Activity-Dependent Maintenance of Long-Term Potentiation at Visual Cortical Inhibitory Synapses

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (18)

Citing Articles via Google Scholar

Google Scholar

Articles by Komatsu, Y.

Articles by Yoshimura, Y.

Search for Related Content

PubMed

PubMed Citation

Articles by Komatsu, Y.

Articles by Yoshimura, Y.

Pubmed/NCBI databases
Compound via MeSH
Substance via MeSH

Previous Article  |  Next Article

The Journal of Neuroscience, October 15, 2000, 20(20):7539-7546

Activity-Dependent Maintenance of Long-Term Potentiation at Visual Cortical Inhibitory Synapses
Yukio Komatsu and Yumiko Yoshimura
Department of Visual Neuroscience, Research Institute of Environmental Medicine, Nagoya University, Furo-cho, Chikusa-ku, Nagoya 464-8601, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neural activity producing a transient increase in intracellular Ca²⁺ concentration can induce long-term potentiation (LTP) at visualcortical inhibitory synapses similar to those seen at variousexcitatory synapses. Here we report that low-frequency neuralactivity is required to maintain LTP at these inhibitory synapses.Inhibitory responses of layer 5 cells evoked by layer 4 stimulationwere studied in developing rat visual cortical slices under apharmacological blockade of excitatory synaptic transmission usingintracellular and whole-cell recording methods. Although LTP inducedby high-frequency stimulation (HFS) persisted while test stimulationwas applied at 0.1 Hz, it was not maintained in approximatelytwo-thirds of cells after test stimulation was stopped for 30min. In the rest of the cells, LTP seemed to be maintained byspontaneous presynaptic spikes, because presynaptic inhibitorycells discharged spontaneously in our experimental condition andbecause LTP was totally abolished by a temporary application ofNa⁺ channel blockers. Experiments applying various Ca²⁺ channel blockers and Ca²⁺ chelators after HFS demonstrated that LTP maintenance was mediatedby presynaptic Ca²⁺ entries through multiple types of high-threshold Ca²⁺ channels, which activated Ca²⁺-dependent reactions different from those triggering transmitterrelease. The Ca²⁺ entries associated with action potentials seemed to be regulatedby presynaptic K⁺ channels, presumably large-conductance Ca²⁺-activated K⁺ channels, because the application of blockers for these channelsfacilitated LTP maintenance. In addition, noradrenaline facilitatedthe maintenance of LTP. These findings demonstrate a new mechanismby which neural activity regulates the continuation and terminationof LTP at visual cortical inhibitorysynapses.

Key words: long-term potentiation; maintenance; inhibitory synaptic transmission; Ca²⁺ channels; Ca²⁺-activated K⁺ channels; visual cortex

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activity-dependent long-term modification of synaptic transmission is thought to underlie information storage and learning(Brown et al., 1990; Bliss and Collingridge, 1993; Hawkins etal., 1993). Induction and maintenance phases can be distinguishedin this modification process. During the induction phase, neuralactivity producing a transient increase in intracellular Ca²⁺ concentration ([Ca²⁺]_i) initiates a series of biochemical reactions that lead to enduringmodification of synaptic strength (Lynch et al., 1983; Malenkaet al., 1988). For example, at excitatory synapses in hippocampalCA1 pyramidal cells, high-frequency stimulation (HFS) of presynapticfibers can produce postsynaptic Ca²⁺ entry through NMDA receptors, leading to long-term potentiation(LTP) (Gustafsson and Wigstrom, 1988; Brown et al., 1990; Madisonet al., 1991; Bliss and Collingridge, 1993). During the maintenancephase, modified synaptic strength is preserved by mechanisms independentof neural activity, which have still not been clarified sufficiently.It was proposed that NMDA receptor-mediated postsynaptic [Ca²⁺]_i increase produces autophosphorylation of Ca²⁺/calmodulin-dependent protein kinase II (CaM kinase II), convertingthe molecule into a Ca²⁺-independent active form, which maintains LTP by persistent phosphorylationof its substrates (Lisman, 1994).

LTP is also produced by HFS of presynaptic fibers in GABA-mediated inhibitory synaptic transmission of rat visual cortex (Komatsuand Iwakiri, 1993). This LTP is input-specific and associativeand requires postsynaptic [Ca²⁺]_i increase for induction (Komatsu, 1994, 1996), as is the casewith NMDA receptor-dependent LTP. However, the induction of LTPlacks dependence on postsynaptic membrane potentials, and postsynaptic[Ca²⁺]_i increase originates from internal Ca²⁺ stores rather than from an extracellular source (Komatsu, 1994,1996). The activation of GABA_B receptors, which is also requiredfor induction, seems to contribute to postsynaptic [Ca²⁺]_i increase by facilitating monoamine receptor-mediated inositoltrisphosphate formation, which produces Ca²⁺ release from the internal stores (Komatsu, 1996). This LTP occursfar more frequently in developing than in mature animals (Komatsu,1994), suggesting that it is a cellular mechanism underlying experience-dependentdevelopment of visual responsiveness in corticalcells.

Although LTP at visual cortical inhibitory synapses resembles the NMDA-receptor dependent LTP in basic properties, such asinput specificity, associativity, and involvement of postsynaptic[Ca²⁺]_i increases in induction, the present study demonstrates thatthe former is a new form of LTP, different from the latter inthat the maintenance of increased synaptic strength requires alow-frequency firing of presynaptic cells. This maintenance ismediated by action potential-associated presynaptic [Ca²⁺]_i increases, which activate Ca²⁺-dependent reactions different from those triggering transmitterrelease.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Sprague Dawley rats at postnatal ages of 20-29 d were deeply anesthetized with isoflurane before the whole brain was removedfrom the skull and immersed in an ice-cold oxygenated (95% O₂and 5% CO₂) Krebs'-Ringer's solution containing (in mM): 124 NaCl,5 KCl, 1.3 MgSO₄, 4 CaCl₂, 1.2 KH₂PO₄, 26 NaHCO₃, and 10 glucose.Then, coronal slices of primary visual cortex (400-µm-thick) wereprepared using a Microslicer (DTK-1000; Dosaka, Kyoto, Japan)and kept in a recovery chamber perfused with Krebs'-Ringer's solutionat 33°C. During recording experiments, the medium, maintainedat 33°C, contained 100 µM DL-2-amino-5-phosphonovaleric acid (APV),an NMDA receptor antagonist, and 40 µM 6,7-dinitroquinoxaline-2,3-dione(DNQX), a non-NMDA receptor antagonist. For some experiments,the concentration of CaCl₂ was altered without changing othersolutes.

