cAMP-Dependent Long-Term Potentiation of Nitric Oxide Release from Cerebellar Parallel Fibers in Rats

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(L)-ARGININE
NITRIC OXIDE

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The Journal of Neuroscience, November 1, 1998, 18(21):8551-8558

cAMP-Dependent Long-Term Potentiation of Nitric Oxide Release from Cerebellar Parallel Fibers in Rats
Shinji Kimura¹^,², Seiji Uchiyama², Hideaki E. Takahashi², and Katsuei Shibuki¹
¹ Department of Neurophysiology, Brain Research Institute, and ² Department of Orthopedic Surgery, School of Medicine, Niigata University, Niigata 951-8585, Japan

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Nitric Oxide (NO) is released from parallel fibers (PFs) after PF stimulation. NO-cGMP signaling is essential for long-termdepression (LTD) in cerebellar PF-Purkinje cell synapses, whichalso exhibit presynaptic long-term potentiation (LTP) after tetanicPF stimulation. This LTP is dependent on cAMP but not NO-cGMPsignaling. In this study, we analyzed long-term changes of NOrelease from PFs in rat cerebellar slices using electrochemicalNO probes. Repetitive PF stimulation at 10 Hz for 2 sec eliciteda transient increase in NO concentration (2.2 ± 0.1 nM; mean ±SEM; n = 116). This NO release exhibited long-term potentiation(LTP_NO) by 36 ± 3% (n = 15) after tetanic PF stimulation. Inductionof LTP_NO was not affected by Glu receptor antagonists. NO releasefrom PFs was also potentiated by L-Arg (ARG) (100 µM), forskolin(50 µM), and 8-bromo-cAMP (Br-cAMP) (1 mM) but not by 1,9-dideoxyforskolin(50 µM), a biologically inactive analog of forskolin. The potentiationinduced by forskolin was significantly suppressed by H89 (10 µM),a blocker of cAMP-dependent protein kinase. The potentiation inducedby forskolin, but not that induced by Arg, interfered with LTP_NO.H89 (10 µM) and KT5720 (1 µM), another blocker of cAMP-dependentprotein kinase, but not KT5823 (300 nM), a blocker of cGMP-dependentprotein kinase, significantly suppressed LTP_NO. These data indicatethat neural NO release is under activity-dependent control, justas synaptic transmitter release is. LTP_NO might play a role incross talk between presynaptic and postsynaptic plasticity byfacilitating NO-cGMP-dependent postsynaptic LTD after inductionof cAMP-dependent presynaptic LTP and LTP_NO.

Key words: nitric oxide; cAMP; cGMP; long-term potentiation; cerebellum; parallel fiber

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
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Discussion
References

Nitric oxide (NO) has various biological functions (Bredt and Snyder, 1994). Induction of long-term potentiation (LTP) inthe hippocampal area CA1 is facilitated by NO (Böhme et al.,1991; Schuman and Madison, 1991; Arancio et al., 1996; Son etal., 1996), although the NO dependence is affected by variousexperimental conditions, such as temperature or animal age (Williamset al., 1993). Induction of LTP in layer II/III in the visualcortex does not depend on NO signaling (Kirkwood and Bear, 1994),whereas induction of LTP in layer V of the medial frontal cortexdoes (Nowicky and Bindman, 1993). Cerebellar long-term depression(LTD) in parallel fiber (PF)-Purkinje cell synapses is also dependenton NO-cGMP signaling for the induction (Crepel and Jaillard, 1990;Ito and Karachot, 1990; Shibuki and Okada, 1991; Daniel et al.,1993; Lev-Ram et al., 1995; Hartell, 1996a), whereas NO does notaffect LTD of Glu-induced currents in cultured Purkinje cells(Linden et al., 1995) or LTD elicited by strong PF stimulation(Hartell, 1996b). Certain types of cerebellar motor learning,for which LTD is regarded as the cellular mechanism (Ito, 1989),are also dependent on NO signaling (Nagao and Ito, 1991; Li etal., 1995; Yanagihara and Kondo, 1996). These studies stronglysuggest that NO is a modulator of synaptic plasticity.

Of the isozymes of NO synthase (NOS), the neuronal type (nNOS) is widely distributed in the brain (Bredt et al., 1991). ThenNOS activity is controlled by neural activities via Ca²⁺-calmodulin (Bredt and Snyder, 1990). The nNOS molecule has severalphosphorylation sites so that the function of nNOS may be modulatedby phosphorylation (Brüne and Lapetina, 1991; Bredt et al., 1992).Although nNOS is a cytosolic enzyme, it has a high affinity forcertain molecules, such as postsynaptic density proteins (Brenmanet al., 1996a,b), and the intracellular distribution of nNOS mayaffect NO release. Activity-dependent changes in the distributionof nNOS immunoreactivity are found in the monkey visual cortex(Aoki et al., 1993). These data suggest the possibility that neuralNO release may be under activity-dependent control. In our previousstudy, a slight potentiation of NO release has been found aftertetanic PF stimulation (Shibuki and Kimura, 1997). The purposeof this paper is to study activity-dependent changes in NO releasefrom PFs.

The mechanism of NO-cGMP-dependent LTD in PF-Purkinje cell synapses is explained by desensitization of postsynaptic Glu receptors(Ito et al., 1982; Linden et al., 1991; Nakazawa et al., 1995).Glu release from PFs, however, shows presynaptic LTP after tetanicPF stimulation (Salin et al., 1996; Linden, 1997), and this presynapticLTP is dependent on cAMP but not cGMP (Salin et al., 1996). NOrelease in the molecular layer of the cerebellum is primarilyderived from PFs, and the NO release is triggered by Ca²⁺ influx via voltage-gated Ca²⁺ channels (Shibuki and Kimura, 1997), just as Glu release fromPFs is. Therefore, NO release from PFs may be modulated by cAMP.In this study, we investigate the roles of cyclic nucleotidesin NO release from PFs.

