Extracellular 3',5' Cyclic Guanosine Monophosphate Inhibits Kainate-Activated Responses in Cultured Mouse Cerebellar Neurons

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Vol. 286, Issue 1, 99-109, July 1998

Extracellular 3',5' Cyclic Guanosine Monophosphate Inhibits Kainate-Activated Responses in Cultured Mouse Cerebellar Neurons¹

Cornelia Poulopoulou² and Linda M. Nowak

Department of Pharmacology, College of Veterinary Medicine, Cornell University, Ithaca, New York

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

The effects of extracellularly applied 3'-5' cyclic guanosine monophosphate (cGMP) on kainate responses from cultured cerebellargranule and Purkinje neurons were investigated using whole-celland outside-out patch recording modes. Cerebellar granule cellresponses to kainate were not homogeneous, nor were the effectsof cGMP. Therefore, effects of cGMP are described for two groupsof granule cells categorized on the basis of the underlying channelconductance estimated by variance analysis. Cells with high-noisekainate responses had average channel conductances of 5 to 7 picoseimens,whereas the average conductances of low-variance noise responseswere 0.3 to 2.0 picoseimens. High-noise kainate responses wereinhibited by externally applied cGMP (5-1000 µM) in a rapidlyreversible and dose-dependent manner. IC₅₀ values were estimatedat ~150 µM cGMP for 25 µM kainate and ~500 µM cGMP for 100 µMkainate. Evidence that cGMP-mediated inhibition of high-noisekainate responses occurred by a competitive mechanism includedthe following: 1) cGMP-mediated inhibition was overcome by increasingagonist concentration. 2) The shape of kainate current-voltage(I-V) curves and their reversal potentials were unchanged in cGMP.3) Neither the estimated conductance nor the kinetics of the kainate-activatedchannels was affected by cGMP. In contrast to the uniform effectsof cGMP on the high-noise kainate responses, the effects on low-noisekainate responses were variable. Half of the low-noise kainateresponses were inhibited by cGMP to a similar extent as the high-noiseresponses; however, the other 50% of cells exhibiting low-noisekainate responses appeared to be less sensitive to the cyclicnucleotide. Moreover, cGMP coapplication decreased the estimatedconductances for some low-noise kainate responses and alteredtheir noise kinetics, which suggests either that cGMP-sensitiveand -insensitive kainate receptor channels are coexpressed inthese cells or that cGMP-mediated inhibition is not competitivefor this subgroup of glutamate receptor channels. Overall, thesedata indicate that there are direct inhibitory effects of extracellularcGMP on a large group of excitatory synapses in the CNS $---$ effectsthat need to be taken into account when investigators utilizemembrane-permeable cGMP analogs. Whether this cGMP-mediated inhibitionhas a functional role in brain is unknown.

	Introduction

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Studies of cGMP in mammalian brain begin with the early reports that activation of glutamate receptors in cerebellum causesa dramatic increase in the cGMP content of this tissue (Mao etal., 1974; Rubin and Ferrendelli, 1977; Garthwaite and Balázs,1978). Subsequently, the signaling pathway mediating cGMP productionin neurons was shown to involve an increase in intracellular Ca⁺⁺, leading to a Ca⁺⁺-calmodulin-dependent activation of NOS (Bredt and Snyder, 1989;Mayer et al., 1992) and NO stimulation of soluble guanylate cyclasetypically located in cells in close proximity (Garthwaite, 1991).In the cerebellum, NOS appears to be localized to granule cells(Bredt et al., 1991) and the NO-sensitive soluble guanylate cyclaseis localized to granule cells (Southam et al., 1992; Southam andGarthwaite, 1993) and to Purkinje neurons (Zwiller et al., 1981;Ariano et al., 1982; Matsuoka et al., 1992), which are thoughtto be largely responsible for the dramatic kainate-mediated increasein cerebellar cGMP (Rubin and Ferrendelli, 1977).

The consequences of glutamate receptor-linked elevation of intracellular cGMP in Purkinje and granule neurons are poorly understood,but it is likely that cGMP activates G-kinase in the Purkinjeneurons (DeCamilli et al., 1984), which contain high levels ofa 23-kd cytosolic protein called G-substrate (Aswad and Greengard,1981). cGMP is also the intracellular ligand for cyclic nucleotide-gatednonselective cation channels, thus depolarizing a number of celltypes (Yau and Baylor, 1989; Zagotta and Siegelbaum, 1996). Animportant role is proposed for cGMP in LTD in cerebellum (Itoand Karachot, 1992; Daniel et al., 1993; Hartell, 1994; Lev-Ramet al., 1997). In single Purkinje neurons, for example, LTD hasbeen linked to an increase of cGMP, in synergy with an increaseof intracellular Ca⁺⁺ and of NO production (Lev-Ram et al., 1997). The mechanism bywhich an elevation of intracellular cGMP contributes to synapticdepression is as yet unknown.

A less widely known area of investigation is the interaction between the extracellular domain of glutamate receptor channelsand guanosine nucleotides. Interestingly, most guanosine compoundsappear to interact with the extracellular domains of glutamatereceptors. Early studies of goldfish brain kainate binding proteinssuggested that a G protein-coupled mechanism may be involved inguanosine compound-mediated inhibition of [³H]kainate binding (Willard et al., 1991; Willard and Oswald, 1992;Ziegra et al., 1992a; 1992b). Subsequent work provided evidencethat GTP $gamma$ S-mediated inhibition of [³H]kainate binding in goldfish brain membranes was at least partiallyexplained by competitive interactions at the agonist binding siteon either the kainate binding proteins or ionotropic glutamatereceptors (Barnes et al., 1993). Gorodinsky et al. (1993) demonstrateda low-affinity (IC₅₀ = 1 mM) competitive inhibition by GTP forthe low-affinity [³H]AMPA binding site in rat cerebral cortex and a noncompetitiveinhibition of high-affinity [³H]AMPA binding to rat cortex non-NMDA receptors. Likewise, a competitivemechanism was suggested by studies of [³H]kainate binding to detergent-solubilized recombinant kainatebinding proteins where GTP and GDP analogs were equipotent competitors;in this study, however, cGMP was minimally effective (Paas etal., 1996a). By contrast, in a crude preparation of rabbit cerebellarmembranes (P₂ fraction) high-affinity [³H]kainate binding was inhibited competitively by all the guanosinecompounds tested, including cGMP, GMP, GDP and GTP, with comparablelow affinity (IC₅₀ = 1.5 mM) (Poulopoulou, 1994). The differencesbetween the binding data from partially purified receptors anda crude synaptosomal preparation, coupled with reports that cGMPdoes inhibit glutamate responses in electrophysiological studieswhen applied at the extracellular surface (Linden et al., 1995),suggested that cGMP may preferentially interact with intact non-NMDAreceptors in cell membranes, in contrast to the other guanosinenucleotides that interact with sites on soluble receptors (Paaset al., 1996a).