Two pairs of bipolar stimulating electrodes (Fig. 1A, s1, s2) made of tungsten wires (diameter, 100 µm; interpolar distance,200 µm) were placed in layer 4, separated from each other by ~0.5mm. Layers 2-4 was surgically cut between s1 and s2 to ensurethat separate groups of presynaptic fibers were activated. Teststimulation was applied alternately to s1 and s2 at intervalsof 5 sec. As a conditioning stimulation, HFS (50 Hz, 1 sec) wasapplied to one of the electrodes 10 times at intervals of 10 sec.The intensity of the test stimulation and HFS was adjusted to1.5-2 and 5 times the threshold intensity to evoke IPSPs, respectively.

View larger version (30K):
[in this window]
[in a new window]
Figure 1. Temporary cessation of test stimulation disturbs LTP maintenance. A, Experimental arrangement of stimulating (s1 and s2) and recording electrodes (r), with the left figures and a dashed line indicating cortical layers and surgical cuts, respectively. B, C, LTP was maintained in cells in which test stimulation (0.l Hz) was continued after HFS. B, Top (a) and middle (b) traces show superimposed average (n = 6) responses in a cell before and after HFS for conditioned (left) and unconditioned (right) pathways, respectively. Bottom traces (a, b) are the top and middle traces superimposed. Recorded time of the traces is indicated in C. Resting membrane potential was $-$ 54 and $-$ 55 mV before and 100 min after HFS, respectively. Input resistance (42 M $Omega$ ) was unchanged before and 100 min after HFS. C, The initial falling slope of IPSPs (percent of the mean baseline) plotted against the time after HFS for 12 cells. Squares and triangles (mean ± SEM) represent responses for conditioned and unconditioned pathways, respectively. No significant difference (p > 0.4; n = 12) was found in either resting membrane potential or input resistance before ( $-$ 55 ± 2 mV, 44 ± 4 M $Omega$ ) and 100 min after HFS ( $-$ 56 ± 3 mV, 44 ± 5 M $Omega$ ), which was also the case for other experimental groups of cells to which HFS was applied. D, E, Similar to B and C, but test stimulation for the conditioned pathway (s1) was stopped for the period indicated by the horizontal bar in E. D, Left and right superimposed traces represent responses in two cells that did not and did maintain LTP after cessation of test stimulation, respectively. E, Squares and circles represent responses for conditioned pathways that did (n = 3) and did not maintain LTP (n = 5), respectively, and triangles indicate unconditioned pathways (n = 8).

Intracellular recording was conducted with microelectrode pipettes containing 2 M K-methylsulfate (50-100 M $Omega$ ). The electrodewas mounted on a three-dimensional oil-driven micromanipulator(MO-103; Narishige, Tokyo, Japan). For analysis, we selected cellswith a stable resting membrane potential hyperpolarized more than $-$ 50 mV. When the resting membrane potential was deeper than $-$ 60mV and consequently the amplitude of IPSPs evoked by test stimulationwas too small, the membrane potential was depolarized by currentinjection through the recording electrode to increase the IPSPamplitude. Input resistance was monitored throughout the experimentsby injecting 0.05-0.1 nA hyperpolarizing current pulses. A bridgecircuit was used to record the membrane potential while currentinjection was made through the recording electrode (Axoclamp 2A;Axon Instruments, Foster City, CA). In experiments recording spontaneousIPSCs, whole-cell recording was made from pyramidal cells usinginfrared differential contrast optics (BX50WI; Olympus Optical,Tokyo, Japan). Patch pipettes (5-6 M $Omega$ ) were filled with a solutioncontaining (in mM): 126 D-gluconate, 140 CsOH, 8 CsCl, 2 NaCl,0.2 EGTA, 10 HEPES, 3 MgATP, and 0.5 Na₂GTP, pH 7.2 with CsOH.We selected cells with a high seal resistance (>1 G $Omega$ ) and a seriesresistance <25 M $Omega$ (15-21 M $Omega$ ) for analysis. Cells were voltageclamped at 0 mV, and series resistance was not compensated. Thelaminar location of the stimulating and recording electrodes wasidentified on histological sections stained with cresyl violetafter the recordings, as described previously (Komatsu, 1994).Data are expressed as mean ± SEM, and either Student's t testor Welch's test wasapplied.

The compounds used were obtained from the following sources: APV, DNQX, and CHS50911 from Tocris Cookson (Bristol, UK); iberiotoxin,tetrodotoxin (TTX), bicuculline methiodide, noradrenaline, andserotonin from Sigma (St. Louis, MO); 4-aminopyridine, charybdotoxin, $omega$ -conotoxin GVIA, and nifedipine from Research Biochemicals (Natick,MA); $omega$ -agatoxin IVA from Peptide Institute (Osaka, Japan); EGTA-AMfrom Calbiochem (La Jolla, CA); saxitoxin (STX) from Alexis (SanDiego, CA); and isoflurane from Abbott Laboratories (North Chicago,IL).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Intracellular recording studies were conducted in visual cortical slices of developing rats at ages of postnatal 20-29 d,when LTP of IPSP occurs frequently (Komatsu, 1994) and visualresponses are easily modified by visual experience (Fagioliniet al., 1994). IPSPs evoked by layer 4 stimulation were recordedfrom layer 5 neurons under a blockade of excitatory synaptic transmissionusing high doses of the NMDA receptor antagonist APV (100 µM)and the non-NMDA receptor antagonist DNQX (40 µM). In all thecases in which the LTP was analyzed, sharp electrodes were usedto record IPSPs, because stable recording was possible for longerperiods compared with patch electrodes. One of two stimulatingelectrodes placed in layer 4 was used to test the effect of HFS,and the other served as a control (Fig. 1A). Synaptic strengthwas assessed by test stimulation at a low frequency (0.1 Hz),which is in a range commonly used in studies of LTP at excitatorysynapses. Experiments were conducted in the solution containinga high concentration (4 mM) of Ca²⁺ (Komatsu, 1994, 1996) in which strong HFS used in this studyalways (12 of 12) produced LTP lasting >120 min as long as therecording remained stable (Fig. 1B,C).

