7.35± 0.05. The brain was glued at its frontal surface to a brassplatform, and coronal brain slices (450 µm thick) were preparedwith a Vibratome (Lancer Series 1000). The slices were then hemisectedand stored submerged in 2 mM kynurenic acid containing ACSF at32°C until they were individually transferred to the recordingchamber. Recordings were performed at 34-35°C with slices immobilizedwith a piece of lens paper and two small platinum weights. Duringeach recording, 1 µM tetrodotoxin (Calbiochem) was added to theACSF in the continued presence of the nonspecific glutamate receptorantagonist kynurenic acid (2 mM).

With the exception of Rp-8-CPT-cAMPS, the compounds used to alter cellular phosphorylation events were membrane-impermeantpeptides. PKC and PKA were isolated and purified from bovine brainas described previously (Browning et al., 1990). Only constitutivelyactive catalytic subunits of these kinases were used. The catalyticsubunit of PKA was purified from bovine heart as described previously(Browning et al., 1990). The catalytic fragment of PKC was preparedfrom bovine brain PKC as described previously (Wang et al., 1994).PKA-I (H₂N-TYADFIASGRTGRRNAI-amide) was a generous gift of Dr.John Haycock. PKA, PKC, inactivated PKC, PKA inhibitor, and microcystinhave been diluted 50-1000 times when incorporated into the intracellularsolution. Microcystin-LR (Calbiochem, La Jolla, CA) and Rp-8-CPT-cAMPSwere first prepared as 1000-fold concentrated stock solutionsin DMSO. PKA (0.3 mg/ml) and the PKA inhibitory peptide (PKA-I;0.33 mM) were initially prepared in the following buffer solution(in mM): 100 NaCl, 20 MES, pH 6.5, 30 $beta$ -mercaptoethanol, 0.1 EDTA,and 50% ethylene glycol solution; PKC (0.3 mg/ml) was preparedin a solution consisting of the following (in mM): 2 TEA, 5 EGTA,6 MgCl₂, 140 KCl, 1 CaCl₂, adjusted to pH 7.5 with KOH. An equivalentdilution of the buffer alone, when perfused into the cytoplasmof GC or CA1 neurons, did not produce any changes of GABA_AmIPSCs.

Whole-cell recordings and data collection. Whole-cell voltage-clamp recordings were obtained using borosilicate glass capillarieswith an inner filament (KG-33, 1.12 mm inner diameter, 1.5 mmouter diameter; Garner Glass) pulled to tip diameters of ~1.5µm in two stages using a vertical puller (Narishige PP-83). Intrapipettesolutions contained the following (in mM): 130 CsCl, 2 MgCl₂,10 HEPES, 0.8 CsOH, 2 MgATP (pH was adjusted with CsOH; totalosmolarity 255-285 mOsm). Recordings were obtained by loweringpatch electrodes into the CA1 and/or dentate granule cell layerwhile monitoring current responses to 5 mV voltage pulses andapplying suction to form >G $Omega$ seals. An Axopatch-200A amplifier(Axon Instruments) was used, and series resistance (R_s) was compensatedby 70-90% (lag value, 7-10 µsec). The value of R_s was monitoredthroughout each experiment, and only recordings with R_s < 15 M $Omega$ lasting >20 min were considered acceptable for analysis. Recordedmembrane currents were filtered (DC to 10 kHz, Bessel filter ofthe amplifier), digitized in a pulse-code-modulated form (88 kHz;Neurocorder, Neurodata), and stored on videotape. Off-line, recordingswere filtered (DC to 3 kHz; $-$ 3 dB, eight-pole Bessel filter; FrequencyDevices 9002) and sampled at 20 kHz on an Intel-Pentium-basedcomputer. Data were acquired and analyzed using the StrathclydeElectrophysiology software (courtesy of Dr. J. Dempster, U. ofStrathclyde, Glasgow, UK) and our own software designed by Y.De Koninck and I.Mody.

Event detection and selection. Detection of individual mIPSCs was performed using a software trigger described previouslyin detail (Otis and Mody, 1992; Soltesz et al., 1995). More than95% of events that satisfied the trigger criteria were detected,even during compound mIPSCs. For each experiment, all detectedevents were examined, and any spurious noise that triggered thedetector wasrejected.