We have examined the nature of the extracellular cGMP inhibition of non-NMDA responses of cultured neurons to slow bath applicationof kainate, which activates primarily AMPA receptor channels becausekainate receptor channels are rapidly and profoundly desensitizedby continuous exposure to kainate (Lerma et al., 1993). Patch-clamprecordings in whole-cell mode for cerebellar granule cells andin outside-out patches excised from Purkinje neurons were usedto determine whether the effects of cGMP may depend on differencesin the expression of non-NMDA receptor channel subunits by differentcells. Cerebellar granule cells were chosen because there is evidencethat their responses to different non-NMDA agonists are not homogeneousfrom cell to cell (Wyllie et al., 1993; Poulopoulou, 1994).

	Materials and Methods

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Primary cultures. Purkinje cell cultures were prepared as micro-explants from newborn mouse pups (12-36 h after birth) by the method of Moonenet al. (1982). Pups were anesthetized and killed with CO₂ accordingto an IACUC-approved protocol. Brains were rapidly dissected andplaced in ice-cold Puck's saline with sucrose for ~10 min untilthe cerebella were dissected. Vermal, floccular and parafloccularareas were removed and discarded. The neocortical lobes of cerebellumwere minced with irridectomy scissors and lightly dissociatedby trituration (3-4 passes) through a large-bore Pasteur pipetin a MEM (Gibco BRL, Grand Island, NY) solution containing 10%fetal bovine serum and 10% heat-inactivated horse serum (Hyclone,Logan, UT). Small pieces of tissue and suspended cells were collectedand plated on collagen-coated (Sigma Chemical Co., St. Louis,MO) 35-mm dishes (Falcon, Lincoln Park, NJ). When the explantswere well attached (12-24 h), 1 ml of medium containing FUDR,Sigma was added. Cultures were grown in MEM/10-10 with FUDR for2 days before changing to MEM/10% horse serum medium. Subsequently,culture solutions were partially changed at 3 to 4-day intervals.Purkinje neurons were recognized by their size, morphology andsynaptic activity; recordings were performed between 10 and 20days in vitro.

Cerebellar granule cells were cultured in an enriched 25 mM KCl-containing medium following the protocol of Messer (1977)

with modifications. Cerebella were dissected from 5 to 8-day-oldmice. Cerebellar neocortices were dissociated in serum-free culturemedium containing 1% trypsin (Sigma) for 5 to 8 min at room temperature.Trypsin activity was quenched with serum-containing culture medium,and the 2-ml cell suspension was triturated gently. Dissociatedcells were suspended in Hams F12 (Gibco) with added vitamins,glutamine, glucose, 24.5 mM K⁺ and 10% each of fetal calf serum and heat-inactivated horse serum.The cell suspension was plated on 35-mm collagen-coated culturedishes and left to grow for 4 to 6 days before the addition ofFUDR. After 24 to 36 h of exposure to mitotic inhibitors, thecells were maintained in the modified Hams F12 supplemented with10% horse serum.

Recording conditions. Experiments were performed at room temperature (22°-25°C). Agonist responses were recorded in conventional whole-cell andoutside-out patch modes as described by Hamill et al. (1981) witha List EPC-7 amplifier (Medical Systems) using borosilicate glasspipets (2-8 M $Omega$ ; WPI TW150). Glass recording pipets were coatedwith Sylgard (Dow Corning, Midland, MI) and their tips lightlyfire-polished. Patch pipets contained (in mM): 140 or 145 CsCl,10 K-EGTA, 1 CaCl₂, 10 K-HEPES (pH 7.2). The majority of recordingswere made with 4 mM ATP-Mg added to the pipet solution. Extracellular("bath") solutions contained (in mM): 150 NaCl, 2.8 KCl, 1.0 CaCl₂,10 Na-HEPES (pH 7.2) with 300 nM TTX (Sigma).

Pharmacological agents. Kainate (Sigma Chemicals and Research Biochemicals Inc.; RBI, Natick, MA), AMPA (RS- $alpha$ -amino-3-hydroxy-5-methylisoxazole-4-propionicacid; Cambridge Research Biochemicals, and RBI, Natick, MA), cGMPand 8 bromo-cGMP (Sigma) were prepared as concentrated stock solutions,divided into aliquots and frozen. Frozen stock solutions wereused within 20 days of preparation.

At the beginning of an experiment, stock solutions were diluted with the extracellular recording buffer. Drug and controlsolutions were applied to excised patches by gravity-fed superfusionin the vicinity of the patch pipet through a large-bore Pasteurpipet. Solution changes were initiated by opening a valve at areservoir containing the drug or drugs, and the solution was appliedafter a delay of 30 to 60 s, depending on the length of the tubingbetween the particular reservoir and the Pasteur pipet tip andon the perfusion rate. The drug concentration at the patch increasedover a period of 20 to 60 s in most recordings before reachingequilibrium. There was continuous perfusion of the bath, eitherby control or by drug-containing solutions, throughout the courseof the experiments.

Data acquisition and analysis. Amplified data (List EPC7) were initially filtered at 4 kHz through an 8-pole low-pass Bessel filter (902LPF, Frequency Devices,Haverhill, MA), converted to digital format (Medical Systems,PCM-1B) and recorded on video tapes (Sony Beta SL HF450 usingMaxell Gold, Fuji Beridox and BASF-HG tapes). Data were reconverted(PCM-1B) to analog signals and refiltered (Butterworth) at thedesired cutoff frequency. Data analysis was done on personal computers(AST Premium) using CAP software (R. C. Electronics, Goleta, CA)and additional software written in the laboratory. Whole-celland large-amplitude responses in excised patches were subjectedto noise analysis.

