Activation of Group II Metabotropic Glutamate Receptors Induces Long-Term Depression of Synaptic Transmission in the Rat Amygdala

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The Journal of Neuroscience, December 15, 2000, 20(24):9017-9024

Activation of Group II Metabotropic Glutamate Receptors Induces Long-Term Depression of Synaptic Transmission in the Rat Amygdala
Hui-Ching Lin, Su-Jane Wang, Ming-Zen Luo, and Po-Wu Gean
Department of Pharmacology, College of Medicine, National Cheng-Kung University, Tainan, Taiwan 701

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

An animal model most sensitive for measuring anticipatory anxiety is fear conditioning, which is expressed by an enduringincrease in synaptic strength in the amygdala. A converse viewpredicts that agents that induce long-term depression (LTD) ofsynaptic efficacy in the amygdala may be useful in the ameliorationof stress disorders. In the present study, we show that activationof group II metabotropic glutamate receptor (mGluR II) by (2S,3S,4S)-2-(carboxycyclopropyl)glycine (L-CCG) induces an LTD in the basolateral amygdala neurons.The effect was concentration-dependent with a maximal inhibitionof ~30%. The induction of L-CCG LTD required concurrent synapticactivity, required presynaptic but not postsynaptic Ca²⁺ increases, and was independent of NMDA receptors. L-CCG LTD wasassociated with an increase in the ratio of paired-pulse facilitationand was not occluded by low-frequency stimulation-induced LTD,suggesting that these two forms of LTD did not share a commonunderlyingmechanism.
After eliciting LTD with L-CCG, application of isoproterenol increased the synaptic responses back to its original baseline,demonstrating that chemically depressed synapses could be potentiatedby another chemical. A selective PKA inhibitor, KT 5720, by itsown caused a depression of synaptic transmission and blocked L-CCGLTD, presumably by mimicking and thereby occluding any furtherdepression. Together, these results suggest that L-CCG LTD isinduced by presynaptically mGluR II-mediated inhibition of Ca²⁺-sensitive adenylyl cyclase, resulting in a decrease in cAMP formationand PKA activation, which leads to a long-lasting decrease intransmitterrelease.

Key words: amygdala; cAMP; PKA; synaptic plasticity; LTD; mGluR

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The amygdala has been suggested to include an essential circuit for certain forms of neuroplasticity, such as emotional memoryand epilepsy (Goddard et al., 1969; Davis et al., 1994; LeDoux1994). One cellular model thought to store aversive emotionalexperiences in this structure is fear conditioning, which consistsof freezing behavior evoked by the pairing of a conditioned stimulus(CS), such as a tone, with a noxious unconditioned footshock.The neural pathways mediating fear conditioning involve the transmissionof sensory information about the CS to the lateral nucleus ofamygdala (LA), which then projects to the basolateral nucleus(BLA) and other amygdala regions (LeDoux et al., 1990; Pitkanenet al., 1997; Maren, 1999). Several lines of evidence indicatethat the BLA plays an important role in both acquisition and expressionof conditioned fear. For example, reversible inactivation of theBLA neurons with lidocaine (Parent and McGaugh, 1994), as wellas blockade of NMDA or glucocorticoid receptors in the BLA (Miserendinoet al., 1990; Fanselow and Kim, 1994; Liang et al., 1994; Roozendaaland McGaugh, 1997), prevents the acquisition of conditioned fear.Thus, the BLA receives synaptic input from many primary sensorystructures, and lesion of this structure yields deficits in Pavlovianfearconditioning.

Long-term potentiation (LTP) of synaptic responses, triggered by high-frequency stimulation (HFS) of excitatory afferents,is a leading cellular mechanism for learning and memory (Blissand Collingridge, 1993). In view of the facts that fear conditioninginduces increases in amygdala synaptic transmission that resembleLTP (McKernan and Shinnick-Gallagher, 1997; Rogan et al., 1997),it is hypothesized that they may share a common mechanism (Maren,1999). This hypothesis receives convincing support from geneticstudies of mice that lack RasGRE, a neuron-specific guanine nucleotide-releasingfactor. These mice have profound deficits in amygdala LTP, aswell as impairments in consolidation of long-term memories forfear conditioning to both contextual and acoustic stimuli (Brambillaet al., 1997). If this theory is correct, one may predict thatdrugs that induce the converse form of LTP, long-term depression(LTD), of synaptic efficacy in the amygdala is useful for theamelioration of conditionedfear.