  MATERIALS AND METHODS

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Abstract
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Materials & Methods
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References

Slice preparations. Slices of the cerebellar vermis were prepared from Wistar rats of either sex (4-7 weeks old). The rat,anesthetized with ether, was immersed in ice-cold water, exceptfor the nose, for 3 min to reduce brain temperature. Immediatelyafter decapitation, the brain was removed, and coronal slices(400-µm-thick) of cerebellar vermis were prepared with a microslicer(DTK-2000; Dosaka, Osaka, Japan). The obtained slices were incubatedin an artificial medium bubbled with 95% O₂ and 5% CO₂. The compositionof the medium was (in mM): NaCl 124, KCl 5, NaH₂PO₄ 1.24, MgSO₄1.3, CaCl₂ 2.4, NaHCO₃ 26, and glucose 10, unless otherwise specified.When the Ca²⁺ concentration in the medium was changed, the sum of MgSO₄ andCaCl₂ concentrations was kept constant. After incubation at roomtemperature for more than 1 hr, the slices were transferred toa small recording chamber (~0.3 ml in volume) in which the sliceswere kept submerged. The recording chamber was maintained at 30°Cand was continuously perfused with the oxygenated medium at theflow rate of 1 ml/min. The experiments were performed accordingto the guidelines of Niigata University and had been approvedby the ethics committee of Niigata University.

Drugs. Forskolin was purchased from Wako Pure Chemical Industries (Osaka, Japan), and N^G-nitro-L-arginine (NA) was purchased from Sigma (St. Louis, MO).6-Cyano-7-nitroquinoxaline-2,3-dione (CNQX), D-2-amino-5-phosphonovalerate(APV), and (RS)- $alpha$ -methyl-4-carboxyphenylglycine (MCPG) were obtainedfrom Tocris Cookson (Bristol, UK). H89 and KT5720 were obtainedfrom Biomol Research Laboratory (Plymouth Meeting, MA), 1,9-dideoxyforskolinwas from Research Biochemicals (Natick, USA), and KT5823 was fromKyowa Medex (Tokyo, Japan). These drugs were applied to the slicesby adding into the perfusing medium.

NO probes. Electrochemical NO probes were fabricated as reported previously (Shibuki and Kimura, 1997). A glass pipette wasobliquely polished such that the diameter of the tip was ~250µm. After the edge was smoothed by flaming, the pipette was filledwith a solution containing 30 mM NaCl and 0.3 mM HCl. The tipwas sealed with a thin membrane of silicon rubber (TSE399; Toshiba).This membrane was prepared by placing a drop of TSE399 (~20-30µl) on the surface of water. This drop spread over the surfaceof the water and polymerized within 50 min. The glass pipettewas inserted slowly into the water through the silicon rubbermembrane so that the tip of the pipette was sealed with the siliconrubber membrane. The shank of the pipette was painted with a smallamount of TSE399 to ensure electrical insulation. The pipetteswere left for several hours to allow hardening of the siliconrubber. As a working electrode, Teflon-coated Pt wire (metal diameter,125 µm) was used. The tip was cut obliquely and heated in thetip of the flame of an ethyl alcohol lamp for a few seconds toremove the Teflon coating. The Pt wire, except at the tip, wasinsulated with heat-melted dental wax. The Pt wire was insertedinto the pipette. The tip was protruded from the pipette (seeFig. 2A). A reference (Teflon-coated Ag wire) was also insertedinto the pipette and was connected to the ground. The workingPt wire was connected to a current-voltage converter. The anodevoltage between the working Pt wire and the reference Ag wirewas maintained at +0.9 V. Each NO probe was calibrated by measuringthe probe currents in response to a 30 µM NO solution, which wasprepared by dissolving 36 µl of NO gas in 50 ml of degassed salinein a glass syringe. The sensitivity of the probes to NO was 0.2-1.1nA/µM NO at 30°C at the anode voltage of +0.9 V, and the CO sensitivityunder this condition was ~0.1% of the NO sensitivity. Usually,the NO probes could be used for more than a few weeks withoutsignificant changes in NO sensitivity.

Recording and stimulation. The PF volley potentials and field EPSPs elicited by PF stimulation were recorded extracellularlyon the cut surface of the molecular layer in the slices througha glass micropipette filled with 2 M NaCl. The field potentialswere elicited by single pulse stimulation at 12 sec intervalsor by train pulse stimulation at 10 Hz for 2 sec. The five traceselicited by a single pulse or 20 traces elicited by 10 Hz trainpulses were averaged to estimate the amplitude of the responses.The field EPSPs were isolated from the preceding PF volley potentialsby subtracting the trace recorded in the presence of 10 µM CNQXfrom that recorded before CNQX application.

PFs were stimulated with biphasic pulses through the cut end of a Teflon-coated Ag wire placed on the surface of the slices.AgCl was deposited on the surface of the Ag wire by passing positivecurrents through the stimulating electrode in a NaCl solution.Every negative stimulus pulse was followed by a positive pulse,the absolute amplitude of which was 5% larger than that of thepreceding negative pulse. Under these conditions, negative currentfrom the stimulating electrode was mediated by Cl dissociated from AgCl, and generation of H₂ gas, which interferedwith NO recording, was suppressed. The intensity of the negativestimulus pulse was 500 µA, unless otherwise specified. The durationof each pulse phase was 100 µsec. The tip of NO probe was placedon the surface of the molecular layer of cerebellar slices. Thedistance between the NO probe and the stimulating electrode was100-200 µm. Although NO release elicited by PF stimulation withsingle pulse is not detected with NO probes, the NO release exhibitsmarked frequency facilitation (Shibuki and Kimura, 1997). Therefore,we used PF stimulation with pulse trains at 10 Hz for 2 sec forevoking NO release from PFs. The pulse trains were applied toslices at 2 min intervals. After the amplitude of NO release wasstabilized, tetanic PF stimulation (TS) (5 pulses at 50 Hz, repeatedat 2 sec intervals for 10 min) was applied to the slices. Becausemild TS was not sufficient to potentiate NO release after theNO release elicited by 10 Hz stimulation was stabilized, we chosethis prolonged tetanus protocol. To estimate the effect of TSon NO release, the amplitude of NO release was normalized by theaveraged value in three consecutive traces recorded immediatelybefore TS. The amplitude of potentiation of NO release was evaluatedat 30 min after TS. Statistical significance between the datawere evaluated by the Mann-Whitney U test, unless otherwise specified.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