Power spectral density analysis. Power spectral density analysis as described by Wright et al. (1991) was performed on control and agonist recordings fromcells and excised patches that gave large responses. Currentswere filtered ( $-$ 3 db point at 1.0 or 1.5 kHz) using an 8-poleButterworth filter to minimize frequency-dependent changes inpower density. Data were sampled at the Nyquist frequency (2 or3 kHz) in blocks of 4096 points. Agonist-evoked current noiseand control noise (instrument plus background membrane patch noise)were fast-Fourier-transformed into component frequencies. Powerspectra were obtained by averaging between 40 and 70 blocks ofdata. Equal numbers of control and agonist blocks were used togenerate any given pair of power spectra; agonist noise spectraare shown with control noise subtracted. Spectra were fitted (Simplexalgorithm) by one Lorentzian function or the sum of two Lorentzianfunctions of the form

S(f)=S0[1/1+(f/fc)2] (1)

where S_(f) is the spectral density frequency f in Hz, S₀ is the zero frequency asymptote and f_c is thefrequency at which the spectral density is 0.5 S₀. The proportionof the two components in two Lorentzian fit spectra is shown onthe figures as S_0₁ and S_0₂, and the time constants ( $tau$ values)underlying the noise were calculated as follows:

&tgr;=1/2&pgr;fc (2)

Variance analysis. The variance method was used to estimate channel conductance ( $gamma$ ) in patches exhibiting large-amplitude responses, becauseindividual channel events could not be detected, and in whole-cellrecordings. Variance ( $sigma$ ²) of the agonist noise response was determined in pseudostationaryconditions as the drug concentration increased from control toits equilibrium concentration. Data segments (4096 points) werechosen in control, during the onset and growth of the responseand after the steady-state drug concentration was reached. A linewas fitted to each data segment to determine the mean currentlevel (I) in it, and the $sigma$ ² of the current noise about the I mean was calculated and plottedagainst I ( $sigma$ ²/I plots). Under the conditions of our experiments, where thefinal agonist concentration is less than the agonist EC₅₀, thedata were fitted by a straight line using linear regression. Theslope of the line was taken to be the elementary current of theactive channels. The $gamma$ of the channels was estimated by the formula

&ggr;=i<UP>e</UP>/(V<UP>R</UP>−V<UP>H</UP>) (3)

where i_e is the elementary current, V_R is the reversal potential of the response and V_H is the membrane holding potentialduring the response. The value i_e was determined as the slopeof the ratio of the variance in the agonist-evoked current noise( $sigma$ ² in pA²) to the mean transmembrane current (I in pA) as the agonist concentrationis increasing from control to the full agonist response. Typically,if the final concentration is less than the EC₅₀ for the agonist;the pseudostationary variance analysis as performed here providesa condition where less than 50% of channels are likely to be active,and the slope of the $sigma$ ²/I plots was fitted by linear regression. In performing the powerspectral density and variance analyses, we took care to use kainateconcentrations 3- to 4-fold higher than needed to obtain a thresholdagonist response, but less than the EC₅₀. Where noise analysisdata are compared from different cells or under different conditions,mean values +/ $-$ S.E.M. are given.

	Results

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Whole-cell and outside-out patches from cerebellar granule cells and patches from some Purkinje neurons responded to applicationof 25 to 300 µM kainate with large-amplitude inward currents ata holding potential of $-$ 60 mV. All the neurons and patches examinedresponded to kainate. During the 20 to 75-min recordings, thecells and patches were subjected to multiple solution changesto ensure reproducibility of the drug effects. Cerebellar granulecells were grouped according to the characteristics of the agonist-evokednoise. Figure 1 shows two different types of responses to kainateobserved in these cells. Variance analysis on these responsesgave an average estimated conductance of 5.51 +/ $-$ 0.83 pS (n =8) for the group of cells with high-noise responses referred toas type I cells. Meanwhile, the average conductance for the cellswith low-noise responses (type II cells) was 0.88 +/ $-$ 0.55 pS(n = 18). None of the cells in this sample had estimated conductancesbetween 2 and 4 pS.

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Fig. 1. Whole-cell currents from mouse cerebellar neurons from primary cultures in response to kainate application were initially classified into two groups according to the estimated aggregate conductance of the current responses. A) Application of 11 to 100 µM kainate to some cerebellar neurons evoked inward current responses associated with robust increases in the noise. Variance analysis on the current noise of one such response to 100 µM kainate gave an estimated i_e of $-$ 0.37 pA in this cell for an estimated average $gamma$ of ~6.2 pS. B) In other cells, 33 to 300 µM kainate routinely evoked inward currents that were accompanied by a modest increase in the noise. Variance analysis of the current noise in the cell depicted here gave an estimated $gamma$ = 0.83 pS. In both examples, the holding potential was $-$ 60 mV and the reversal potential was 0 mV.

Concentration-effect data were collected from eight cerebellar granule cells for kainate between 8 µM and 1 mM; these dataalso indicated that mouse cerebellar granule cells are not uniformlysensitive to kainate. The high-noise responses in kainate (n =3) were more sensitive to this agonist than the cells exhibitinglow-noise responses (n = 5). Typical type I cells showed a smallresponse to 11.1 µM kainate, whereas 33.3 µM kainate was requiredto evoke small-amplitude responses routinely in type II cells.Approximate EC₅₀ values were between 150 and 200 µM kainate forthe type I cells and between 300 and 400 µM kainate for the typeII cells. The type II cells exhibited larger average current responsesin 100 to 300 µM kainate than the type I cells, a result consistentwith the low-noise cells containing low-conductance non-NMDA channels,but many more active ones than the cells with high-noise responsesto kainate.

The effects of cGMP/kainate coapplication were reversible and highly reproducible in the type I (high-noise) cells and patches.cGMP inhibited the kainate responses in all type I cells and inpatches excised from Purkinje neurons (cells/patches = 18, trials= 43). Preliminary experiments had indicated that both cGMP andthe membrane-permeable analog 8 Br-cGMP inhibited the kainateresponses in type I patches at the same concentrations, and theirtime courses for inhibition and washout were similar. Subsequently,the membrane-impermeable form cGMP was used for recordings tocontrol for the possibility that the patches/cells might containsome cyclic nucleotide-gated ion channels.