LTP maintenance requires presynaptic action potentials but not postsynaptic responses

To test whether neural activity is necessary to maintain LTP, test stimulation of the conditioned pathway was stopped for30 min after HFS. Figure 1, D and E, illustrates cases in whichstimulation cessation was started 30 min after HFS. Before stimulationcessation, the responses for the conditioned pathway were significantlylarger (p < 0.005) than the baseline level for all of the testedcells. After test stimulation was resumed, potentiated responsesreturned almost to the baseline level (p > 0.2) in approximatelytwo-thirds of the cells (circles), whereas almost the same levelof potentiation, which was significantly larger (p < 0.01) thanthe baseline, was maintained for the rest of cells (squares).The same effect was produced by cessation started either soon,or 30 or 120 min after HFS as shown in Figure 2, which shows themagnitude of LTP before and after stimulation cessation (filledsquares). No such LTP abolition was found when test stimulationwas continued (open circles). Once LTP was abolished, no recoverywas found, although test stimulation was continued for 30-75 min.To rule out the possibility that cessation of the stimulationreduces test responses irrespective of LTP, test stimulation wasstopped for a separate group of cells to which HFS was not applied.No change was found in the responses after the stimulation cessation(99 ± 3% of the values before cessation; p > 0.3; n = 6).

View larger version (29K):
[in this window]
[in a new window]
Figure 2. Summary of effects of test stimulation cessation on LTP. A, Magnitude of LTP at 50-60 min after HFS in cells for which test stimulation was not (open circles) and was stopped from 0 to 30 min after HFS (filled squares). B, Magnitude of LTP (filled squares) before (20-30 min after HFS; left) and after (80-90 min after HFS; right) test stimulation cessation (30-60 min after HFS) and those (open circles) for corresponding values when test stimulation was not stopped. C, Similar to B, but test stimulation was stopped from 120 to 150 min after HFS.

We tested the possibility that spontaneous presynaptic spikes contributed to LTP, which persisted even after stimulation cessation,because inhibitory neurons fire spontaneously in rat somatosensorycortical slices even under a pharmacological blockade of ionotropicglutamate receptors (Salin and Prince, 1996). We first confirmedthat inhibitory cells innervating layer 5 cells also dischargedspontaneously in our experimental conditions. For this purpose,we tested whether spontaneous IPSCs were sensitive to a pharmacologicalblockade of action potentials using the whole-cell recording method,which is more effective in the detection of small responses thanthe method using sharp electrodes. Bath application of the Na⁺ channel blocker TTX (1 µM) significantly (p < 0.05) reduced themean frequency of spontaneous IPSCs from 10.1 ± 2.4 to 3.4 ± 0.6Hz and their mean amplitude from 21.9 ± 1.7 to 14.0 ± 1.2 pA inlayer 5 cells (n = 6), as shown in Figure 3, indicating that thesecells received inhibitory inputs, mediated by spontaneous presynapticspikes, at a frequency of ~7 Hz (3.2-14.6 Hz) on average. Therefore,these spontaneous spikes may have contributed to maintaining LTPduring the cessation of test stimulation. This supposition wassupported by experiments in which action potentials were temporarilyabolished after HFS (Fig. 4A,B). We used another sodium channelblocker, STX, instead of TTX to block spikes, because it is washedout more rapidly than TTX (Narahashi, 1974). Test responses disappearedtemporarily and returned to the baseline level for both conditionedand unconditioned pathways after washout at the time when LTPwas still demonstrated in the control experiment (Fig. 1C). Similarly,a temporary application of STX also abolished the LTP, which hadpersisted even after the cessation of test stimulation (Fig. 4C,D).These results indicate that presynaptic action potentials occurringat a low frequency are necessary to maintain LTP.

View larger version (27K):
[in this window]
[in a new window]
Figure 3. Inhibitory presynaptic cells discharge spontaneously. A-C, Spontaneous IPSCs recorded from a layer 5 cell, which was voltage clamped at 0 mV. Traces in A, B, and C show spontaneous postsynaptic responses in the control solution containing both non-NMDA and NMDA receptor antagonists (DNQX and APV), after adding TTX (1 µM), a sodium channel blocker, and after further addition of bicuculline methiodide (20 µM), a GABA_A receptor antagonist, respectively. D, Frequency histogram of peak amplitudes of IPSCs, recorded from the cell shown in A and B in the control solution (broken line) and in the presence of TTX (solid line). The total number of events was 1290 (control) and 341 (TTX).

View larger version (34K):
[in this window]
[in a new window]
Figure 4. Blockade of presynaptic action potentials, but not of GABA receptors, abolishes LTP. A, B, Effects of STX (0.1 µM), a sodium channel blocker, on LTP maintenance (n = 6). After LTP induction, STX was applied for the period indicated by the horizontal bar in B. Recorded time of traces in A is indicated in B. Squares and triangles represent responses for conditioned and unconditioned pathways, respectively. C, D, Similar to A and B, but STX was applied to cells (n = 3) in which LTP was maintained even after test stimulation for the conditioned pathway (S1 off) was stopped for 30 min. E, F, Similar to A and B, but selective antagonists for GABA_A receptors (bicuculline methiodide, 20 µM) and GABA_B receptors (SCH 50911, 50 µM) were simultaneously applied for the period indicated by the horizontal bar in F (n = 6). Filled triangles in F indicate responses of unconditioned pathways for STX application, which were obtained from the experiments shown in B.

The effect of presynaptic action potentials on LTP maintenance can be mediated by postsynaptic responses. To test this possibility,we applied high doses of the selective GABA_A receptor antagonistbicuculline methiodide and the selective GABA_B receptor antagonistCHS 50911 after HFS (Fig. 4E,F). IPSPs were completely abolishedby these compounds. After washout, the responses of conditionedand unconditioned pathways returned to the respective levels beforethe drug application. A comparison of unconditioned pathway responsesfor GABA receptor antagonists (open triangles) and STX (filledtriangles) in Figure 4F demonstrated that the time course of IPSPblockade by the two treatments was almost the same. These resultssuggest that the maintenance of LTP requires neither postsynapticresponses nor activation of either GABA_A or GABA_Breceptors.