NO recording in cerebellar slices

NO release was recorded in the molecular layer of coronal cerebellar slices using an electrochemical NO probe placed on thesurface of the molecular layer (Fig. 1A). Repetitive PF stimulation(10 Hz for 2 sec) elicited a transient current increase in theNO probe (Fig. 1B). The current increase reached a peak between3.0 and 4.2 sec after initiation of the PF stimulation (peak amplitudelatency), and the time period during which the current changeexceeded half the amplitude of the peak (half amplitude duration)was between 3.1 and 4.3 sec (n = 116). We varied extracellularCa²⁺ concentrations between 0 and 3.0 mM. Amplitude of the currentin the NO probe was positively correlated with extracellular Ca²⁺ concentration (Fig. 1B). The current increase, which correspondedto 0.7-4.6 nM NO (2.2 ± 0.1 nM; mean ± SEM; n = 116), was completelyblocked by the addition of 10 µM NA, a specific NOS blocker, intothe medium perfusing the slice (Fig. 1C). These data indicatethat NO release from PFs was reflected in the increase of currentthrough the NO probe, as reported previously (Shibuki and Kimura,1997).

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Figure 1. NO release from PFs in coronal cerebellar slices. A, Schema showing the experimental setup. B, NO release elicited by repetitive PF stimulation (10 Hz for 2 sec) and recorded under different extracellular Ca²⁺ concentrations (0-3.0 mM) in a slice. C, Amplitude of NO release elicited by repetitive PF stimulation at 2 min intervals and blockade of NO release by 10 µM NA. Inset shows superimposed original traces recorded before (a) and during (b) NA application.

LTP of NO release from PFs

NO release elicited by repetitive PF stimulation exhibits gradual potentiation for 30-50 min after initiation of NO recording(Shibuki and Kimura, 1997). In this study, we observed similargradual potentiation after initiation of NO recording (Fig. 2A).TS (5 pulses at 50 Hz, repeated at 2 sec interval for 10 min)was applied to the slices after the amplitude of NO release wasstabilized. Potentiation of NO release was elicited by TS (Fig.2A). The maximal amplitude of this potentiation (67 ± 7%; n =15) was observed within a few minutes after cessation of TS. Subsequently,amplitude of NO release was gradually reduced. However, the potentiationlasted for >30 min (Fig. 2B), and the amplitude of potentiation30 min after cessation of TS was 36 ± 3% (n = 15). Neither thepeak amplitude latency nor half amplitude duration was changedby TS (Fig. 2A, inset). In the absence of TS, no clear potentiationof NO release was observed (Fig. 2B,a). PF volley potentials elicitedby a single pulse (n = 5) (Fig. 2B,b) or the averaged potentialsof 20 traces elicited by PF stimulation at 10 Hz for 2 sec (n= 5) (Fig. 2B,c) exhibited no potentiation after TS. These datastrongly suggest that LTP_NO was elicited by TS.

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Figure 2. LTP_NO elicited by TS. A, Amplitude of NO release recorded before and after TS. Inset shows superimposed traces of NO release recorded at the initiation of recording (a), immediately before initiation of TS (b), immediately after cessation of TS (c), and 30 min after cessation of TS (d). B,a, Time course of relative NO release before and after TS (filled circles) or in the absence of TS (open circles). B,b, Averaged PF volley potentials elicited by single pulse stimulation immediately before initiation and 30 min after cessation of TS (asterisk). B,c, Averaged PF volley potentials elicited by 10 Hz train pulses immediately before initiation and 30 min after cessation of TS (asterisk). C, Changes in NO release (hatched bars) and field EPSPs (filled bars). Gradual potentiation during the initial 50 min of the recording (Gradual), TS-induced potentiation (TS), the reduction caused by the change in stimulus intensity from 500 to 400 µA (Stimulus), and the reduction caused by the change in extracellular Ca²⁺ concentration from 2.4 to 1.8 mM (Ca2+) are shown. The amplitude of each change was normalized by the amplitude of NO release or field EPSPs recorded before the change occurred. Each bar and error bar represent the absolute value of the mean ± SEM of five experiments. Except for the experiment in which extracellular Ca²⁺ concentration was decreased, NO release and field EPSPs were simultaneously recorded in the same slice, as shown by the inset.

Presynaptic LTP of Glu release is also elicited by TS (Salin et al., 1996). Therefore, field EPSPs in Purkinje cells and NOrelease were simultaneously recorded at the both sides of singlestimulating electrode in five slices (Fig. 2C, inset). Duringthe initial 50 min of recording, NO release was gradually potentiatedby 28 ± 6% (n = 5), whereas the averaged field EPSPs of 20 traceselicited by PF stimulation at 10 Hz for 2 sec exhibited only modestpotentiation (8 ± 9%; n = 5) (Fig. 2C). TS elicited LTP_NO by 38± 7% in the five slices, whereas no clear potentiation of theaveraged field EPSPs were observed after TS (Fig. 2C). The differencein the TS-induced potentiation between NO release and averagedfield EPSPs was significant (p < 0.05; Wilcoxon signed rank test).Similar discrepancy between NO release and field EPSPs was alsofound in the experiments in which the stimulus intensity was decreasedfrom 500 to 400 µA (n = 5), or the Ca²⁺ concentration in the perfusing medium was decreased from 2.4to 1.8 mM (n = 5) (Fig. 2C). The reduction of NO release was significantlylarger than that of the field EPSPs in these experiments (p <0.05 for both experiments; Wilcoxon signed rank test). These resultsstrongly suggest that field EPSPs were saturated under the experimentalconditions used for recording LTP_NO. Therefore, we reduced theintensity of PF stimulation from 500 to 50 µA so that only fieldEPSPs were recorded clearly (data not shown). However, the fieldEPSPs elicited by test stimuli of 10 Hz for 2 sec exhibited almostno change after TS at the stimulus intensity of 50 µA, and theamplitude of the averaged field EPSPs 30 min after cessation ofTS was 99 ± 3% (n = 5) of that recorded immediately before TS.