Statistical analyses and curve fitting. The mean values of the median conductances, decay time constants, and frequenciesof mIPSC occurrence were compared between groups using ANOVA.Decay time constants of mIPSCs were fitted using a simplex-basednonlinear least square method; goodness of fit was evaluated onthe basis of fitting subsets of points drawn from the whole setof data points, from evaluation of the reduced $chi$ ² values, and from the change in the F values calculated by dividingthe percentage reduction in the sum of squares by the percentagechange in the number of degrees of freedom used for fitting (Solteszand Mody, 1995; Williams et al., 1998). The conductance of mIPSCsis represented graphically in cumulative probability plots drawnon a probability scale ordinate. All numerical data are expressedas mean ±SD.

Simulation of mIPSCs. Simulations of mIPSCs were performed using the SCoP software (Simulation Resources, Berrien Springs,MI) according to a model based on that published by Jones andWestbrook (1995). For monoexponentially decaying mIPSCs, the modelincluded two equal and independent GABA-binding steps, and a double-ligandedopen state. The maximum open probability at the peak of IPSCs(P_MAX) was taken to be 0.8-0.85 (Auger and Marty, 1997), a valuesimilar to that derived by nonstationary noise analysis at hippocampalinhibitory synapses (De Koninck and Mody, 1994). The reportedparameters represent the values producing the best fits to theexperimentaldata.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Characteristics of GABAR-mediated mIPSCs in CA1 pyramidal cells and GCs

GABAR-mediated mIPSCs were recorded from CA1 neurons and GCs with CsCl-containing electrodes (E_Cl = 0 mV) at holding potentialsaround $-$ 60 mV in the presence of kynurenic acid (2 mM) and tetrodotoxin(1 µM).

Under these recording conditions, mIPSCs of CA1 neurons had fast rise times (10-90% rise time <0.8 msec) and predominantlymonoexponential decays (Table 1, Fig. 1). However, a subpopulationof mIPSCs (~6%) was better fit by a biexponential decay function(Table 1). This fraction of biexponentially decaying mIPSCs wasnot significantly changed in CA1 neurons in recordings with CsMeSO₄-containingelectrodes (E_Cl $congruent$ $-$ 55 mV) at a holding potential around 0 mV (n= 8; data not shown). The fast component (fast decay time constant, $tau$ _{BIEXP FAST}) accounted for 40% of the mIPSC amplitude. At negativeholding potentials ( $-$ 60 mV), mIPSC amplitudes ranged between 10and 150 pA, with a mean conductance (mIPSG) of 0.79 ± 0.08 nS(n = 19). Because the mIPSG histograms were skewed [data not shown,but see Otis and Mody (1992)], we used the median values of thedistributions obtained from the cumulative probability graphs(Table 1). No correlations were found between the 10-90% risetimes, decay time constants (monoexponential, biexponential fastor slow), and mIPSC amplitudes. Biexponentially and monoexponentiallydecaying mIPSCs had similar median amplitudes and total areas.The frequency of GABAR-mediated mIPSCs was ~20 Hz (Table 1).GABAR-mediated mIPSCs recorded from GCs displayed similar kinetics(Table 2, Fig. 2) but occurred with a significantly lower frequency(~10 Hz) (Table 2).


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Table 1. Summary of mIPSC characteristics recorded in CA1 pyramidal cells (indicated by n in each case) after intracellular perfusion of PKA, PKC, microcystin, and PKA-I peptide

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Figure 1. Effects of protein kinase A (PKA) and protein kinase C (PKC) on mIPSCs recorded in CA1 pyramidal cells. A, Representative recordings (2.5 sec in total) depicting mIPSCs recorded with control intracellular solutions (left) and with 6 µgm/ml PKC (middle) or 6 µgm/ml PKA (right) in the patch pipette. Note the reduced mIPSCs amplitudes in the presence of PKA. B, The left panel shows cumulative probability distributions of mIPSC peak conductances under the three different experimental conditions. Compared with control (thin line; n = 393 mIPSCs), PKA (thick line; n = 525 mIPSCs) shifted the conductance distribution to the left in a roughly parallel manner, indicating a reduction in mIPSCs amplitude. PKC (thick line; n = 278 mIPSCs) had no significant effect compared with control. Right panel represents log-binned (10 bins/decade) interevent intervals plotted on a square root ordinate. The mean frequency in control (circles; n = 393 mIPSCs) was 22.4 Hz, compared with 22.2 Hz with intracellular PKA (triangles; n = 525 mIPSCs) and 25.9 Hz with intracellular PKC (diamonds; n = 278 mIPSCs). Fitted lines are fitted exponential probability density functions illustrating the random occurrence of mIPSCs. C, Representative examples of monoexponentially and biexponentially decaying mIPSCs. Each trace represents an average of 25 mIPSCs. The decay time constants were unaltered after dialysis of PKC. However, intracellular perfusion of PKA produced a significant increase in the fraction of biexponentially decaying mIPSCs (20.6 ± 4.8%) compared with control (5.9 ± 0.5%) or PKC (5.8 ± 1.8%).