LTP maintenance is mediated by presynaptic Ca²⁺ entry through multiple types of high-threshold Ca²⁺ channels

The above results prompted us to test the involvement of presynaptic Ca²⁺ channels in LTP maintenance. Accordingly, we applied Ca²⁺ channel blockers after HFS. LTP always disappeared without anychanges in unconditioned pathway responses after application of20 µM nifedipine (Fig. 5A), a selective L-type Ca²⁺ channel blocker (Fox et al., 1987; Aosaki and Kasai, 1989). Thesame effects were produced by low doses of $omega$ -agatoxin IVA (30-50nM), blocking selectively P-type Ca²⁺ channels at this range of doses (Fig. 5B) (Mintz et al., 1992;Sather et al., 1993). At a high dose (1 µM), which also blocksQ-type Ca²⁺ channels (Mintz et al., 1992; Sather et al., 1993; Wheeler etal., 1994), both conditioned and unconditioned pathway responsesdisappeared (Fig. 5C). Application of a high dose of $omega$ -conotoxinGVIA (1 µM), a selective N-type Ca²⁺ channel blocker (Aosaki and Kasai, 1989; Plummer et al., 1989),also abolished LTP and reduced slightly both conditioned (84 ±2% of the baseline at 70-80 min after HFS; n = 5) and unconditionedpathway responses (80 ± 2%). Although the reduction was significantfor both pathways (p < 0.02), no significant difference (p > 0.1)was found in the amount of reduction between the two pathways(Fig. 5D). Application of 50 µM Ni²⁺, which rather selectively blocks T- and R-type Ca²⁺ channels (Fox et al., 1987; Narahashi et al., 1987; Zhang etal., 1993), affected neither LTP nor baseline responses (Fig.5E). These results indicate that transmitter release is mediatedmostly by Q-type and partially by N-type Ca²⁺ channels, whereas Ca²⁺ entries through P-, N-, and L-type Ca²⁺ channels are all necessary for LTP maintenance. We could nottest the involvement of Q-type Ca²⁺ channels in maintenance because no specific blockers are available.

View larger version (46K):
[in this window]
[in a new window]
Figure 5. Effects of Ca²⁺ channel blockers and chelators on LTP maintenance. A, Nifedipine (20 µM) was applied for the period indicated by the horizontal bar (n = 5). B-F, Similar to A, but 30-50 nM (B) or 1 µM $omega$ -agatoxin IVA (C), 1 µM $omega$ -conotoxin GVIA (D), 50 µM Ni²⁺ (E), or 2 µM EGTA-AM (F) was applied instead. The number of cells was five for each of A-E and eight for F. Squares and triangles represent responses for conditioned and unconditioned pathways, respectively.

It is likely that presynaptic, but not postsynaptic, high-threshold Ca²⁺ channels contribute to LTP maintenance, because test stimulationproduced only small hyperpolarizing responses in postsynapticcells and because LTP was maintained under voltage clamp at hyperpolarized( $-$ 90 mV) or very depolarized (between +20 and +40 mV) membranepotentials (Komatsu, 1994) and even under no postsynaptic responses(Fig. 4E,F). This suggests that LTP maintenance requires presynaptic[Ca²⁺]_i elevation. We tested this possibility with EGTA-AM, which ismembrane-permeable and converted into EGTA, a slow Ca²⁺ chelator, in the cytoplasm. Bath application of the compound(2 µM) after HFS abolished LTP without any effects on the unconditionedpathway (Fig. 5F). LTP persisted during the whole-cell recordingwith patch electrodes containing 1 mM EGTA (Komatsu, 1994, 1996).These results are consistent with the idea that increases in presynaptic[Ca²⁺]_i are necessary for LTPmaintenance.

Temporary reduction in presynaptic Ca²⁺ entry abolishes LTP

Temporarily applied Ca²⁺ channel blockers and chelators might remain in tissues after washout, because this procedure is noteasily accomplished. If so, abolition of LTP can be attributableto continuous, but not temporary, reduction in presynaptic [Ca²⁺]_i increases. We, thus, tested the effect of temporary reductionin Ca²⁺ entry on LTP maintenance by changing extracellular Ca²⁺ concentrations ([Ca²⁺]_o). For this purpose, we first examined the dependence of LTPon [Ca²⁺]_o. LTP (>15% increase from the baseline at 40-50 min after HFS)occurred rarely at a normal value (2.4 mM) of [Ca²⁺]_o, more frequently with the increase of [Ca²⁺]_o, and always at 3.6-4.8 mM (Fig. 6A). When [Ca²⁺]_o was temporarily reduced from a high to normal value, LTP wasabolished and never recovered after restoration of high [Ca²⁺]_o for 40-90 min (Fig. 6B). This suggests that, once LTP is abolishedby a reduction in Ca²⁺ entry, it could not be reestablished, even by restoring the previousamount of Ca²⁺ entry. In consideration of this result and the experiment usingEGTA-AM, it is extremely unlikely that the complete abolitionof LTP by any of the three Ca²⁺ channel blockers (Fig. 5A,B,D) merely resulted from the blockadeof Ca²⁺ channels recruited to transmitter releases after HFS, althoughsuch recruitment did take place. High [Ca²⁺]_o was not required for LTP induction, because HFS, applied undernormal [Ca²⁺]_o, produced LTP if high [Ca²⁺]_o was resumed immediately after HFS (Fig. 6C).

View larger version (22K):
[in this window]
[in a new window]
Figure 6. Temporary reduction in [Ca²⁺]_o abolishes LTP. A, Incidence of LTP (>15% increase from the baseline at 40-50 min after HFS) plotted against [Ca²⁺]_o with figures indicating the number of tested cells. B, C, [Ca²⁺]_o was changed between 4 and 2.4 mM, indicated in the middle. The number of cells was six (B) and five (C). Squares and triangles represent responses for conditioned and unconditioned pathways, respectively.

Presynaptic K⁺ channels regulate the maintenance of LTP

The above results suggest that the amount of Ca²⁺ entry was insufficient to maintain LTP at normal [Ca²⁺]_o in our experimental conditions (Fig. 7A). Using various K⁺ channel blockers, we tested the possibility that open K⁺ channels disturb LTP maintenance, because they reduce Ca²⁺ entry associated with action potentials. In the presence of 60nM charybdotoxin or 100 nM iberiotoxin, LTP occurred frequently(7 of 9 for charybdotoxin, and 5 of 5 for iberiotoxin) even atnormal [Ca²⁺]_o, although the magnitude was significantly smaller (p < 0.02)than that at high [Ca²⁺]_o (compare Fig. 7B with Fig. 1C). These toxins are known to blocklarge-conductance Ca²⁺-activated K⁺ (BK) channels (Miller et al., 1985; Galvez et al., 1990). However,they could block some other K⁺ channels (Lewis and Cahalan, 1988; MacKinnon et al., 1988; Schweitzet al., 1989; Galvez et al., 1990). The same effect was producedby 1 mM Cs⁺, which blocks various K⁺ channels including BK channels (Hille, 1992), without affectingbaseline responses (Fig. 7C). In contrast, 4-aminopyridine (10-50µM), which blocks various K⁺ channels but not BK channels (Hermann and Hartung, 1982; Hille,1992), was ineffective for LTP production, although it increasedbaseline responses to 154 ± 23% (n = 7) of the value before drugapplication (Fig. 7D). This increase may be attributable to enhancedtransmitter release, as shown for various synapses (Thesleff,1980). If LTP is expressed presynaptically, the ineffectivenessof this blocker for LTP production could be attributable to anocclusion of LTP by the enhanced transmitter release before HFS.However, this possibility was not supported by similar experimentsconducted at high [Ca²⁺]_o. Application of the blocker increased test responses to 158± 6% of the control value, but HFS still produced LTP (186 ± 10%at 30-40 min after HFS compared with the value just before HFS;n = 3). Cs⁺ was used to confirm that blockade of these K⁺ channels is involved in the maintenance of LTP, because it wasfar more quickly washed in and out than those toxins. LTP occurredwhen Cs⁺ was added to the solution after, but not during, HFS (Fig. 8).Thus, it is thought that closure of BK or pharmacologically relatedK⁺ channels facilitates the maintenance of LTP.