In the molecular layer, PFs make synapses with neurons, among which basket neurons express nNOS (Bredt et al., 1991). To ascertainthe possible contribution of postsynaptic neurons of PFs to LTP_NO,we applied CNQX (10 µM), an antagonist of non-NMDA receptors.However, amplitude of NO release was not clearly affected by CNQX(Fig. 3A), suggesting that most of the NO was derived from PFs.Furthermore, LTP_NO was elicited by TS in the presence of 10 µMCNQX. Although LTP_NO was slightly reduced in the presence of 10µM CNQX, no significant difference was found in the LTP_NO amplitudeelicited in the absence or presence of 10 µM CNQX (Fig. 3D). Westudied the contribution of other Glu receptors to the inductionof LTP_NO. However, LTP_NO amplitude was significantly affectedby neither APV (50 µM), a blocker of NMDA receptors, nor MCPG(500 µM), a blocker of metabotropic Glu receptors (Fig. 3B-D).Simultaneous application of CNQX and MCPG, both of which blockpostsynaptic Glu receptors in Purkinje cells, was also ineffective(Fig. 3D).

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Figure 3. Effects of Glu blockers on LTP_NO. A, Amplitude of NO release recorded before, during, and after application of CNQX (10 µM) and TS. Insets show superimposed traces recorded immediately before application of CNQX (a) or TS (b) and 30 min after cessation of TS (c). B, Superimposed traces recorded before and 30 min after TS (asterisk), which was applied to the slice in the presence of 50 µM APV. C, Traces recorded before and 30 min after TS (asterisk) applied in the presence of 500 µM MCPG. D, Amplitude of control LTP_NO and LTP_NO elicited in the presence of 10 µM CNQX, 50 µM APV, 500 µM MCPG, or 10 µM CNQX plus 500 µM MCPG. The mean ± SEM are shown.

NO is produced from L-arginine (Arg). NO release from PFs was augmented by the addition of Arg into the perfusing medium ina dose-dependent manner (Fig. 4A). The augmentation of the NOrelease by Arg reached a plateau at an Arg concentration of 100µM (Fig. 4A). Because this augmentation by 100 µM Arg (41 ± 8%;n = 5) is comparable with the LTP_NO amplitude, the mechanism ofLTP_NO might involve augmentation of Arg supply to PFs. To investigatethis possibility, induction of LTP_NO was tested in the presenceof 100 µM Arg (Fig. 4B,C). However, the LTP_NO amplitude (35 ±4%; n = 5) was not significantly different from that in normalmedium (Fig. 4C), suggesting that the mechanism of LTP_NO probablydoes not involve augmentation of Arg supply to PFs.

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Figure 4. LTP_NO in the presence of excessive Arg. A, Dependence of the amplitude of NO release on Arg concentration in the perfusing media. Data represent the mean ± SEM of five experiments. The values are normalized by that recorded in the perfusing medium not containing Arg. Inset shows superimposed traces recorded in a slice in perfusing media containing 0-100 µM Arg. B, Changes in amplitude of NO release elicited by 100 µM Arg application and TS. Inset shows superimposed traces recorded immediately before Arg application (a), immediately before initiation (b), and 30 min after cessation of TS (c). C, Time courses of LTP_NO in the presence (open circles) or absence of 100 µM Arg (filled circles).

Dependence of the induction of LTP_NO on cAMP

Presynaptic LTP of Glu release from PFs is dependent on cAMP (Salin et al., 1996). Therefore, we studied the effect of forskolin,an activator of adenylate cyclase, on NO release from PFs. NOrelease exhibited potentiation after the addition of 50 µM forskolininto the perfusing medium (Fig. 5A). Potentiation of NO releaseoccurred gradually during forskolin application of 50 min. Themaximal amplitude of the potentiation was 62 ± 17% (n = 7), whichis comparable with the maximal amplitude of the potentiation elicitedby TS. The forskolin-induced potentiation continued even aftercessation of forskolin application, and the amplitude of the potentiation30 min after cessation of forskolin application was 56 ± 18% (n= 7). The corresponding potentiation elicited by forskolin was10 ± 12% (n = 5) in the presence of 10 µM H89, a blocker of cAMP-dependentprotein kinase, and this value was significantly smaller thanthat in normal medium (p < 0.05) (Fig. 5A). Furthermore, the amplitudeof the potentiation observed 30 min after cessation of the applicationof 1,9-dideoxyforskolin (50 µM for 50 min), a biologically inactiveforskolin analog, was only 1 ± 4% (n = 5) (Fig. 5B) and was significantlysmaller than that observed after forskolin application (p < 0.001).These results strongly suggest that the forskolin-induced potentiationof NO release is mediated by cAMP.

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Figure 5. Potentiation of NO release induced by forskolin (FSK) and a cAMP analog. A, Potentiation of NO release induced by 50 µM forskolin (filled circles). Inset shows superposed traces recorded before application of forskolin (a), in the presence of forskolin (b), and 30 min after the cessation of forskolin application (c). Forskolin-induced potentiation in the presence of 10 µM H89 is also shown (open circles). In this experiment, slices were incubated with 10 µM H89 for at least 2 hr before and throughout the recording. B, Potentiation of NO release induced by forskolin and TS (filled circles). Inset shows traces recorded before application of forskolin (a), before initiation of TS (b), and 30 min after the cessation of forskolin application and TS (c). Changes in NO release elicited by application of 1,9-dideoxyforskolin (50 µM, DideoxyFSK) are also shown (open circles). C, Potentiation of NO release induced by 1 mM Br-cAMP (horizontal bar). D, Effect of 1 mM Br-cGMP (horizontal bar) on NO release.

We speculated that forskolin-induced potentiation of NO release may share the mechanism with that of LTP_NO elicited by TS.To investigate this possibility, TS was applied to the slicesduring forskolin application. However, TS elicited only transientpotentiation of NO release (Fig. 5B), and the maximal amplitudeof the potentiation elicited by TS during forskolin application(78 ± 5%; n = 5) was comparable with that elicited by TS alone(67 ± 7%; n = 15). Furthermore, the amplitude of the potentiation30 min after cessation of forskolin application and TS together(57 ± 9%; n = 5) was not significantly different from the amplitudeof the potentiation elicited by forskolin alone (56 ± 18%; n =7). These findings are well explained if forskolin-induced potentiationand TS-induced LTP_NO share the same molecular mechanism.