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Table 2. Summary of mIPSC characteristics recorded in GCs (indicated by n in each case) after intracellular perfusion of PKA, PKC, and microcystin

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Figure 2. Effects of protein kinase A (PKA) and protein kinase C (PKC) on mIPSCs recorded in dentate gyrus granule cells. A, Raw traces (2.5 sec in total) of mIPSCs recorded with control intracellular solutions (left) and with solutions containing 6 µgm/ml PKC (middle) or 6 µgm/ml PKA (right) in the patch pipettes. Note the increased incidence of large amplitude mIPSCs in the recording with a PKC-containing pipette. B, The left panel shows the cumulative probability distribution of mIPSC peak conductances. The effect of PKA on the conductance distribution (thick left trace; n = 245 mIPSCs) is not significantly different from control (thin trace; n = 324 mIPSCs). PKC (thick right trace; n = 403 mIPSCs) elicited a marked increase in larger amplitude mIPSCs compared with control. Right panel shows log-binned (10 bins/decade) interevent intervals plotted on a square root ordinate. The mean frequency of mIPSCs under control conditions was 8.4 Hz (circles; n = 324 mIPSCs), compared with 8.3 Hz with PKA (triangles; n = 245 mIPSCs) and 8.8 Hz with PKC (diamonds; n = 403 mIPSCs) in the pipette. Fitted lines are exponential probability density functions illustrating the random nature of mIPSCs. C, Illustration of monoexponentially (top left, middle, and right traces) and biexponentially decaying mIPSCs (lower left, middle, and right traces). Each trace is an average of 25 mIPSCs. In the presence of PKC and PKA, the single or double exponential decay time constants were similar to control values. However, PKC was found to increase the fraction of biexponentially decaying mIPSCs to 24.4 ± 7.8% of total, compared with control (5.2 ± 0.9% of total) or intracellular PKA conditions (6.8 ± 3.3% of total).

Intracellular PKA reduces the amplitude of mIPSCs in CA1 neurons

We first compared mIPSC properties between CA1 neurons recorded with different intracellular solutions: mIPSCs recorded incells with control solutions were compared with events recordedwhen the patch pipette was filled with similar solutions alsocontaining constitutively active PKA or PKC. Intracellular PKA(0.6 or 6 µgm/ml) in CA1 neurons produced a dose-dependent decreaseof mIPSC conductance ( $-$ 19.8 and $-$ 39.6%, respectively) (Table 1,Fig. 1), as well as a threefold increase in the fraction of biexponentiallydecaying mIPSCs. The reduction in amplitude affected the wholepopulation of mIPSCs as shown in Figure 1B (left panel), wherea parallel shift of the amplitude distribution is evident. Nochanges in mIPSC kinetics (rise time, decay) or frequency (Fig.1B, right panel) were detected (Table 1).

The properties of mIPSCs in CA1 neurons were unaltered by inclusion of PKC (0.6 or 6 µgm/ml) in the patch pipette (Table 1,Fig. 1). This did not stem from the ineffectiveness of the perfusedPKC, because we regularly observed a progressive reduction ofthe holding current during the first 5 min of recordings withPKC in the electrode (data not shown; n = 8). This was never seenin control recordings or during perfusion with inactive PKC (n= 4). The change in the holding current most likely results fromthe effect of PKC on the hyperpolarization-activated Cl current through ClC2 channels known to be present in CA1 pyramidalcells (Smith et al., 1995). This was further corroborated by ourfinding that in recordings with CsMeSO₄ in the pipette (n = 7;E_Cl $congruent$ $-$ 56 mV), at positive holding potentials (+20 mV) where thereshould be no ClC2 current (Smith et al., 1995), PKC did not alterthe holding current and had no effect onmIPSCs.