The cGMP-mediated inhibition of these kainate currents was rapidly reversed by subsequent perfusion with 25 µM kainate alone(fig. 2). A typical example of a large-current response to 25µM kainate from a granule neuron is shown in figure 2A. Afterthe response to the first application of 25 µM kainate had reachedits steady-state amplitude, kainate and cGMP were coapplied. Asillustrated, kainate currents were inhibited by cGMP in a dose-dependentfashion (fig. 2, B and C). Coapplication of 200 µM cGMP with 25µM kainate resulted in a 60% reduction of the kainate current.

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Fig. 2. High-noise inward currents are inhibited by cGMP in a dose-dependent manner. A) The response of a type I cerebellar granule neuron to 25 µM kainate is inhibited ~60% by coapplication of 200 µM cGMP. B) Responses of an outside-out patch from a Purkinje neuron are shown. 25 µM kainate evoked large increases in the current and the noise (V_H = $-$ 60 mV), a result consistent with the patch containing many kainate-sensitive receptor channels. Slow bath coapplication of 200 µM cGMP with 25 µM kainate in this patch decreased the kainate current by 70% (solid arrow). The current was further reduced to 92% (open arrow) by subsequent application of 600 µM cGMP, which indicates concentration-dependent inhibition of the kainate current by cGMP. C) Dose-inhibition data for cGMP in the kainate current responses from mouse cerebellar cells/patches. Currents activated by 25 µM kainate in the absence and presence of increasing concentrations of cGMP (5-1000 µM) were recorded from mouse cerebellar neurons and patches that contained many kainate-activated channels. Patches from cells as small as the granule neurons used in this study were generally nucleated (Sather et al., 1990

). Standard-error bars are shown. The curve was drawn between the data points and the IC₅₀ estimated from the graph.

Recordings from four cells and 12 outside-out patches that gave high-noise responses were used for estimating an IC₅₀ forcGMP-mediated inhibition in the following set of conditions: 25µM kainate was applied alone, and then it was coapplied with threeor four different concentrations of cGMP between 5 and 1000 µM.The steady-state control kainate current amplitude was measured,and the percent inhibition for each dose of cGMP was calculated.The dose-inhibition curve in figure 2C was constructed by plottingthe percent of kainate current remaining in each concentrationof cGMP against the log of the nucleotide concentration for eachpatch/cell. The IC₅₀ under these conditions was 150 (+/ $-$ 25) µMcGMP. Increasing the kainate concentration to 100 µM increasedthe agonist response amplitude in the absence and presence ofcGMP. Cells with high-variance noise responses to 100 µM kainatewere inhibited by 49.5% (n = 4 cells; 7 trials) in 500 µM cGMP.Approximately half of the granule cells with low-noise responseswere comparably affected (fig. 3, A and B).

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Fig. 3. cGMP-mediated inhibition appears to be competitive. A) Whole-cell current responses of a granule cell to the application of 33 µM kainate (panel A₁) and 100 µM kainate (panel A₂) show the dose-dependent increase in the agonist response. B) Coapplication of 33 µM kainate and 500 µM cGMP (panel B₁) and 100 µM kainate plus 500 µM cGMP (panel B₂) responses on the same cell. Recordings in panels A and B were at $-$ 60 mV. Open triangles indicate changing to control solution. C) A current-voltage (I-V) relationship for a type I response from an outside-out patch is shown. The I-V relationships shown were obtained by subtracting the I-V obtained at control solution from the ones obtained in the presence of 25 µM kainate, with and without cGMP coapplication. The I-V relationship of the kainate responses in the absence of cGMP rectifies similar to macroscopic currents recorded in whole cells with kainate (Ascher and Nowak, 1988

). In the presence of 500 µM cGMP, the I-V relationship is smaller at all voltages away from the reversal potential. D) The kainate current inhibited by 500 µM cGMP is plotted as a function of membrane potential. The relationship is linear, which indicates that the nucleotide inhibition of the kainate current is independent of voltage.

The mechanism of cGMP-mediated inhibition of kainate currents was investigated in several experiments: increasing the kainateconcentration in the coapplied cGMP/kainate mixture to overcomethe inhibition of cGMP (fig. 3, A and B), examining the voltagesensitivity of the cGMP-mediated inhibition (fig. 3C) and analyzingthe effects of the cGMP on the noise variance and power spectra(fig. 4).

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Fig. 4. Noise analysis of type I kainate responses in the absence and presence of cGMP. Variance (panel A₁) and power spectral density (panel A₂) analyses of the kainate-activated noise recorded at $-$ 60 mV (raw data shown in fig. 2B) are presented for comparison with results of similar analyses conducted in the presence of 200 µM cGMP (panel B). The estimated elementary current during the application of 25 µM kainate alone was $-$ 0.45 pA (panel A₁), and it was $-$ 0.44 pA during coapplication of 200 µM cGMP and 25 µM kainate (panel B₁). Spectra of the currents from the same outside-out patch in response to 25 µM kainate in the absence of cGMP (panel A₂) were fitted by the sum of two Lorentzian curves with slow and fast time constants of 3.5 and 0.6 ms, respectively. In the presence of 200 µM cGMP, the spectra (panel B₂) of the remaining kainate current had a profile similar to the one in kainate alone. The spectrum for the 25 µM kainate (panel A₂) was obtained by subtracting the power density in the control noise from the power density in the agonist-evoked current noise; control noise was also subtracted from the spectrum for the kainate-activated noise remaining during cGMP/kainate coapplication (panel B₂). Control and agonist noise data were filtered at 1500 Hz (Butterworth) and sampled at 3000 Hz. The recording was made at $-$ 60 mV.

Figure 3 shows current traces from a whole-cell recording where application of 33 µM kainate evoked a type II noise and inwardcurrent. In the presence of 500 µM cGMP, this current responsewas nearly abolished. In the subsequent coapplication of a mixtureof 100 µM kainate with 500 µM cGMP, the kainate response was largerthan in 33 µM kainate alone, which indicates that increasing thekainate concentration overcomes cGMP-mediated inhibition. Thisobservation, which is consistent with cGMP being a competitiveantagonist at the kainate binding site, was obtained in the fourcells and two excised patches tested.