To study the relationship between NO release and cAMP further, we applied 8-bromo-cAMP (Br-cAMP), a membrane-permeable analogof cAMP, to the slices (Fig. 5C). During the application of 1mM Br-cAMP, NO release was reduced by 28 ± 4% (n = 5). However,NO release recovered after washing out the Br-cAMP, and substantialpotentiation of NO release (19 ± 5%) was observed 30 min aftercessation of Br-cAMP application (Fig. 5C). In contrast, 8-bromo-cGMP(Br-cGMP) (1 mM), a membrane-permeable analog of cGMP, exhibitedalmost no effect on NO release (Fig. 5D), and there was a significantdifference in the amplitude of potentiation elicited by Br-cAMPand Br-cGMP (p < 0.03).

The facilitatory effect of cAMP on the induction of presynaptic LTP is blocked by H89 or KT5720, another blocker of A kinaseA (Weisskopf et al., 1994; Salin et al., 1996). Therefore, westudied LTP_NO in slices incubated with 10 µM H89 or 1 µM KT5720.Although TS elicited transient potentiation of NO release, amplitudeof the potentiation 30 min after cessation of TS was 2 ± 3% (n= 5) in the presence of 10 µM H89 and 12 ± 3% (n = 5) in the presenceof 1 µM KT5720 (Fig. 6A). These values were significantly smallerthan those recorded in slices incubated in normal medium (p <0.005 for both data). As control, we studied LTP_NO in the slicesincubated with 300 nM KT5823, a specific blocker of G kinase andNO-cGMP-dependent LTD (Ito and Karachot, 1992; Hartell, 1996a).However, no apparent effect of KT5823 on LTP_NO was found (Fig.6A). The amplitude of LTP_NO elicited by TS in the presence ofKT5823 (36 ± 4%; n = 5) was not significantly different from thatof LTP_NO elicited by TS in normal medium. These results, togetherwith the data obtained from the forskolin and Br-cAMP experiments,indicate that LTP_NO is dependent on cAMP but not on cGMP.

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Figure 6. Blockade of LTP_NO and gradual potentiation of NO release by H89 or KT5720. A, Time course of LTP_NO recorded in the presence of 10 µM H89 (open circles), 1 µM KT5720 (open circles), or 300 nM KT5823 (filled circles). B, Time courses of gradual potentiation of NO release induced by test stimuli in the absence (filled circles) or presence of 10 µM H89 (open circles). Slices were incubated with 10 µM H89, 1 µM KT5720, or 300 nM KT5823 for at least 2 hr before and throughout the recording.

Effect of H89 on the gradual potentiation of NO release

NO release from PFs exhibits marked frequency facilitation (Shibuki and Kimura, 1997). In this study, we adopted PF stimulationof 10 Hz pulse trains to elicit clear NO release for quantitativeanalysis. Because repetitive PF stimulation at 8 Hz is sufficientto elicit LTP of Glu release from PFs (Salin et al., 1996), weexpected that PF stimulation at 10 Hz may be sufficient to elicitpotentiation of NO release from PFs. In accordance with this expectation,we observed the gradual potentiation during a period of 30-50min after initiation of NO recording (Figs. 2A, 6B). We recordedthe gradual potentiation in the slices incubated with 10 µM H89(Fig. 6B). The amplitude of the gradual potentiation during theinitial 1 hr of NO recording was 9 ± 4% (n = 6), and this valuewas significantly smaller than that recorded in normal medium(43 ± 10%; n = 7; p < 0.02). This result suggests that repetitivePF stimulation at 10 Hz is sufficient to elicit potentiation ofNO release in a cAMP-dependent manner.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

LTP of NO release from PFs

In this study, we used an electrochemical NO probe whose tip was covered by a thin rubber membrane (Shibuki, 1990; Shibukiand Okada, 1991; Shibuki and Kimura, 1997). Because neither currentnor electrolytes are released from the tip of the probe to thesurrounding space, NO recording using this NO probe is suitablefor detecting long-term changes in NO release without damagingtissue. In our previous study, we detected NO release from PFselicited by PF stimulation using this probe (Shibuki and Kimura,1997). The release of NO was identified by the characteristicdependency of the responses on the anode voltage in the probeand the sensitivity to NA. Furthermore, we found that NO releasefrom PFs elicited by 20 Hz PF stimulation was slightly potentiatedafter TS (Shibuki and Kimura, 1997). However, the amplitude ofthe potentiation 30 min after cessation of TS was only ~10%, andtherefore further analysis was not practicable. In this study,we adopted 10 Hz PF stimulation as test stimuli, and the amplitudeof potentiation 30 min after cessation of TS was increased to36 ± 3% (n = 15). This potentiation is not attributed to changesin the sensitivity of the NO probe, which usually showed stabilityfor more than a few weeks. The probe currents elicited by PF stimulationwere completely blocked by 10 µM NA, even after TS (data not shown),and therefore the changes in the probe current must reflect netchanges in NO concentration. Suppression of degradation of NOis unlikely to be caused by TS, because the time course of theprobe currents was not changed by TS (Fig. 2A, inset). No clearpotentiation of NO release was observed in the absence of TS (Fig.2B,a). Amplitude of PF volley potentials was not potentiated byTS (Fig. 2B,b), and therefore changes in tissue excitability cannotexplain the potentiation of the probe current. From these results,it is concluded that LTP_NO is elicited by TS in cerebellar slices.

Comparison between LTP_NO and cAMP-dependent presynaptic LTP

Although NO release is not dependent on exocytosis, Ca²⁺ influx via voltage-gated Ca²⁺ channels triggers not only Glu release but also NO release fromPFs. Therefore, comparison of NO release and EPSPs in Purkinjecells may be of interest. The filed EPSPs simultaneously recordedwith LTP_NO exhibited no clear potentiation after TS. This resultand the similar discrepancy regarding the dependency on extracellularCa²⁺ concentration or stimulus intensity indicate that field EPSPswere saturated at the stimulus intensity of 500 µA, which wasused for recording LTP_NO. The amplitude of PF volley potentialsis almost linearly correlated to the stimulus intensity up to500 µA under our experimental conditions (Shibuki and Kimura,1997). Therefore, the saturation of field EPSPs at 500 µA cannotbe attributable to saturated PF excitation but is probably explainedby saturated postsynaptic depolarization. At the stimulus intensityof 50 µA, however, field EPSPs elicited by test stimuli of 10Hz for 2 sec exhibited almost no change after TS, suggesting thatLTP_NO and LTP of field EPSP may not necessarily occur in parallel.