Intracellular PKC increases the amplitude of mIPSCs in dentate gyrus granule cells

Using the same protocol as for CA1 pyramidal cells, we compared the effects of intracellular PKA and PKC on mIPSCs recordedin GCs. PKC (0.6 or 6 µgm/ml) increased mIPSG by 13.6% withoutaffecting mIPSC frequency, 10-90% rise time, or decay time constants(Table 2, Fig. 2). As shown in Figure 2B, the increase of mIPSCamplitude only occurred in a subset (60-80%) of the total populationof mIPSCs with a conductance >0.5 nS (Fig. 2B, left panel). Wealso observed a fourfold increase in the proportion of biexponentiallydecaying mIPSCs (Table 2, Fig. 2C). In GCs perfused with heat-inactivatedPKC (n = 4), mIPSCs had characteristics similar to those foundin control neurons. PKA (6 µgm/ml) failed to have any effect onthe mIPSC recorded in GCs (Table 2, Fig. 2).

Simulations of the effects of phosphorylation on GABAR-mediated mIPSCs

GABAR-mediated mIPSCs were simulated according to a seven-state model (Macdonald and Olsen, 1994; Jones and Westbrook, 1995).We found the simplest model to accurately describe the experimentallyobserved mainly monoexponentially decaying mIPSCs to be a subsetof four states of the original model (Fig. 3). The inclusion ofan additional open state was sufficient to describe the biexponentiallydecaying mIPSCs. Additional desensitized states (Jones and Westbrook,1995) did not substantially improve the fit of our simulationsto the experimental data. We next compared the fitted parametersfor simulated CA1 mIPSCs during PKA dialysis and control conditions.Although the fits are by no means unique, certain trends in thevalues of the rate constants (see Table in Fig. 3) are consistentwith previously reported PKA effects on GABARs. For example, single-channelstudies from spinal neurons have shown that PKA decreases themean open time, increases the mean closed time, and decreasesopen probability (Porter et al., 1990). Our model shows at leasta qualitative agreement with the increase in mean closed time(1/ $beta$ 2; Table in Fig. 3) and a decrease in maximum open probabilityat peak (from 0.85 to 0.50). The accurate simulation of the PKAeffect also required the GABA binding rate to be altered. Thismay be warranted in light of the possible effect of phosphorylationon GABA potency, corresponding to a change in binding and unbindingrates (Porter et al., 1990).

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Figure 3. Modeling of monoexponentially and biexponentially decaying mIPSCs. Monoexponentially (A) and biexponentially (B) decaying events were simulated using the models depicted in the left panels (one or two open state). Right panels show the results of simulations with the fitted curves superimposed over the averages of 25 mIPSCs. The y-axis represents open probability, with data normalized to a p_open of 0.85 at the peak of the mIPSC. The table gives the parameters used to simulate the various events.

Continuous regulation of synaptic GABAR function by phosphorylation/dephosphorylation in CA1 neurons

Intracellular perfusion of protein kinases and their constitutively active derivatives is useful to establish whether phosphorylationby the given kinase has any effect on cellular functions. However,a positive finding with a kinase does not necessarily prove theinvolvement of the given kinase in the physiological regulationof channel function. A positive effect of a phosphatase inhibitoris a more convincing and unequivocal evidence for the physiologicalinvolvement of the phosphorylation/dephosphorylation process.If inhibition of the phosphatase significantly affects receptorfunction, the most plausible conclusion is that under basal conditionsa kinase must mediate the phosphorylation of at least one of theproteins involved. To determine this possibility in the phosphorylation-dependentregulation of synaptic GABARs, we next examined the effects ofmicrocystin (20 µM), an inhibitor of protein phosphatases 1 and2A (PP_1/2A). In CA1 pyramidal cells, inclusion of microcystinin the patch pipette gradually reduced mIPSC median conductance( $-$ 33.1%) in a manner analogous to that seen with PKA perfusion(Table 1, Fig. 4A). A 3.6-fold increase in the fraction of biexponentiallydecaying mIPSCs was also observed (Table 1). No other changesin CA1 pyramidal cell mIPSC parameters or their frequency wereobserved when microcystin was present in the intracellular solution(Table 1).