The possible voltage dependence of the cGMP inhibition of kainate steady-state currents was examined in the presence and absenceof the nucleotide, over holding potentials ranging from $-$ 100 to+40 mV, with measurements made at 20-mV increments in whole cellsand outside-out patches that had high-amplitude kainate responses.The current-voltage (I-V) relationships of the cells and patcheswith 5 to 8-pS kainate responses were obtained by subtractingthe I-V obtained in the control solution from that obtained inthe presence of 25 to 100 µM kainate, plus or minus 500 µM cGMP.One example of such a pair of I-V curves from such an outside-outpatch is presented in figure 3C. Macroscopic kainate currentsexhibited a small outward rectification. The fraction of kainatecurrent inhibited by cGMP was a linear function of holding potential(fig. 3D), which indicates that the observed inhibition of thekainate-induced currents by the nucleotide was independent ofvoltage. The reversal potential of the kainate currents, plusor minus the nucleotide, was near 0 mV in the symmetrical cationsolutions used in the recordings. Thus cGMP did not appear toblock the channels, nor did it alter their selectivity in typeI cells/patches.

The noise characteristics of large inward currents evoked by 25 µM kainate in the absence and presence of 200 µM cGMP wereexamined in type I cells and patches. An example is presentedin figure 4. Variance analysis was performed to determine whethercGMP affected the conductance underlying the type I kainate responses.Kainate $sigma$ ² in the absence (fig. 4A₁) and presence of cGMP (fig. 4B₁) indicatedthat cGMP did not affect the i_e of the remaining kainate-activatedcurrents. This observation indicates that the conductances ofthe non-NMDA channels underlying the noise were unchanged by cGMP,a result consistent with the actions of a competitive antagonist.Likewise, power spectral density analysis of the agonist noisein the absence (fig. 4A₂) and presence of cGMP (fig. 4B₂) yieldedsimilar results, which indicates that the cGMP reduced the kainateresponse amplitude without modifying the kinetics of the activereceptor channels. In both cases, the power spectra were fittedby the sum of two Lorentzians, which suggests complicated kineticsof the channels and/or the activation of more than one channelpopulation with different kinetics. Power spectra parameters incGMP were virtually identical to those with kainate alone. Thisbehavior, which is consistent with competitive antagonist actions,was observed in recordings from all high-variance noise responses,and for some cGMP-sensitive low-noise kainate responses (e.g.,fig. 3A and B; power spectra not shown).

Effects of cGMP on low-noise kainate responses. Type II cells have estimated conductances between 0.30 and 2.0 pS (0.88 +/ $-$ 0.55 pS; n = 18). They apparently are not a singlefunctional class, however, because their power spectra, obtainedunder similar experimental conditions, differed considerably fromcell to cell (see below). Moreover, granule cells exhibiting low-noisekainate responses are found to differ considerably with respectto their sensitivity to bath-applied AMPA (Poulopoulou and Nowak,in preparation). The effects of cGMP on some low-noise kainate-responsivecells were investigated systematically to test for cell-to-celldifferences.

Eight low-noise cells were exposed to 100 µM kainate and to 100 µM kainate plus 500 µM cGMP. In contrast to the uniform resultsobtained for the high-noise cells and patches described in theprevious section, the cGMP sensitivity of the type II kainateresponses was indeed variable. Results from three type II cellsrecorded the same day are illustrated in figure 5 and show thediversity in cGMP sensitivity. The first and second cells wereinhibited 30% to 35% by cGMP, whereas the third cell was inhibitedonly ~10%. Variance analysis of the kainate responses for thesecells indicated that $gamma$ was 0.63 pS for the cell in figure 5A,1.57 pS for that in figure 5B and 0.40 pS for that in figure 5C.During cGMP coapplication, the estimated conductances decreasedfor each of these cells to 0.51 pS for the cell in figure 5A,0.34 pS for that in figure 5B and 0.25 pS for that in figure 5C.The estimated conductance did not change for all of the cellsin the presence of cGMP, however, and in some cases the estimatedconductance increased by up to 20%.

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Fig. 5. Examples of low-noise granule cells and the variability of their sensitivity to cGMP coapplication. A) The response to 100 µM kainate in this cell was decreased 32% by coapplication of 500 µM cGMP. Variance analysis gave an estimated conductance of 0.63 pS (mean of 2 measurements) for kainate and of 0.51 pS for the coapplication of cGMP. B) In this cell, the response to 100 µM kainate was decreased by an average of 35% by coapplication of 500 µM cGMP (two trials). The estimated conductance was 1.57 pS for kainate and was 0.34 pS during coapplication of cGMP. C) The response to 100 µM kainate was inhibited by 11% (average of two trials). cGMP decreased the estimated conductance from 0.4 to 0.25 pS. All measurements were made at $-$ 60 mV, and the cells were recorded in the same session so that they were exposed to identical solutions.

The estimated $gamma$ was 0.78 pS (+/ $-$ 0.42 pS) in the kainate alone and 0.79 +/ $-$ 0.47 pS with cGMP coapplication for these eightcells. It was noticed that when cGMP changed the estimated conductancesby ~50% or more, the noise spectra were also markedly changed.Therefore, the variance data were re-examined after separatingthe low-noise cells into two groups: one exhibiting no pronouncedchange in underlying kainate noise kinetics in the presence of500 µM cGMP (n = 4) and the other showing large changes in itspower spectra (n = 4). For the four cells that had no marked changein their spectra with cGMP coapplication, the estimated $gamma$ was0.98 pS (+/ $-$ 0.36) in kainate and 1.14 pS (+/ $-$ 0.40) in kainate/cGMP.However, in the four cells that exhibited a large change in theirpower spectra in the presence of cGMP, the estimated $gamma$ valueswere 0.78 pS (+/ $-$ 0.56) in kainate and 0.43 pS (+/ $-$ 0.16) in kainate/cGMP.Thus in the latter group, cGMP coapplication changed both theestimated conductance and the kinetics of the underlying kainateresponse.