In the hippocampus, there are two typical types of LTP (Bliss and Collingridge, 1993; Nicoll and Malenka, 1995). LTP in CA1pyramidal neurons requires postsynaptic Ca²⁺ rise for the induction, whereas presynaptic LTP in mossy fiber-CA3pyramidal neuron synapses does not require synaptic transmissionand postsynaptic increase in Ca²⁺ concentration for the induction (Castillo et al., 1994; Weisskopfet al., 1994). Presynaptic LTP in sympathetic ganglion synapses(Kuba and Kumamoto, 1986), the mossy fiber synapses (Weisskopfet al., 1994), and cerebellar PF-Purkinje cell synapses (Salinet al., 1996) are dependent on cAMP for induction. LTP_NO was elicitedin the presence of Glu receptor antagonists (Fig. 3) and is unlikelyto be dependent on increase in Ca²⁺ concentration in postsynaptic neurons of PFs. The induction ofLTP_NO was dependent on cAMP and activation of kinase A (Figs.5, 6). These characteristics of LTP_NO are similar to those ofcAMP-dependent presynaptic LTP.

Possible molecular mechanism for LTP_NO

Electrical white matter stimulation causes an increase in the Arg level in rat cerebellar slices (Hansel et al., 1992). Inthe molecular layer, Arg is predominantly localized in Bergmannglial cells (Aoki et al., 1991). Glial synaptic currents exhibitLTP after repetitive stimulation of granule cells (Linden, 1997).Application of Arg to the slices potentiated NO release from PFs(Fig. 4A). Therefore, activity-dependent changes in Arg supplymight be responsible for LTP_NO elicited by TS. However, this hypothesisdoes not seem likely, because the amplitude of LTP_NO elicitedin the presence of excess Arg was not significantly differentfrom that of LTP_NO elicited in normal medium (Fig. 4C). The primarystructure of nNOS has several phosphorylation sites that are recognizedby protein kinases (Bredt et al., 1992). However, activation ofA or C kinases does not potentiate nNOS activity (Brüne and Lapetina,1991; Bredt et al., 1992). Therefore, upregulation of Arg supplyor potentiation of nNOS activity by phosphorylation does not seemto be responsible for the induction of LTP_NO elicited by TS.

NO release from PFs is triggered by Ca²⁺ influx (Shibuki and Kimura, 1997), and NO release was positively correlated with extracellularCa²⁺ concentration (Fig. 1B). Therefore, upregulation of Ca²⁺ influx is a possible mechanism for LTP_NO. Presynaptic LTP inthe mossy fiber synapses interferes with paired pulse facilitationor frequency facilitation of synaptic transmission (Weisskopfet al., 1994). However, presynaptic LTP, but not paired pulsefacilitation or frequency facilitation, is impaired in the Rab3A deficient mice (Castillo et al., 1997). Rab 3A is a small G-proteininvolved in exocytosis of synaptic vesicles (Geppert et al., 1994,1997). Therefore, changes in Ca²⁺ influx may not be responsible for cAMP-dependent presynapticLTP, although Ca²⁺ influx is required for the induction (Castillo et al., 1994).Because NO release from PFs is also triggered by presynaptic Ca²⁺ influx (Shibuki and Kimura, 1997), changes in Ca²⁺ influx might not be responsible for LTP_NO.

Although nNOS is a cytosolic enzyme, it has affinity for specific molecules, such as postsynaptic density (PSD) proteins (Brenmanet al., 1996a,b). In the monkey visual cortex, monocular deprivationelicits a decrease in nNOS immunoreactivity in the axon terminalsin the corresponding cortical columns (Aoki et al., 1993). BecausePSD proteins are also found in the cerebellum (Brenman et al.,1996a,b), distribution of nNOS molecules might be inhomogeneousin granule cells, and activity-dependent changes in nNOS distributionin granule cells might be elicited by TS. It has been proposedthat exocytotic fusion is elicited by a very large and localizedincrease in Ca²⁺ concentration near the Ca²⁺ channels immediately after each action potential (Simon and Llinás,1985). The NO release from PFs was sensitively dependent on extracellularCa²⁺ concentration (Fig. 1B), and therefore even a slight change inthe distribution of nNOS molecules with respect to the locationof voltage-gated Ca²⁺ channels in PFs might be sufficient to modify NO release. However,no direct evidence supporting this presumption is available atpresent. Transmitter release is dependent on the complex mechanisms,including Ca²⁺-dependent exocytosis, whereas NO release from PFs is elicitedsimply by activation of nNOS via Ca²⁺-calmodulin. Therefore, understanding the mechanism for LTP_NOmight help the elucidation of the mechanism for presynaptic plasticity.

Physiological roles of LTP_NO

Although we used TS with 50 Hz pulses for induction of LTP_NO, gradual potentiation of NO release, which probably shares amolecular basis with LTP_NO, was elicited by 10 Hz PF stimulation.Because granule cells can fire at high frequency in vivo (Eccleset al., 1966), LTP_NO may be elicited in vivo. What is the physiologicalrole of LTP_NO in vivo? Cerebellar LTD in PFs-Purkinje cell synapsesis elicited by conjunctive stimulation of climbing fibers andPFs (Ito et al., 1982; Sakurai, 1987), and PF stimulation maybe replaced with application of NO (Lev-Ram et al., 1995). ThisLTD is thought to reflect desensitization of postsynaptic Glureceptors (Ito et al., 1982; Linden et al., 1991; Nakazawa etal., 1995). LTP of PF-Purkinje cell synapses is also elicitedby Br-cGMP when EGTA is injected into the Purkinje cells (Shibukiand Okada, 1992). Because soluble guanylate cyclase is localizedin Purkinje cells (Ariano et al., 1982), this LTP might be ofpostsynaptic origin. Presynaptic LTD has been demonstrated inthe mossy fiber synapses (Kobayashi et al., 1996; Yokoi et al.,1996). Because there is a similarity between presynaptic LTP inmossy fiber synapses and in PF-Purkinje cell synapses, PF-Purkinjecell synapses may also exhibit presynaptic LTD. Therefore, theoreticallyfour types of synaptic plasticity can be present in PFs-Purkinjecell synapses. Plasticity of NO release might serve as a coordinatorbetween presynaptic and postsynaptic plasticity in PF-Purkinjecell synapses. Changes in the ability to induce synaptic plasticityare known in various synapses, and these are referred to metaplasticity(Abraham and Bear, 1996). Dynamic changes in NO release couldcause metaplasticity in synapses that exhibit NO-dependent synapticplasticity.