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Figure 4. A, B, Effect of microcystin on mIPSCs recorded from dentate gyrus GCs and CA1 pyramidal cells. Left panels show five consecutive raw traces (500 msec each, i.e., 2.5 sec in total) from a CA1 pyramidal cell (A) and a dentate gyrus GC (B). The middle panels show recordings from cells with 20 µM microcystin inside the patch pipette. Note the diminished amplitudes of mIPSCs in the CA1 pyramidal cell, but not in the GC, in the presence of microcystin. The graphs on the right show cumulative probability distributions of mIPSC peak conductances in the control recordings (thin lines) and in recordings with microcystin (20 µM) in the electrode (thick lines). In CA1 pyramidal cells (A), mIPSCs conductances (n = 654 events) were smaller in the presence of microcystin when compared with those recorded in a cell under control conditions (n = 393 events), indicating a reduction of mIPSC amplitudes. In the two GCs (B), there was no significant difference between mIPSC conductances in control recordings (n = 324 events) and those with 20 µM microcystin included in the pipette (n = 262 events). C, Time course of PKC, PKA, and microcystin effects in CA1 pyramidal cells and GCs. In CA1 pyramidal cells, the gradual diffusion of PKA (gray circles) and microcystin (black circles) into the cells through the patch electrode caused a significant (p < 0.05; t test) decrease in mIPSC conductance that reached steady state after 6-7 min of whole-cell recordings. No time-dependent changes were noted with PKC included in the patch pipette. In contrast, in GCs, PKC but not PKA significantly (p < 0.05; t test) potentiated mIPSCs 9-10 min after the start of the whole-cell recordings. Each point represents the mean conductance (±SD) of >1000 events pooled from n = 3-5 cells at each of the indicated time periods.

In GCs, microcystin (20 µM) did not change the mIPSG (Table 2, Fig. 4B) but caused a 1.8-fold increase in the fraction ofbiexponentially decaying mIPSCs (Table 2). As in CA1 neurons,mIPSC 10-90% rise times and frequency of occurrence were unaffectedby microcystin (Table 2).

The time course of PKC, PKA, and microcystin effects on mIPSCs

Figure 4C displays the time-dependent changes in mIPSG recorded in CA1 pyramidal cells and GCs in the presence of controlintracellular solutions, PKC, PKA, or microcystin. In controlwhole-cell recordings, the median mIPSG remained stable, but inCA1 neurons, PKA (6 µgm/ml) and microcystin (20 µM) decreasedmIPSG during whole-cell recordings in a time-dependent manner,whereas in GCs only PKC (6 µgm/ml) had a gradual, time-dependenteffect on mIPSG. As indicated in the figure, significant effectswere seen after 6-7 min and after 9-10 min of whole-cell recordingsin the presence of PKA in CA1 cells and PKC in the GCs, respectively

Endogenous PKA is responsible for the microcystin-induced reduction of mIPSC amplitudes in CA1 pyramidal cells

To ascertain whether PKA was the endogenous protein kinase involved in the regulation of mIPSCs in CA1 pyramidal cells, wesuppressed endogenous phosphatase activity by microcystin andsimultaneously reduced the activity of protein kinase A. Specificinhibitors of PKA (PKA-I, 0.66 µM included in the patch electrode;and Rp-8CPT-cAMP-S, 100 µM perfused extracellularly) were appliedwith or without intracellular microcystin (20 µM). According toan in vitro biochemical assay, the intrapipette concentrationof PKA-I was sufficient to inhibit 15 µgm/ml of PKA (M. D. Browning,unpublished observations). The microcystin-associated reductionin mIPSG was completely antagonized by inclusion of PKA-I in theelectrode or by perfusion of Rp-8-CPT-cAMP-S (Table 1, Fig. 5).Although Rp-8-CPT-cAMP-S is cell-permeant, it produced no apparentpresynaptic changes as seen by the constant frequency of mIPSCs.In all of these experiments the mIPSC kinetics remained comparableto those observed in control recordings or in cells with boiledPKA in the electrode (Table 1). It is interesting to note thatinclusion of active PKA together with the phosphatase inhibitorproduced no additive effects on mIPSCs (Fig. 5). This may meanthat the rate of dephosphorylation is most likely the rate-limitingstep in the control of synaptic GABAR function.