Frequency analysis of the kainate noise and the kainate/cGMP noise for the cell in figure 5A indicated that its power spectrum(not shown) was not much affected by cGMP coapplication, eventhough the apparent conductance was decreased ~20%. The kainatenoise was fitted by the sum of two Lorentzian functions ( $tau$ ₁ =28.1 ms, S_0₁ = 91.8%; $tau$ ₂ = 1.3 ms, S_0₂ = 8.2%). After cGMP coapplication,these values were not particularly different ( $tau$ ₁ = 19.6 ms, S_0₁= 80.3%; $tau$ ₂ = 1.7 ms, S_0₂ = 19.7%). In contrast, the estimatedconductance for the cell depicted in figure 5B decreased by 78%,and cGMP changed its kinetics also (see fig. 6B).

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Fig. 6. Kinetics of cGMP-inhibited non-NMDA receptor channel noise in type II cells were modified by the presence of the antagonist. A) The spectrum for 100 µM kainate alone (panel A₁) was fitted by the sum of two Lorentzian functions as described in "Materials and Methods." In the presence of 500 µM cGMP (panel A₂), the shape of the spectrum was altered. It was now fitted with a single Lorentzian function with $tau$ = 1.2 ms, which suggests that this is the principal time constant of the cGMP-insensitive component of the kainate-activated noise. B) The power density spectrum of another cell in 100 µM kainate was also fitted by the sum of two Lorentzians. In this example, the power spectrum in cGMP/kainate resembled the one from the cell in panel A and again was fitted by a single time constant. This particular pair of spectra were generated from the responses exemplified by the raw data in figure 5B. We performed power density analysis of the underlying noise for kainate responses and of cGMP-insensitive and cGMP-sensitive fractions of kainate noise. All spectra shown have a control noise file of equal length subtracted from the response spectra. Control and agonist noise data were filtered at 1500 Hz (Butterworth) and sampled at 3000 Hz. The recordings were made at $-$ 60 mV.

Figure 6A and B and figure 7A show examples of pairs of power spectra from three different cells where cGMP coapplicationchanged the spectra. There are two alternative interpretationsof the affect on the power spectra: 1) cGMP inhibits a sensitivefraction of the kainate-activated receptor channels in cells containingmultiple non-NMDA receptor-channel types with different conductancesand kinetics. 2) The cGMP-mediated inhibition of the receptorchannels in these cells is not due to a simple competitive mechanism.

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Fig. 7. Additional examples of power spectra from low-noise kainate responses illustrate the kinetic diversity and varying degrees of cGMP sensitivity of the so-called type II cells. A) The noise in this cell was analyzed to determine the nature of the kinetics of cGMP-sensitive currents. In panel A₁, the spectrum shows that the noise in 100 µM kainate is fitted by the sum of two Lorentzians, and there is significantly more low-frequency noise in this spectrum than in many others shown in this report. In this cell, cGMP partially inhibited the kainate response, and the shape of the spectrum of the remaining noise (panel A₂) was different from the one obtained in kainate alone (panel A₁). Subtracting the cGMP/kainate spectrum (panel A₂) from the kainate spectrum (panel A₁) revealed the kinetics of the non-NMDA channels inhibited by cGMP in this cell (panel A₃). Both low and high frequencies were inhibited. The relatively cGMP-insensitive portion contained mainly the intermediate frequencies ( $tau$ = 3 ms). B) In this spectrum, from the patch in figure 5C, the kainate noise was fitted by the sum of two Lorentzians ( $tau$ ₁ = 95.4 ms, S_0₁ = 94.1%; $tau$ ₂ = 2.12 ms, S_0₂ = 5.9%). The coapplication of 500 µM cGMP did not change the amplitude of the kainate response more than 12.5%, nor did it change the shape of the spectrum remarkably (data not shown). However, the spectrum was no longer fit using our software, because it would not converge to the sum of two theoretical Lorentzian functions using the Simplex algorithm. Noise data were filtered at 1500 Hz (Butterworth) and sampled at 3000 Hz. The control files subtracted from the response files were of identical length. Recordings were made in cells voltage-clamped to $-$ 60 mV.

At the present time, we favor the first hypothesis rather than a noncompetitive mechanism of cGMP-mediated inhibition of somenon-NMDA receptor channels. The main reason for this is that thespectra taken from the cGMP-insensitive component of the kainatenoise are very similar (e.g., in fig. 6A₂ and B₂), which suggeststhat these cells contain a similar, relatively cGMP-insensitive,kainate-activated receptor channels. These spectra of the cGMP-insensitivekainate noise were fitted by a single Lorentzian function, andthey have essentially the same time constant (between 1.1 and1.3 ms). If there are populations of cGMP-insensitive, kainate-activatedchannels, as suggested by the type II responses, cells such asthose exemplified in figure 6 probably contain a mixture of non-NMDAreceptor channels, including variable amounts of the relativelycGMP-insensitive ones. The variance data in the presence of cGMPare consistent with the cGMP-insensitive receptor channels havingan estimated $gamma$ of 0.5 +/ $-$ 0.2 pS (n = 3).

The data in figures 6 and 7 also indicate that both the low-frequency and the high-frequency components of the kainate responsesin type II cells are sensitive to cGMP-mediated inhibition. Thisis illustrated by example in figure 7A where panel A₂ shows thespectrum obtained during the cGMP/kainate response. Subtractingthis spectrum from the one in kainate alone (fig. 7A₁) yieldsthe spectrum of the cGMP-sensitive noise shown in figure 7A₃,which was fitted by the sum of two Lorentzians with time constantsof ~24 ms and 0.5 ms. The noise remaining in the cGMP/kainatenoise spectrum was also fitted by two Lorentzians, but only theintermediate-frequency range (1-3 ms) could be fitted with somecertitude, because there was insufficient power remaining in thelow-frequency component to provide a meaningful measurement ofits time constant.