View larger version (44K):
[in this window]
[in a new window]
Figure 7. Effects of K⁺ channel blockers on LTP. A, Effect of HFS on IPSPs at normal (2.4 mM) [Ca²⁺]_o (n = 8). B, Effect of charybdotoxin (open symbols; n = 9) and iberiotoxin (filled symbols; n = 5) on LTP at normal [Ca²⁺]_o. Both toxins were present all the time. C, Effect of 1 mM Cs⁺ on LTP at normal [Ca²⁺]_o (n = 8). Blocker application time is indicated by the horizontal bar. D, Similar to C, but 10-50 µM 4-aminopyridine was applied (n = 7).

View larger version (24K):
[in this window]
[in a new window]
Figure 8. Cs⁺ facilitates the maintenance of LTP. Similar to Figure 7C, but Cs⁺ (1 mM) was applied to the bath during (A) or after HFS (B). Number of cells was five (A) and six (B).

Noradrenaline facilitates the maintenance of LTP

The inability to maintain LTP at normal [Ca²⁺]_o might result from the absence of neuromodulatory inputs from other parts ofthe brain to the cells. We tested the involvement of noradrenalineand serotonin. In the presence of noradrenaline (5 µM), LTP wasconsistently (8 of 8) produced under normal [Ca²⁺]_o (Fig. 9), although the magnitude was significantly smaller(p < 0.01) than that under high [Ca²⁺]_o (Fig. 1C). On the other hand, no LTP was produced (95 ± 4%of the baseline; n = 5) in the presence of high doses of serotonin(100 µM). These results suggest that noradrenaline controls themaintenance of LTP by modulating the presynaptic Ca²⁺ and/or K⁺ channels.

View larger version (29K):
[in this window]
[in a new window]
Figure 9. Noradrenaline enables the maintenance of LTP under normal [Ca²⁺]_o. Effects of HFS on IPSPs in the presence of noradrenaline (5 µM) under normal [Ca²⁺]_o (2.4 mM). Noradrenaline was present all the time. Number of cells was eight.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study demonstrated that low-frequency spike activity of presynaptic neurons is required to maintain LTP at visual corticalinhibitory synapses. The effect of action potentials is mediatedby presynaptic Ca²⁺ entry through multiple types of high-threshold Ca²⁺ channels, which activates Ca²⁺-dependent reactions different from those triggering transmitterrelease. Our results also suggest that presynaptic K⁺ channels regulate the Ca²⁺ entry involved inmaintenance.

Our results suggest that triggering presynaptic spikes at a frequency of 0.1 Hz is almost sufficient for the maintenance ofLTP. However, one cannot exclude the possibility that this maintenancecould be observed using a lower presynaptic spike frequency. Althoughthe time course of the [Ca²⁺]_i increase associated with action potentials at axon terminalsof these inhibitory cells has not been clarified, it has beendemonstrated that Ca²⁺ transients at hippocampal excitatory nerve terminals return tothe baseline level within a few to several seconds, a period shorterthan the stimulus intervals used in this study (Regehr et al.,1994; Wu and Saggau, 1994). Thus, it is likely that intermittentoccurrences of Ca²⁺ transients or a continuously elevated low level of [Ca²⁺]_i is sufficient for the activation of Ca²⁺-dependent processes responsible for LTPmaintenance.

The inhibitory synaptic transmission studied in this experiment was mediated by $omega$ -agatoxin IVA- and $omega$ -conotoxin GVIA-sensitiveCa²⁺ channels, as was the case in other central excitatory and inhibitorysynapses (Dunlap et al., 1995; Reuter, 1996). Because dihydropyridinesdid not affect transmitter release at central synapses, it hasbeen suggested that L-type Ca²⁺ channels are almost absent at the presynaptic terminals of theCNS, although they contribute to hormone secretion from neuroendocrinecells (Dunlap et al., 1995; Reuter, 1996). The results of thepresent study provided evidence for the presence of L-type Ca²⁺ channels at central nerve terminals, which was also reportedrecently for cultured hippocampal cells in which they were involvedin post-tetanic potentiation but not basal responses (Jensen etal., 1999). It has been suggested that multiple types of Ca²⁺ channels, which are involved in transmitter release, coexistat a single nerve terminal (Dunlap et al., 1995). Our resultsshowed that the blockade of any of the multiple types of Ca²⁺ channels involved in LTP maintenance abolished LTP totally inall of the tested cells, suggesting that these channels also coexistat a nerve terminal. If only a subset of these channels are presentat individual terminals, the blockade of one type of these channelsmay produce a partial, but not total, blockade of LTP. The questionof why such multiple channels are involved in LTP maintenanceremainsunclarified.

The observation that charybdotoxin and iberiotoxin enabled LTP production at normal [Ca²⁺]_o suggests that BK channels are involved in the regulation ofLTP maintenance. Although charybdotoxin blocks K⁺ channels other than BK channels (Lewis and Cahalan, 1988; MacKinnonet al., 1988; Schweitz et al., 1989; Galvez et al., 1990), iberiotoxinseems to block BK channels more specifically. However, we cannotstill deny the possibility that the latter toxin blocks some otherK⁺ channels. Therefore, we conclude at present that BK or pharmacologicallyrelated K⁺ channels are involved in the regulation of LTP maintenance. NeuronalBK channels are usually opened by simultaneous Ca²⁺ increase and depolarization in association with action potentials,contributing to repolarization of action potentials (Lancasterand Nicoll, 1987; Storm, 1987). Therefore, activation of thesechannels may reduce the Ca²⁺ entry associated with action potentials, contributing to theabolition ofLTP.