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Figure 5. Modulation of GABAR-mediated mIPSC conductance by intracellular perfusion of protein kinases, protein kinase inhibitors, and protein phosphatase inhibitors. All conductance values were normalized to the control conductance (dotted line, 100%) and are represented as percentage. In CA1 neurons (filled gray bars) boiled PKA, inactive PKC, and PKA inhibitors alone (intracellular PKA-I, 0.66 µM, and extracellular Rp-8-CPT-cAMP-S, 100 µM) had conductances similar to control. However, PKA (Low PKA, 0.6 µg/ml and High PKA, 6 µg/ml) and microcystin alone (20 µM) or in combination with PKA (6 µg/ml) showed a significant reduction in mIPSC amplitude. The effects of microcystin were completely abolished by PKA inhibitors (intracellular PKA-I, 0.66 µM, or extracellular Rp-8-CPT-cAMP-S, 100 µM). In GCs (open bars), only PKC (6 µgm/ml) induced a significant potentiation of mIPSC conductance. Microcystin, inactive PKC, or PKA (6 µgm/ml) were without effect.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

We have studied the regulation of GABAR-mediated mIPSCs by protein kinases and phosphatases. Our results are consistent withthe involvement of PKA and PKC in the regulation of synaptic GABARfunction in CA1 pyramidal cells and GCs, respectively. There wereremarkable differences, however, between the phosphorylation-dependentmodulation of mIPSCs in the two cell types. Activation of PKAalters synaptic GABAR function only in CA1 pyramidal cells, whereasPKC changes mIPSCs recorded in GCs. Moreover, PKA decreased mIPSCamplitudes in CA1 pyramidal cells, whereas PKC increased mIPSCamplitudes in GCs. The 10-90% rise and decay time constants ofmIPSCs in both CA1 and GCs were unaffected by intracellular kinaseadministration. Both kinases produced an increase in the fractionof biexponentially decaying mIPSCs. The results with intracellularmicrocystin, a PP_1/2A inhibitor, are consistent with endogenousPKA being steadily active in CA1 neurons but not in GCs. Thus,the net balance between phosphorylation and dephosphorylationwill critically alter the strength of GABA_Asynapses.

Specificity of the phosphorylation effect to synaptic GABARs

In acute or cultured hippocampal slices, membrane-permeable activators of PKC and PKA dramatically increase the frequencyof mIPSCs recorded in CA1 and CA3 pyramidal cells (Pitler andAlger, 1994; Aniksztejn et al., 1995; Capogna et al., 1995), withoutaltering mIPSC amplitudes. However, any possible postsynapticeffect of the membrane-permeable compounds might have been obscuredby the powerful presynaptic action. In our studies, the directintracellular administration of membrane-impermeable compoundssuch as microcystin or constitutively active PKC and PKA was designedto eliminate interference with presynaptic mechanisms, thus allowingus to strictly monitor the postsynaptic regulation of synapticGABARs. Some of our findings, such as the lack of PKC effect onGABAR-mediated mIPSC amplitude in CA1, are in agreement with previousstudies reporting purely presynaptic effects of extracellularlyapplied PKC activators (Pitler and Alger, 1994). Nevertheless,it is possible that the lack of effect of PKC in the CA1 regioncould be caused by our failure to apply the correct PKC isotype.We consider this possibility unlikely because our PKC preparationcontains three isoforms ( $alpha$ , $beta$ , and $gamma$ ), and the various isoformsdo not appear to have unique substrates, only some differencesin the kinetics of phosphorylation (Kazanietz et al., 1993).

Despite the purely postsynaptic route of administration of active compounds, we have observed effects on mIPSC frequency thatmight be interpreted as being of presynaptic origin. For example,when the PP_1/2A inhibitor microcystin was coadministered withPKA-I, there was a significant 50% increase in the frequency ofmIPSCs without any significant change in their amplitudes. Ifthis effect is indeed presynaptic, one possibility is that thesimultaneous inhibition of PKA and of PP_1/2A may have releaseda transsynaptic messenger that leads to an enhanced GABA releaseor to a reduced tonic inhibitory effect on the presynaptic terminals.A transsynaptic modulation of GABA release is believed to occurthrough release of glutamate onto presynaptic metabotropic glutamatereceptors (Glitsch et al., 1996), most likely belonging to groupI (Morishita et al., 1998). Alternatively, the observed increasein mIPSC frequency may be entirely of postsynaptic origin. Ifone assumes that GABA_A synapses can be kept "silent" (Poisbeauet al., 1997), the simultaneous inhibition of PKA and PP_1/2 mayproduce a conversion of silent synapses into active ones. Then,if the unitary events generated at these synapses are similarto mIPSCs recorded under control conditions, the "uncovered" eventswould be indistinguishable from controls and would simply addto existing mIPSCs producing the increase in frequency. At present,there are no data to support eitherpossibility.