  FOOTNOTES

Received Feb. 2, 1998; revised Aug. 3, 1998; accepted Aug. 10, 1998.

This work was supported by grants from the Japanese Government, Toyota RIKEN, and the Uehara Foundation. We thank Y. Tamuraand N. Taga for technical assistance.
Correspondence should be addressed to K. Shibuki, Department of Neurophysiology, Brain Research Institute, Niigata University,1 Asahi-machi, Niigata 951-8585, Japan.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Abraham WC, Bear MF (1996) Metaplasticity: the plasticity of synaptic plasticity. Trends Neurosci 19:126-130[Web of Science][Medline].
Aoki C, Fenstemaker S, Lubin M, Go CG (1993) Nitric oxide synthase in the visual cortex of monocular monkeys as revealed by light and electron microscopic immunocytochemistry. Brain Res 620:97-113[Web of Science][Medline].
Aoki E, Semba R, Mikoshiba K, Kashiwamata S (1991) Predominant localization in glial cells of free L-arginine. Immunocytochemical evidence. Brain Res 547:190-192[Web of Science][Medline].
Arancio O, Kiebler M, Lee CJ, Lev-Ram V, Tsien RY, Kandel ER, Hawkins RD (1996) Nitric oxide acts directly in the presynaptic neuron to produce long-term potentiation in cultured hippocampal neurons. Cell 87:1025-1035[Web of Science][Medline].
Ariano MA, Lewicki JA, Brandwein HJ, Murad F (1982) Immunohistochemical localization of guanylate cyclase within neurons of rat brain. Proc Natl Acad Sci USA 79:1316-1320[Abstract/Free Full Text].
Bliss TV, Collingridge GL (1993) A synaptic model of memory: long-term potentiation in the hippocampus. Nature 361:31-39[Medline].
Böhme GA, Bon C, Stutzmann JM, Doble A, Blanchard JC (1991) Possible involvement of nitric oxide in long-term potentiation. Eur J Pharmacol 199:379-381[Web of Science][Medline].
Bredt DS, Snyder SH (1990) Isolation of nitric oxide synthetase, a calmodulin-requiring enzyme. Proc Natl Acad Sci USA 87:682-685[Abstract/Free Full Text].
Bredt DS, Snyder SH (1994) Nitric oxide: a physiologic messenger molecule. Annu Rev Biochem 63:175-195[Web of Science][Medline].
Bredt DS, Glatt CE, Hwang PM, Fotuhi M, Dawson TM, Snyder SH (1991) Nitric oxide synthase protein and mRNA are discretely localized in neuronal populations of the mammalian CNS together with NADPH diaphorase. Neuron 7:615-624[Web of Science][Medline].
Bredt DS, Ferris CD, Snyder SH (1992) Nitric oxide synthase regulatory sites. Phosphorylation by cyclic AMP-dependent protein kinase, protein kinase C, and calcium/calmodulin protein kinase; identification of flavin and calmodulin binding sites. J Biol Chem 267:10976-10981[Abstract/Free Full Text].
Brenman JE, Christopherson KS, Craven SE, McGee AW, Bredt DS (1996a) Cloning and characterization of postsynaptic density 93, a nitric oxide synthase interacting protein. J Neurosci 16:7407-7415[Abstract/Free Full Text].
Brenman JE, Chao DS, Gee SH, McGee AW, Craven SE, Santillano DR, Wu Z, Huang F, Xia H, Peters MF, Froehner SC, Bredt DS (1996b) Interaction of nitric oxide synthase with the postsynaptic density protein PSD-95 and alpha1-syntrophin mediated by PDZ domains. Cell 84:757-767[Web of Science][Medline].
Brüne B, Lapetina EG (1991) Phosphorylation of nitric oxide synthase by protein kinase A. Biochem Biophys Res Commun 181:921-926[Web of Science][Medline].
Castillo PE, Weisskopf MG, Nicoll RA (1994) The role of Ca channels in hippocampal mossy fiber synaptic transmission and long-term potentiation. Neuron 12:261-269[Web of Science][Medline].
Castillo PE, Janz R, Südhof TC, Tzounopoulos T, Malenka RC, Nicoll RA (1997) Rab3A is essential for mossy fibre long-term potentiation in the hippocampus. Nature 388:590-593[Medline].
Crepel F, Jaillard D (1990) Protein kinases, nitric oxide and long-term depression of synapses in the cerebellum. NeuroReport 1:133-136[Medline].
Daniel H, Hemart N, Jaillard D, Crepel F (1993) Long-term depression requires nitric oxide and guanosine 3':5' cyclic monophosphate production in rat cerebellar Purkinje cells. Eur J Neurosci 5:1079-1082[Web of Science][Medline].
Eccles JC, Llinás RR, Sasaki K (1966) The mossy fibre-granule cell relay of the cerebellum and its inhibitory control by Golgi cells. Exp Brain Res 1:82-101[Web of Science][Medline].
Geppert M, Bolshakov VY, Siegelbaum SA, Takei K, Camilli PD, Hammer RE, Südhof TC (1994) The role of Rab3A in neurotransmitter release. Nature 369:493-497[Medline].
Geppert M, Goda Y, Stevens CF, Südhof TC (1997) The small GTP-binding protein Rab3A regulates a late step in synaptic vesicle fusion. Nature 387:810-814[Medline].
Hansel C, Batchelor A, Cuenod M, Garthwaite J, Knopfel T, Do KQ (1992) Delayed increase of extracellular arginine, the nitric oxide precursor, following electrical white matter stimulation in rat cerebellar slices. Neurosci Lett 142:211-214[Web of Science][Medline].
Hartell NA (1996a) Inhibition of cGMP breakdown promotes the induction of cerebellar long-term depression. J Neurosci 16:2881-2890[Abstract/Free Full Text].
Hartell NA (1996b) Strong activation of parallel fibers produces localized calcium transients and a form of LTD that spreads to distant synapses. Neuron 16:601-610[Web of Science][Medline].
Ito M (1989) Long-term depression. Annu Rev Neurosci 12:85-102[Web of Science][Medline].