At squid giant synapses, presynaptic injections of EGTA blocked both HFS-induced short-term potentiation and slow Ca²⁺ signals, whereas they had no effect on basal transmitter releasetriggered by fast Ca²⁺ signals (Swandulla et al., 1991). Thus, the experiment usingthe membrane-permeable Ca²⁺ chelator EGTA-AM suggests that presynaptic slow Ca²⁺ signals activate reactions that maintain LTP. Although this Ca²⁺-dependent process is unresolved yet, Ca²⁺-dependent protein kinases and phosphatases are possible candidatesfor molecules mediating these Ca²⁺ signals. These reactions could act on some transmitter releasingprocesses modified by HFS, because the presynaptic localizationof maintenance mechanisms strongly suggests the presynaptic expressionof LTP. The BK or related K⁺ channels may be located apart from transmitter release sitesand control Ca²⁺ entry relevant to LTP maintenance but not triggering transmitterrelease, because Cs⁺ facilitated LTP maintenance but not baseline responses, whereas4-aminopyridine facilitated baseline responses but not LTP maintenance.This supposition is compatible with the observation that P- andL-type Ca²⁺ channels contributed to LTP maintenance but not the baselineresponses. In addition, Ca²⁺ imaging of presynaptic axons has suggested that high-thresholdCa²⁺ channels are also located at sites other than transmitter releasesites, although their density is less than those at release sites(Mackenzie et al., 1996).

Although the maintenance of LTP depends on neural activity and Ca²⁺ signals at visual cortical inhibitory synapses, it has been reportedthat LTP at hippocampal excitatory synapses persists after theblockade of presynaptic spikes or Ca²⁺ channels (Malgaroli and Tsien, 1992; Manabe et al., 1992; Cormieret al., 1993; Castillo et al., 1994; Wheeler et al., 1994). Amechanism has been proposed for NMDA receptor-dependent LTP, whichis suggested to be expressed, at least partly, by phosphorylationof AMPA receptors by CaM kinase II (Lisman, 1994; Pettit et al.,1994; Barria et al., 1997). The phosphorylated state could bemaintained by Ca²⁺-dependent autophosphorylation of the kinase, switching the moleculeinto an active state even at low [Ca²⁺]_i (Saitoh and Schwartz, 1985; Miller and Kennedy, 1986).

In regard to synaptic plasticity as a basis of learning and memory, the reversibility of modified synaptic strength couldbe important. At CA1 excitatory synapses, HFS (10-100 Hz)-inducedLTP is reversed by low-frequency (1-5 Hz) stimulation continuedfor 10-15 min (Staubli and Lynch, 1990; Fujii et al., 1991). Thistype of LTP reversal has been reported for other excitatory synapses(Kirkwood et al., 1993; Chen et al., 1996; Tzounopoulos et al.,1998). In contrast, at visual cortical inhibitory synapses, LTPis induced by stimulation of a wide range (2-50 Hz) of frequencies(Komatsu, 1994), and its reversal is attained by reducing thefrequency of stimulation to a level lower than that for test stimulation.This difference suggests that the two forms of LTP operate verydifferently and play different functionalroles.

LTP at these inhibitory synapses was consistently produced in the presence of noradrenaline at normal [Ca²⁺]_o, suggesting that the activity of noradrenergic cells, whichwere shown to be involved in visual cortical plasticity (Kasamatsuand Pettigrew, 1976; Bear and Singer, 1986), regulates the maintenancemechanism by modulating presynaptic K⁺ and/or Ca²⁺ channels. Because this synaptic plasticity could underlie theexperience-dependent refinement of visual responsiveness proceedinggradually during a critical period in early life (Komatsu, 1994),a single episode of neural activity evoked by visual inputs mayproduce LTP, which is reversible depending on the following neuralactivity. The modified visual responsiveness consequent to theLTP may not persist unless the strengthened inhibitory synapsesare activated at least at a low frequency. Orientation selectivityis improved to almost adult level in the middle of the criticalperiod (Frégnac and Imbert, 1984), and deprivation of light inthat period, even for a few days, degrades the selectivity (Freemanet al., 1981). This observation supports the idea that neuralactivity plays a crucial role to maintain visual responsivenessrefined depending on experience. If LTP at the inhibitory synapsesindeed contributes to developmental plasticity of visual responsiveness,a temporary pharmacological blockade of spike activity in corticalinhibitory cells during the critical period may degrade the selectivityof visual responses, which is experimentally testable. Repetitiveuse of the modified synapse during the critical period might leadeventually to a more persistent form independent of activity,requiring RNA and protein synthesis, as is the case in the latephase of hippocampal NMDA receptor-dependent LTP (Frey et al.,1988; Nguyen et al., 1994).

  FOOTNOTES

Received Feb. 1, 2000; revised July 31, 2000; accepted July 31, 2000.