Finally, the kainate power spectra from the two minimally inhibited cells did not much resemble each other. Whereas one hada power spectrum very similar to figure 6A₂ and B₂, the secondone gave the power spectrum shown in figure 7B. Taken together,the spectral analysis data suggest there is likely to be additionaldiversity among the cGMP-insensitive non-NMDA channels.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Diverse expression of kainate-activated receptor channels in cerebellar granule cells. Noise analysis of the kainate-activated responses from cultured mouse cerebellar granule cells points out the diversity ofthese small neurons with respect to their expression of functionalnon-NMDA receptor channels. Variance analysis suggested that therewere at least two different groups of cells, those with high-noisekainate responses (5.51 +/ $-$ 0.83 pS) and a second group with low-noiseresponses (0.88 +/ $-$ 0.55 pS), referred to respectively as typeI and type II cells. Surprisingly, none of the 26 cells analyzedhad estimated conductances between 2 and 4 pS, which suggeststhat there may be two distinct populations of cells. Preliminaryconcentration-effect studies also suggest that the non-NMDA receptorsin type I cells may be more sensitive to kainate than those intype II cells. However, the differences in the effects of cGMPon low-noise kainate responses indicate that the hypothesis ofthere being two distinct populations of granule cells is too simple.

Extracellular cGMP inhibits kainate responses. Extracellular application cGMP to cerebellar granule cells demonstrated that this nucleotide inhibits kainate responses ina concentration-dependent fashion in the majority of neurons tested.In the case of the high-noise kainate responses, and also in theoutside-out patches from Purkinje neurons, cGMP appears to bea weak competitive antagonist. The classical approach of comparingcomplete concentration-effect curves in the absence of the inhibitor,and observing a rightward shift in the curve in the presence ofthe cGMP, was not pursued here because of the technical problemsassociated with gathering such data from cells 4 to 6 µm in diameter.The conclusion that cGMP acts as a competitive inhibitor of thehigh-noise kainate responses is based on several observations:1) The inhibition was voltage-independent. 2) The conductanceof kainate-activated channels, estimated by variance analysis,is unchanged. 3) The kinetics of the agonist noise in the powerspectra are unaffected by cGMP. 4) cGMP-mediated inhibition wasovercome by increasing the kainate concentration.

In contrast, the effects of cGMP on the low-noise kainate responses observed in some granule cells were more diverse and suggestthat some non-NMDA receptor channels are not sensitive to guanosinenucleotides. Although the highly reproducible inhibition of higher-noiseresponses by cGMP was by a competitive mechanism, the effectsof cGMP on the low-noise cells are not always consistent withcompetitive inhibition, unless some of the granule cells withlow-noise kainate responses contained both cGMP-sensitive andcGMP-insensitive kainate-activated receptor channels.

It is highly unlikely that cGMP exerts the inhibitory effects described in this report by diffusing through the membrane andacting on the inside. For a polar molecule like cGMP to diffuseinto and out of the cell or patch by traversing the membrane wouldrequire time. This would be manifest as delays in the on and offrates of the cGMP-mediated inhibition of kainate responses. Suchdelays were not observed here, where the on and off rates forcGMP effects were comparable to the on and off rates of kainateresponses when the agonist was applied alone. The possibilitythat guanosine nucleotides may also act at intracellular sitesof kainate-activated ion channels, or upon other effectors insidethe cell, given the opportunity, is not excluded by the experimentspresented here.

Does extracellular cGMP play a physiological role in cerebellum? The direct inhibition of non-NMDA receptor-mediated responses by cGMP requires relatively high concentrations (100-1000 µM),which raises the question of what, if any, physiological roleextracellular cGMP may play. The most recent estimates from invivo microdialysis studies in rat cerebellum indicate the basalextracellular cGMP to be ~200 nM (Luo et al., 1994). Two groupshave reported large increases in extracellular cGMP levels invivo, in rat hippocampus stimulated with NO donor agents (Vallebuonaand Raiteri, 1994) and in rat cerebellum after harmaline stimulationof climbing fiber input (Luo et al., 1994). The cerebellum studyis of particular interest, because although the increase in extracellularcGMP measured by microdialysis was more modest (about a 5-foldincrease above the basal level) compared with the hippocampalstudy, the cGMP release was inhibited by local TTX and nifedipineinfusion, and it was mimicked by direct application of NMDA andnon-NMDA agonists in the presence of TTX. Luo et al. (1994) alsoindicated that the increase in extracellular cGMP was rapid andtransient, which suggests that cGMP may be released from Purkinjeneurons. They did not speculate on the nature of the release mechanismbut implied that it is more rapid than a purely diffusional process.

Our findings suggest that extracellular cGMP is not likely to affect membrane potential directly. However, if it were releasedtransiently and reached sufficiently high extracellular concentrationduring neural activity in the cerebellum, it could serve a regulatoryfunction by feeding back onto granule cells and the parallel fiberinput to Purkinje cells, turning down the gain of these excitatoryinputs to Purkinje neurons. In such a case, stimulated releaseof cGMP would make extracellular cGMP a candidate chemical mediatorin the LTD-like phenomenon, as was reported in cerebellar Purkinjeneurons exposed to cGMP analogs (Shibuki and Okada, 1991

; Danielet al., 1993

). The suppression reported here of glutamate receptor-mediatedresponses by extracellular cGMP points to the necessity, wheninvestigating the role of cGMP in the LTD phenomenon, of excludingthe possibility that the reagents used to increase intracellularcGMP inhibit glutamate receptors directly.

What is the site of the competitive cGMP interaction? Ionotropic glutamate receptors and kainate binding proteins are thought to have a large extracellular N-terminal "lobe," threetransmembrane spanning portions and a cytoplasmic C-terminal (Hollmannet al., 1994; Wo and Oswald, 1994, 1995). The hypothesized sitesof ligand-receptor interaction include portions of the N-terminallobe and the extracellular loop between transmembrane spanningregions 3 and 4, which suggests that the agonist may span a pocketbetween the two lobes during binding (Stern-Bach et al., 1994;Mano et al., 1996).

In the context of an extensive mutagenesis study, which included changes in 43 positions in the putative excitatory aminoacid binding domain of a kainate binding protein, Paas et al.(1996b)

concluded that the main non-NMDA ligands, glutamate andkainate, interact with different amino acids in overlapping butnot identical binding pockets. In their study, the competitivenon-NMDA antagonist, CNQX interacted with one amino acid commonto both of the agonists and strongly with a single proline (P)residue within the binding pocket. Alanine (A) substitution atthis P had no effect on the binding of any of the agonist molecules,however. Thus competitive antagonists and agonists need not interactwith identical sites in kainate binding proteins, and they probablydo not do so in the non-NMDA receptor-channel subunits either,because the key amino acids in the primary sequence are conservedin both kainate and AMPA glutamate receptor subfamilies.