The GABAR subunit as a possible target of phosphorylation

With the exception of their frequency of occurrence, there are remarkable similarities between mIPSCs recorded in CA1 pyramidalcells and GCs. It is therefore puzzling to find such differentactions of PKA and PKC on the function of synaptic GABARs. Ifa direct phosphorylation of GABAR subunits is involved in theeffects seen in our study, a different subunit composition ofthe receptors in the two regions might explain the observed differencesin their phosphorylation-dependent regulation. Albeit minor, thereare some divergences in the molecular identities of GABARs presentin the two cell types. For example, GCs express $delta$ and $alpha$ 4 subunits,whereas $alpha$ 5 subunits are mostly found in CA1 pyramidal cells. Mostother subunits are shared by the two populations. Accordingly,the presence of specific subunits in synaptic GABAR aggregatesmay be responsible for the region specificity as well as for thedirection of the alterations induced by phosphorylation. In thiscontext, however, it is interesting to note that to date thereare no reports about differential effects of phosphorylation on $alpha$ 4 and $alpha$ 5 subunits, and possible effects of phosphorylating $delta$ subunits may be discounted, because at least in the cerebellum, $delta$ subunit-containing receptors are found exclusively extrasynaptically(Jones et al., 1997; Nusser et al., 1998).

Our experiments do not allow us to reach conclusions about a direct phosphorylation of GABARs by PKA or PKC. However, thesimplest explanation supported by strong experimental evidenceis that specific GABAR subunits can be phosphorylated and thatthis phosphorylation modifies GABAR function (Levitan, 1994; Macdonaldand Olsen, 1994; Sieghart, 1995; Sigel, 1995; Moss and Smart,1996). It appears that $beta$ subunits are the best substrates forPKA- and PKC-dependent phosphorylation, but unequivocal conclusionsare complicated by the fact that $beta$ subunits are not the sole potentialtargets for phosphorylation (Macdonald and Olsen, 1994). Mutagenesisof Ser409 of the $beta$ 1 subunit eliminates PKA-induced regulationof GABAR function (Moss et al., 1992a,b). A recent report (McDonaldet al., 1998) has further characterized the differential effectsof PKA-dependent phosphorylation of $beta$ subunit-containing recombinantGABARs. It appears that $beta$ 2 subunit-containing receptors, whichshould be the most predominant $beta$ subunits in hippocampal neurons(McKernan and Whiting, 1996), are not affected by PKA-dependentphosphorylation. The phosphorylation of $beta$ 1 subunits reduces thecurrent flow through recombinant GABARs, whereas the same processon $beta$ 3 subunit-containing receptors produces the opposite effect.If the effect of PKA on mIPSCs stems indeed from phosphorylationof $beta$ subunits, the $beta$ subunit selectivity of the PKA-dependentphosphorylation may indicate that GABARs at synapses of CA1 pyramidalcells preferentially contain $beta$ 1 subunits, whereas those at inhibitorysynapses on GCs contain mainly $beta$ 2subunits.

As mentioned above, our findings do not necessarily demonstrate a direct phosphorylation of a given GABAR subunit. Indeed,phosphorylation of a GABAR-associated protein that controls itsfunction may be responsible for the regional differences observedin our study. Such proteins have yet to be conclusively demonstratedat GABA_A synapses, but there is ample evidence from glutamatesynapses that such proteins can be closely associated with synapticreceptors (Kennedy, 1997; Sheng and Wyszynski, 1997). Regardlessof the exact mechanism for the disparate regulation of synapticGABARs in CA1 pyramidal cells and GCs, there is a noteworthy similaritybetween our present findings and the differential effect of withdrawalfrom chronic benzodiazepine treatment in these two types of neuron(Poisbeau et al., 1997). The mIPSCs of GCs are insensitive toin vivo benzodiazepine withdrawal, whereas the size of mIPSCsrecorded in CA1 pyramidal neurons significantly decreases duringthe withdrawal period. Whether there is a relationship betweenthe sensitivity of synaptic GABARs to PKA-dependent phosphorylationreported in the present study and the effects of long-term benzodiazepinetreatment on these receptors remain to bedetermined.