This work was supported by Grants-in Aid for Scientific Research Projects 07279104, 08458271, and 12053228 from the JapaneseMinistry of Education, Science, Sports, andCulture.
Correspondence should be addressed to Dr. Yukio Komatsu, Department of Visual Neuroscience, Research Institute of EnvironmentalMedicine, Nagoya University, Furo-cho, Chikusa-ku, Nagoya 464-8601,Japan. E-mail: komatsu{at}riem.nagoya-u.ac.jp.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aosaki T, Kasai H (1989) Characterization of two kinds of high-voltage-activated Ca-channel currents in chick sensory neurons. Differential sensitivity to dihydropyridines and $omega$ -conotoxin GIVA. Pflügers Arch 414:150-156[Web of Science][Medline].
Barria A, Muller D, Derkach V, Griffith LC, Soderling TR (1997) Regulatory phosphorylation of AMPA-type glutamate receptors by CaM-KII during long-term potentiation. Science 276:2042-2045[Abstract/Free Full Text].
Bear MF, Singer W (1986) Modulation of visual cortical plasticity by acetylcholine and noradrenaline. Nature 320:172-176[Medline].
Bliss TVP, Collingridge GL (1993) A synaptic model of memory: long-term potentiation in the hippocampus. Nature 361:31-39[Medline].
Brown TH, Kairiss EW, Keenan CL (1990) Hebbian synapses: biophysical mechanisms and algorithms. Annu Rev Neurosci 13:475-511[Web of Science][Medline].
Castillo PE, Weisskopf MG, Nicoll RA (1994) The role of Ca²⁺ channels in hippocampal mossy fiber synaptic transmission and long-term potentiation. Neuron 12:261-269[Web of Science][Medline].
Chen WR, Lee S, Kato K, Spencer DD, Shepherd GM, Williamson A (1996) Long-term modifications of synaptic efficacy in the human inferior and middle temporal cortex. Proc Natl Acad Sci USA 93:8011-8015[Abstract/Free Full Text].
Cormier RJ, Mauk MD, Kelly PT (1993) Glutamate iontophoresis induces long-term potentiation in the absence of evoked presynaptic activity. Neuron 10:907-919[Web of Science][Medline].
Dunlap K, Luebke JI, Turner TJ (1995) Exocytotic Ca²⁺ channels in mammalian central neurons. Trends Neurosci 18:89-98[Web of Science][Medline].
Fagiolini M, Pizzorusso T, Berardi N, Domenici L, Maffei L (1994) Functional postnatal development of the rat primary visual cortex and the role of visual experience: dark rearing and monocular deprivation. Vision Res 34:709-720[Web of Science][Medline].
Fox AP, Nowycky MC, Tsien RW (1987) Kinetic and pharmacological properties distinguishing three types of calcium currents in chick sensory neurons. J Physiol (Lond) 394:149-172[Abstract/Free Full Text].
Freeman RD, Mallach R, Hartley S (1981) Responsivity of normal kitten striate cortex deteriorates after brief binocular deprivation. J Neurophysiol 45:1074-1084[Free Full Text].
Frégnac Y, Imbert M (1984) Development of neuronal selectivity in primary visual cortex of cat. Physiol Rev 64:325-434[Free Full Text].
Frey U, Krug M, Reymann KG, Matthies H (1988) Anisomycin, an inhibitor of protein synthesis, blocks late phases of LTP phenomena in the hippocampal CA1 region in vitro. Brain Res 452:57-65[Web of Science][Medline].
Fujii S, Saito K, Miyakawa H, Ito K, Kato H (1991) Reversal of long-term potentiation (depotentiation) induced by tetanus stimulation of the input to CA1 neurons of guinea pig hippocampal slices. Brain Res 555:112-122[Web of Science][Medline].
Galvez A, Gimenez-Gallego G, Reuben JP, Roy-Contancin L, Feigenbaum P, Kaczorowski GJ, Garcia ML (1990) Purification and characterization of a unique, potent, peptidyl probe for the high conductance calcium-activated potassium channels from venom of the scorpion Buthus tamulus. J Biol Chem 265:11083-11090[Abstract/Free Full Text].
Gustafsson B, Wigstrom H (1988) Physiological mechanisms underlying long-term potentiation. Trends Neurosci 11:156-162[Web of Science][Medline].
Hawkins RD, Kandel ER, Siegelbaum SA (1993) Learning to modulate transmitter release. Annu Rev Neurosci 16:625-665[Web of Science][Medline].
Hermann A, Hartung K (1982) Properties of a Ca²⁺ activated K⁺ conductance in Helix neurones investigated by intracellular Ca²⁺ ionophoresis. Pflügers Arch 393:248-253[Web of Science][Medline].
Hille B (1992) In: Ionic channels of excitable membranes. Sunderland, MA: Sinauer.
Jensen K, Jensen MS, Lambert JDC (1999) Role of presynaptic L-type Ca²⁺ channels in GABAergic synaptic transmission in cultured hippocampal neurons. J Neurophysiol 81:1225-1230[Abstract/Free Full Text].
Kasamatsu T, Pettigrew JD (1976) Depletion of brain catecholamine: failure of ocular dominance shift after monocular occlusion in kitten. Science 194:206-209[Abstract/Free Full Text].
Kirkwood A, Dudek SM, Gold JT, Aizenman CD, Bear MF (1993) Common forms of synaptic plasticity in the hippocampus and neocortex in vitro. Science 260:1518-1521[Abstract/Free Full Text].
Komatsu Y (1994) Age-dependent long-term potentiation of inhibitory synaptic transmission in rat visual cortex. J Neurosci 14:6488-6499[Abstract].
Komatsu Y (1996) GABA_B receptors, monoamine receptors, and postsynaptic inositol trisphosphate-induced Ca²⁺ release are involved in the induction of long-term potentiation at visual cortical inhibitory synapses. J Neurosci 16:6342-6352[Abstract/Free Full Text].
Komatsu Y, Iwakiri M (1993) Long-term modification of inhibitory synaptic transmission in developing visual cortex. NeuroReport 4:907-910[Web of Science][Medline].
Lancaster B, Nicoll RA (1987) Properties of two calcium-activated hyperpolarizations in rat hippocampal neurones. J Physiol (Lond) 389:187-203[Abstract/Free Full Text].
Lewis RS, Cahalan MD (1988) Subset-specific expression of potassium channels in developing murine T lymphocytes. Science 239:771-775[Abstract/Free Full Text].
Lisman J (1994) The CaM kinase II hypothesis for the storage of synaptic memory. Trends Neurosci 17:406-412[Web of Science][Medline].
Lynch G, Larson J, Kelso S, Barrionuevo G, Schotler F (1983) Intracellular injections of EGTA block induction of hippocampal long-term potentiation. Nature 305:719-721[Medline].
Mackenzie PJ, Umemiya M, Murphy TH (1996) Ca²⁺ imaging of CNS axons in culture indicates reliable coupling between single action potentials and distal functional release sites. Neuron 16:783-795[Web of Science][Medline].
MacKinnon R, Reinhart PH, White MM (1988) Charybdotoxin block of shaker K⁺ channels suggests that different types of K⁺ channels share common structural features. Neuron 1:997-1001[Web of Science][Medline].
Madison DV, Malenka RC, Nicoll RA (1991) Mechanisms underlying long-term potentiation of synaptic transmission. Annu Rev Neurosci 14:379-397[Web of Science][Medline].
Malenka RC, Kauer JA, Zucker RS, Nicoll RA (1988) Postsynaptic calcium is sufficient for potentiation of hippocampal synaptic transmission. Science 242:81-84[Abstract/Free Full Text].
Malgaroli A, Tsien RW (1992) Glutamate-induced long-term potentiation of the frequency of miniature synaptic currents in cultured hippocampal neurons. Nature 357:134-139[Medline].
Manabe T, Renner P, Nicoll RA (1992) Postsynaptic contribution to long-term potentiation revealed by the analysis of miniature synaptic currents. Nature 355:50-55[Medline].
Miller C, Moczydlowski E, Latorre R, Phillips M (1985) Charybdotoxin, a protein inhibitor of single Ca²⁺-activated K⁺ channels from mammalian skeletal muscle. Nature 313:316-318[Medline].
Miller SG, Kennedy MB (1986) Regulation of brain type II Ca²⁺/calmodulin-dependent protein kinase by autophosphorylation: a Ca²⁺-triggered molecular switch. Cell 44:861-870[Web of Science][Medline].
Mintz IM, Adams ME, Bean BP (1992) P-type calcium channels in rat central and peripheral neurons. Neuron 9:85-95[Web of Science][Medline].
Narahashi T (1974) Chemicals as tools in the study of excitable membranes. Physiol Rev 54:813-889[Free Full Text].
Narahashi T, Tsunoo A, Yoshii M (1987) Characterization of two types of calcium channels in mouse neuroblastoma cells. J Physiol (Lond) 383:231-249[Abstract/Free Full Text].
Nguyen PV, Abel T, Kandel ER (1994) Requirement of a critical period of transcription for induction of a late phase of LTP. Science 265:1104-1107[Abstract/Free Full Text].
Pettit DL, Perlman S, Malinow R (1994) Potentiated transmission and prevention of further LTP by increased CAMKII activity in postsynaptic hippocampal slice neurons. Science 266:1881-1885[Abstract/Free Full Text].
Plummer MR, Logothetis DE, Hess P (1989) Elementary properties and pharmacological sensitivities of calcium channels in mammalian peripheral neurons. Neuron 2:1453-1463[Web of Science][Medline].
Regehr WG, Delaney K, Tank DW (1994) The role of presynaptic calcium in short-term enhancement at the hippocampal mossy fiber synapse. J Neurosci 14:523-537[Abstract].
Reuter H (1996) Diversity and function of presynaptic calcium channels in the brain. Curr Opin Neurobiol 6:331-337[Web of Science][Medline].
Saitoh T, Schwartz JH (1985) Phosphorylation-dependent subcellular translocation of a Ca²⁺/calmodulin-dependent protein kinase produces an autonomous enzyme in Aplysia neurons. J Cell Biol 100:835-842[Abstract/Free Full Text].
Salin PA, Prince DA (1996) Spontaneous GABA_A receptor-mediated inhibitory currents in adult rat somatosensory cortex. J Neurophysiol 75:1573-1588[Abstract/Free Full Text].
Sather WA, Tanabe T, Zhang J-F, Mori Y, Adams ME, Tsien RW (1993) Distinctive biophysical and pharmacological properties of class A (BI) calcium channel $alpha$ ₁ subunits. Neuron 11:291-303[Web of Science][Medline].
Schweitz H, Stansfeld CE, Bidard J-N, Fagni L, Maes P, Lazdunski M (1989) Charybdotoxin blocks dendrotoxin-sensitive voltage-activated K⁺ channels. FEBS Lett 250:519-522[Web of Science][Medline].
Staubli U, Lynch G (1990) Stable depression of potentiated synaptic responses in the hippocampus with 1-5 Hz stimulation. Brain Res 513:113-118[Web of Science][Medline].
Storm JF (1987) Action potential repolarization and a fast after-hyperpolarization in rat hippocampal pyramidal cells. J Physiol (Lond) 385:733-759[Abstract/Free Full Text].
Swandulla D, Hans M, Zipser K, Augustine GJ (1991) Role of residual calcium in synaptic depression and posttetanic potentiation: fast and slow calcium signaling in nerve terminals. Neuron 7:915-926[Web of Science][Medline].
Thesleff S (1980) Aminopyridines and synaptic transmission. Neuroscience 5:1413-1419[Web of Science][Medline].
Tzounopoulos T, Janz R, Sudhof TC, Nicoll RA, Malenka RC (1998) A role for cAMP in long-term depression at hippocampal mossy fiber synapses. Neuron 21:837-845[Web of Science][Medline].
Wheeler DB, Randall A, Tsien RW (1994) Roles of N-type and Q-type Ca²⁺ channels in supporting hippocampal synaptic transmission. Science 264:107-111[Abstract/Free Full Text].
Wu LG, Saggau P (1994) Presynaptic calcium is increased during normal synaptic transmission and paired-pulse facilitation, but not in long-term potentiation in area CA1 of hippocampus. J Neurosci 14:645-654[Abstract].
Zhang J-F, Randall AD, Ellinor PT, Horne WA, Sather WA, Tanabe T, Schwarz TL, Tsien RW (1993) Distinctive pharmacology and kinetics of cloned neuronal Ca²⁺ channels and their possible counterparts in mammalian CNS neurons. Neuropharmacology 32:1075-1088[Web of Science][Medline].