In their effort to localize the site of guanosine nucleotide interaction, Gorodinsky et al. (1993)

postulated that the nucleotidesmay bind to a site that shares partial homology to a glycine-richmotif (GxGxxG) found in G proteins and kinases. Paas et al. (1996a)

carried this hypothesis further in the wild-type chick cerebellarkainate binding protein, observing that photoaffinity-labeled[³²P]GTP interacted with an amino acid motif (aspartate-glycine-lysine-tyrosine-glycine:DGKYG) similar to the nucleotide binding sites in G proteins anda micromolar affinity for [³²P]GTP binding. This DGKYG motif, located in the extracellularN-terminal lobe portion of the non-NMDA and kainate binding proteinbinding pocket studied by Paas et al. (1996b)

, is highly conservedin non-NMDA ionotropic glutamate receptors except for the KA₁and KA₂ subunits (Werner et al., 1991

; Herb et al., 1992

; Kambojet al., 1992

; 1994

), which may account for our observation thatnot all kainate responses in cerebellar neurons were equally inhibitedby cGMP. Point mutations in the DGKYG sequence confirmed thatalanine (A) substitution of the lysine (K72/A) and tyrosine (Y73/A)residues modified GTP displacement of [³H]kainate binding, and the Y73/A mutation decreased [³H]kainate binding affinity, but the K72/A substitution did not(Paas et al., 1996a

Pharmacology of the cGMP binding site. There appears to be at least one common determinant of guanosine nucleotide binding across the kainate binding proteins andnon-NMDA receptor subunits. In addition to observing comparableIC₅₀ values for the guanosine nucleotides (GTP, GDP, GMP and cGMP)in a crude synaptosome preparation, Poulopoulou (1994) found thatthe structurally related molecule theophylline also weakly inhibited[³H]kainate binding to rabbit cerebellar membranes. Preliminaryelectrophysiology experiments indicated that GTP and theophyllinealso inhibited kainate responses recorded in cerebellar cells,a result consistent with the pharmacological profile obtainedin binding assays (Poulopoulou, 1994). Although the guanosinecompounds and the methyl-xanthine compete for [³H]kainate binding in rabbit cerebellar membranes, none of theadenosine purine analogs affected the radioligand binding, whichsuggests that the double-bonded oxygen on the pyrimidine ringof the purine base imparts the selectivity of the guanosine nucleotidesfor interaction with the non-NMDA glutamate receptor subunit bindingsite (Poulopoulou, 1994). Paas et al. (1996a) compared the affinityof adenosine nucleotides and inosine to the guanosine nucleotidesand concluded that the double-bonded oxygen on the guanosine baseis important for the observed pharmacological selectivity forguanine nucleotides in kainate binding proteins. Paas et al. (1996a)also observed that GTP and GDP had higher affinity than cGMP forthe triton X-100-treated receptors and postulated that the presenceof at least one free phosphate moiety increased the affinity ofthe guanosine nucleotides over that of cGMP and guanosine. However,in the rabbit brain membranes, GTP and cGMP were of equally lowaffinity, a phenomenon that reflects either some GTPase activityin preparation or a difference between non-NMDA receptors andkainate binding proteins.

In this regard, it is not clear how far this "G protein-like" model for the guanosine nucleotide binding site should be pushedfor the non-NMDA receptors. In the structurally well-characterizedG proteins, the free phosphates of GTP and GDP would interactwith the lysine in the glycine-rich motif while the base makesa "stacking" interaction with a phenylalanine that is 11 aminoacids carboxy to the lysine (Valencia et al., 1991

). In non-NMDAreceptors and the kainate binding proteins, there is a conservedmethionine at this position; however, it is located outside thepostulated agonist binding pocket (Paas et al., 1996b

). Returningto the specific requirement for the position-6 double-bonded oxygenin the base to confer the selectivity for guanosine over adenosinenucleotides in both the kainate binding proteins and the non-NMDAreceptors, it seems more likely that the negative charge of thisoxygen forms a hydrogen bond with the lysine and or tyrosine residuesin the conserved DGKYG motif, if this is the indeed the site ofthe guanosine interaction underlying the functional competitiveinhibition. This interaction would be consistent with the essentiallycomparable binding affinities for cGMP and GTP observed in rabbitcerebellar membranes, which, like other mammalian brains, undoubtedlyexpress many different non-NMDA receptor subunits but probablylack the kainate binding proteins altogether (Sprengel and Seeburg,1995

	Acknowledgments

We thank Drs. Richard A. Cerione and Nicolas Nassar for helpful discussions and the Department of Pharmacology for supplementalsalary support for Dr. Poulopoulou.

	Footnotes

Accepted for publication March 31, 1998.

Received for publication October 13, 1997.

¹ This work was supported successively by NS 24467 and NS 33166 to L.M.N.

² Present Address: Athens University Medical School, Department of Neurology, Egimition Hospital, Vas. Sofias 72, Athens, GREECE11528.

Send reprint requests to: Linda M. Nowak, Ph.D., C3-117 Veterinary Medical Center, Department of Pharmacology, Cornell University, Ithaca, NY 14853.

	Abbreviations

AMPA, $alpha$ -amino-3-hydroxy-5-methylisoxazole-4-propionic acid; CNQX, 6-cyano-7-nitroquinoxaline-2,3-dione; cGMP, 3',5' cyclic guanosine monophosphate; 8-Br-cGMP, 3',5' cyclic 8-bromo-guanosine monophosphate; FUDR, the mitotic inhibitors 5-fluoro-2'-deoxyuridine and uridine; LTD, long-term depression; MEM, minimal essential medium; NMDA, N-methyl-D-aspartate; NO, nitric oxide; NOS, nitric oxide synthase; $gamma$ , estimated single-channel conductance; i_e, elementary single-channel current amplitude; $sigma$ ², variance; pS, picosiemens; TTX, tetrodotoxin; V_R, reversal potential of the agonist response; V_H, membrane holding potential.

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Extracellular 3',5' Cyclic Guanosine Monophosphate Inhibits Kainate-Activated Responses in Cultured Mouse Cerebellar Neurons1

Extracellular 3',5' Cyclic Guanosine Monophosphate Inhibits Kainate-Activated Responses in Cultured Mouse Cerebellar Neurons¹