Ito M, Karachot L (1990) Messengers mediating long-term desensitization in cerebellar Purkinje cells. NeuroReport 1:129-132[Medline].
Ito M, Karachot L (1992) Protein kinases and phosphatase inhibitors mediating long-term desensitization of glutamate receptors in cerebellar Purkinje cells. Neurosci Res 14:27-38[Web of Science][Medline].
Ito M, Sakurai M, Tongroach P (1982) Climbing fibre induced depression of both mossy fibre responsiveness and glutamate sensitivity of cerebellar Purkinje cells. J Physiol (Lond) 324:113-134[Abstract/Free Full Text].
Kirkwood A, Bear MF (1994) Hebbian synapses in visual cortex. J Neurosci 14:1634-1645[Abstract].
Kobayashi K, Manabe T, Takahashi T (1996) Presynaptic long-term depression at the hippocampal mossy fiber-CA3 synapse. Science 273:648-650[Abstract].
Kuba K, Kumamoto E (1986) Long-term potentiation of transmitter release induced by adrenaline in bull-frog sympathetic ganglia. J Physiol (Lond) 374:515-530[Abstract/Free Full Text].
Lev-Ram V, Makings LR, Keitz PF, Kao JPY, Tsien RY (1995) Long-term depression in cerebellar Purkinje neurons results from coincidence of nitric oxide and depolarization-induced Ca²⁺ transients. Neuron 15:407-415[Web of Science][Medline].
Li J, Smith SS, McElligott JG (1995) Cerebellar nitric oxide is necessary for vestibulo-ocular reflex adaptation, a sensorimotor model of learning. J Neurophysiol 74:489-494[Abstract/Free Full Text].
Linden DJ (1997) Long-term potentiation of glial synaptic currents in cerebellar culture. Neuron 18:983-994[Web of Science][Medline].
Linden DJ, Dickinson MH, Smeyne M, Connor JA (1991) A long-term depression of AMPA currents in cultured cerebellar Purkinje neurons. Neuron 7:81-89[Web of Science][Medline].
Linden DJ, Dawson TM, Dawson VL (1995) An evaluation of the nitric oxide/cGMP/cGMP-dependent protein kinase cascade in the induction of cerebellar long-term depression in culture. J Neurosci 15:5098-5105[Abstract].
Nagao S, Ito M (1991) Subdural application of hemoglobin to the cerebellum blocks vestibuloocular reflex adaptation. NeuroReport 2:193-196[Web of Science][Medline].
Nakazawa K, Mikawa S, Hashikawa T, Ito M (1995) Transient and persistent phosphorylation of AMPA-type glutamate receptor subunits in cerebellar Purkinje cells. Neuron 15:697-709[Web of Science][Medline].
Nicoll RA, Malenka RC (1995) Contrasting properties of two forms of long-term potentiation in the hippocampus. Nature 377:115-118[Medline].
Nowicky AV, Bindman LJ (1993) The nitric oxide synthase inhibitor, N-monomethyl-L-arginine blocks induction of a long-term potentiation-like phenomenon in rat medial frontal cortical neurons in vitro. J Neurophysiol 70:1255-1259[Abstract/Free Full Text].
Sakurai M (1987) Synaptic modification of parallel fibre-Purkinje cell transmission in in vitro guinea-pig cerebellar slices. J Physiol (Lond) 394:463-480[Abstract/Free Full Text].
Salin PA, Malenka RC, Nicoll RA (1996) Cyclic AMP mediates a presynaptic form of LTP at cerebellar parallel fiber synapses. Neuron 16:797-803[Web of Science][Medline].
Schuman EM, Madison DV (1991) A requirement for the intercellular messenger nitric oxide in long-term potentiation. Science 254:1503-1506[Abstract/Free Full Text].
Shibuki K (1990) An electrochemical microprobe for detecting nitric oxide release in brain tissue. Neurosci Res 9:69-76[Web of Science][Medline].
Shibuki K, Kimura S (1997) Dynamic properties of nitric oxide release from parallel fibers in rat cerebellar slices. J Physiol (Lond) 498:443-452[Abstract/Free Full Text].
Shibuki K, Okada D (1991) Endogenous nitric oxide release required for long-term synaptic depression in the cerebellum. Nature 349:326-328[Medline].
Shibuki K, Okada D (1992) Cerebellar long-term potentiation under suppressed postsynaptic Ca²⁺ activity. NeuroReport 3:231-234[Web of Science][Medline].
Simon SM, Llinás RR (1985) Compartmentalization of the submembrane calcium activity during calcium influx and its significance in transmitter release. Biophys J 48:485-498[Web of Science][Medline].
Son H, Hawkins RD, Martin K, Kiebler M, Huang PL, Fishman MC, Kandel ER (1996) Long-term potentiation is reduced in mice that are doubly mutant in endothelial and neuronal nitric oxide synthase. Cell 87:1015-1023[Web of Science][Medline].
Weisskopf MG, Castillo PE, Zalutsky RA, Nicoll RA (1994) Mediation of hippocampal mossy fiber long-term potentiation by cyclic AMP. Science 265:1878-1882[Abstract/Free Full Text].
Williams JH, Li YG, Nayak A, Errington ML, Murphy KP, Bliss TVP (1993) The suppression of long-term potentiation in rat hippocampus by inhibitors of nitric oxide synthase is temperature and age dependent. Neuron 11:877-884[Web of Science][Medline].
Yanagihara D, Kondo I (1996) Nitric oxide plays a key role in adaptive control of locomotion in cat. Proc Natl Acad Sci USA 93:13292-13297[Abstract/Free Full Text].
Yokoi M, Kobayashi K, Manabe T, Takahashi T, Sakaguchi I, Katsuura G, Shigemoto R, Ohishi H, Nomura S, Nakamura K, Nakao K, Katsuki M, Nakanishi S (1996) Impairment of hippocampal mossy fiber LTD in mice lacking mGluR2. Science 273:645-647[Abstract].

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