Copyright © 2000 Society for Neuroscience 0270-6474/00/20207539-08$05.00/0

This article has been cited by other articles:

I. Brosh and E. Barkai
Learning-induced enhancement of feedback inhibitory synaptic transmission
Learn. Mem., June 19, 2009; 16(7): 413 - 416.
[Abstract] [Full Text] [PDF]

F. S. Nugent and J. A. Kauer
LTP of GABAergic synapses in the ventral tegmental area and beyond
J. Physiol., March 15, 2008; 586(6): 1487 - 1493.
[Abstract] [Full Text] [PDF]

Y. Ben-Ari, J.-L. Gaiarsa, R. Tyzio, and R. Khazipov
GABA: A Pioneer Transmitter That Excites Immature Neurons and Generates Primitive Oscillations
Physiol Rev, October 1, 2007; 87(4): 1215 - 1284.
[Abstract] [Full Text] [PDF]

A. Katoh, J. A. Jindal, and J. L. Raymond
Motor Deficits in Homozygous and Heterozygous P/Q-Type Calcium Channel Mutants
J Neurophysiol, February 1, 2007; 97(2): 1280 - 1287.
[Abstract] [Full Text] [PDF]

K. Yamada, T. Inagaki, R. Funahashi, Y. Yoshimura, and Y. Komatsu
High-Frequency Stimulation Together with Adrenoceptor Activation Facilitates the Maintenance of Long-Term Potentiation at Visual Cortical Inhibitory Synapses
Cereb Cortex, September 1, 2006; 16(9): 1239 - 1248.
[Abstract] [Full Text] [PDF]

G. Ohtsuki, S.-y. Kawaguchi, M. Mishina, and T. Hirano
Enhanced Inhibitory Synaptic Transmission in the Cerebellar Molecular Layer of the GluR{delta}2 Knock-Out Mouse
J. Neurosci., December 1, 2004; 24(48): 10900 - 10907.
[Abstract] [Full Text] [PDF]

H. N. Liu, T. Kurotani, M. Ren, K. Yamada, Y. Yoshimura, and Y. Komatsu
Presynaptic Activity and Ca2+ Entry Are Required for the Maintenance of NMDA Receptor-Independent LTP at Visual Cortical Excitatory Synapses
J Neurophysiol, August 1, 2004; 92(2): 1077 - 1087.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (18)

Citing Articles via Google Scholar

Google Scholar

Articles by Komatsu, Y.

Articles by Yoshimura, Y.

Search for Related Content

PubMed

PubMed Citation

Articles by Komatsu, Y.

Articles by Yoshimura, Y.

Pubmed/NCBI databases
Compound via MeSH
Substance via MeSH