Continuous PKA-dependent phosphorylation in CA1 pyramidal cells

We have shown a continuous cycle of a PKA-dependent phosphorylation and a PP_1/2A-dependent dephosphorylation to affect thefunction of synaptic GABARs in CA1 pyramidal cells. It is temptingto speculate that the small fraction of mIPSCs with a double exponentialdecay might be the result of such continuous phosphorylation.However, the proportion of such events was unaffected by inhibitionof PKA. Such a basal phosphorylation/dephosphorylation cycle doesnot seem to alter the function of GABARs at synapses in GCs, althoughactivation of the PKC pathway could induce an increase in mIPSCamplitude. In CA1 pyramidal cells, promoting phosphorylation willinhibit synaptic GABARs, whereas tipping the balance in favorof dephosphorylation will enhance inhibitory events. Thus, dephosphorylationof the GABARs, or of closely associated proteins, by PP_1/2A canplay a crucial role in regulating inhibitory strength in CA1 pyramidalcells. In addition, calcium-dependent phosphatases and kinasesmay also alter currents evoked by GABA in CA1 neurons (Stelzeret al., 1988; Chen et al., 1990; Wang et al., 1995).

How does phosphorylation affect the function of synaptic GABARs?

The precise mechanisms whereby phosphorylation of ligand-gated channels alters channel function are not well understood. Theremight be effects on receptor desensitization, the opening probabilityof the channels, the interaction between ligand and receptor,or the predominant conductance state to which the channels open.One of the most detailed studies to date on this topic has demonstrateda PKA-induced increase in the probability of channel opening atthe peak of currents through homomeric GluR6 channels (Traynelisand Wahl, 1997). The probability of channel opening was intermediate(0.65) under control conditions, but could be increased to 0.85-0.94when the channels were phosphorylated or reduced to 0.5 when dephosphorylatedby the Ca²⁺/calmodulin-dependent protein phosphatase calcineurin. Thus, awide dynamic range may exist for the regulation of the numberof channels open at the peak of synaptic responses. In contrastto homomeric GluR6 channels expressed in HEK293 cells, the functionof GABARs at CA1 pyramidal cell inhibitory synapses was downregulatedby PKA activation. It is tempting to speculate that in these neuronsa continuous phosphorylated state may keep synaptic GABARs consistentlybelow their full inhibitory potential. This might be akin to theoperation of air brakes, where the compressoractively spends energyto keep the brake pads away from the disks to ensure stoppingin the event of a system failure. In the case of GABARs, the steadyphosphorylation by PKA may keep the function of the receptorssufficiently low, so that in the event of a cellular metabolicchallenge and falling ATP levels, GABAergic inhibition could escapefrom the suppressing effect of phosphorylation to provide moreinhibition for theneuron.

It is interesting to note that regardless of an enhancement, as with PKC in the GCs, or a suppression of mIPSCs, as with PKAin CA1 pyramidal cells, the augmented phosphorylation caused anenhanced incidence of biexponentially decaying mIPSCs. In ourmodel, this effect does not need to involve receptor desensitization,but according to a recent study (Jones and Westbrook, 1997), promotingphosphorylation in cultured neurons by inhibiting calcineurinleads to an increased GABA unbinding rate and an enhanced desensitizationof fast GABA currents and IPSCs. The kinase responsible for thephosphorylation was not identified in this study, and in contrastto our results, inhibition of PP_1/2 was without effect on synapticand evoked GABA currents. Yet, an aspect of our results is clearlyconsistent with the findings in cultured neurons: a continuouscycle of phosphorylation/dephosphorylation appears to controlthe function ofGABARs.

In conclusion, we have demonstrated that the function of synaptic GABARs in hippocampal CA1 pyramidal cells is under the controlof a basal phosphorylation by PKA and that mIPSCs in GCs can beaugmented via phosphorylation by PKC. Accordingly, in CA1 pyramidalcells, inhibitory strength will critically depend on the relativeintensities of phosphorylation and dephosphorylation. When dephosphorylationoutweighs phosphorylation, as may happen during metabolic impairment,this mechanism will ensure a decreased excitability through enhancedGABAR-mediatedinhibition.

  FOOTNOTES

Received Sept. 22, 1998; revised Oct. 30, 1998; accepted Nov. 2, 1998.

This work was supported by National Institutes of Health/National Institute of Neurological Diseases and Stroke Grant NS-30549,and the Coelho Endowment to I.M.; P.P. was partly supported bythe Philippe Foundation. We thank Dr. Matt Jones (Vollum Institute)for providing files and parameters used in the SCoP fitting routines,and Brian K. Oyama and Michael T. Kim for technicalassistance.
Correspondence should be addressed to Dr. Istvan Mody, Departments of Neurology and Physiology, University of California atLos Angeles, School of Medicine, Los Angeles, CA90095.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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