Recently, we have demonstrated that homosynaptic LTD could be induced at the amygdala LA-BLA synapse by prolonged low-frequencystimulation (LFS) (Wang and Gean, 1999). The induction of LTDrequired activation of NMDA receptors, postsynaptic Ca²⁺ increases, and phosphatase activity. Thus, the induction of LFSLTD is likely at the postsynaptic site. In the present study,we have investigated the role of group II metabotropic glutamatereceptor (mGluR II) in the induction of LTD using its selectiveagonist (2S,3S,4S)-2-(carboxycyclopropyl) glycine (L-CCG). Wefound that chemical-induced LTD is NMDA receptor-independent.It requires synaptic activation and presynaptic, but not postsynaptic,Ca²⁺ increases and is associated with an increase in paired-pulsefacilitation (PPF). These results suggest that, in contrast toLFS LTD, L-CCG LTD is induced and expressedpresynaptically.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Slice preparation. Male Sprague Dawley 4- to 6-week-old rats were decapitated, and their brains were rapidly removed and placedin cold oxygenated artificial CSF (ACSF) solution. Subsequently,the brain was hemisected and cut transversely posterior to thefirst branch and anterior to the last branch of the superior cerebralvein. The resulting section was glued to the chuck of a Vibroslicetissue slicer (Campden Instruments, Silbey, UK). Transverse slicesof 500 µm thickness were cut, and the appropriate slices wereplaced in a beaker of oxygenated ACSF at room temperature forat least 1 hr before recording. ACSF solution had the followingcomposition (in mM): NaCl 117, KCl 4.7, CaCl₂ 2.5, MgCl₂ 1.2,NaHCO₃ 25, NaH₂PO₄ 1.2, and glucose 11. The ACSF was bubbled continuouslywith 95%O₂-5%CO₂ and had the pH of 7.4.

Intracellular recordings. A single slice was transferred to the recording chamber in which it was held submerged between twonylon nets and maintained at 32 ± 1°C. The chamber consisted ofa circular well of a low volume (1-2 ml) and was perfused constantlyat a rate of 2-3ml/min. Intracellular recording microelectrodeswere pulled from 1.0 mm microfiber capillary tubing on a Brown-Flamingelectrode puller (Sutter Instruments, San Rafael, CA). The electrodeswere filled with 4 M potassium acetate with resistance rangingfrom 70 to 130 M $Omega$ . For chelating intracellular Ca²⁺, the electrodes were filled with 50 mM BAPTA in addition to 3M potassium acetate. When BAPTA-containing electrodes were used,loading of the cells with BAPTA was assayed by the blockade ofCa²⁺-activated afterhyperpolarization. The microelectrode tips werepositioned into theBLA.

Monosynaptic EPSPs were evoked in BLA neurons by electrical stimulation of afferents from the lateral nucleus of amygdalawith a concentric bipolar stimulating electrode (SNE-100; DavidKopf Instruments, Bern, Germany). Electrical stimuli (150 µsecin duration) were delivered at a frequency of 0.05 Hz. To induceLTD, LFS protocol was used, which consists of 900 pulses, deliveredat 1 Hz at the same stimulation intensity used for baseline. Alldata were expressed as mean ± SEM. Statistical analysis was performedusing the Student's t test, and p < 0.05 was considered statisticallysignificant.

Drug application. Drugs were applied directly to the ACSF using a continuous gravity-fed bath application, and the concentrationof applied drug reached equilibrium within 2-3 min. L-CCG, BAPTA-AM,and D-2-amino-5-phosphonovalerate (D-APV) were obtained from ResearchBiochemicals (Natick, MA). 2S,1S'2S'-2-methyl-2-(2'-carboxycyclo-propyl)glycine(MCCG) and (2S)- $alpha$ -ethylglutamic acid (EGLU) were obtained fromTocris Cookson. (Bristol, UK). KT 5720 was obtained from Calbiochem-NovabiochemInternational (San Diego,CA).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

LTD induced by L-CCG

Figure 1 illustrates the effect of a selective mGluR II agonist L-CCG on EPSP in BLA neurons. Superfusion of L-CCG for 10-15min caused a rapid depression of EPSP, which was maintained inthe presence of L-CCG. After washout of L-CCG, the amplitude ofEPSP was only partially recovered to a stable response that wasdepressed relative to the initial baseline value. This L-CCG-inducedLTD typically was stable for at least 60 min; therefore, we usedthe magnitude of LTD at this time point for statistical comparison.The effect of L-CCG was concentration-dependent. One, 10, and30 µM produced an initial depression measuring $-$ 17.1 ± 2.1% (n= 16), $-$ 55.4 ± 4.3% (n = 12) and $-$ 61.0 ± 3.6% (n = 8), respectively,and LTD measuring $-$ 18.8 ± 2.9% (n = 16), $-$ 31.5 ± 3.0% (n = 12),and $-$ 35.0 ± 3.9% (n = 8), respectively (Fig. 1B). Furthermore,the effect of L-CCG was mimicked by another selective mGluR IIagonist (2S,1'R,2'R,3'R)-(2',3'-dicarboxycyclopropyl)glycine (DCG-IV).Superfusion of DCG-IV (2 µM) caused an initial depression of $-$ 46.2± 6.0% (n = 5) and was followed by an LTD with the magnitude of $-$ 29.3 ± 10.1% (n = 5). L-CCG (10 µM)-induced LTD was not attributableto an alteration of resting membrane potential (RMP) or neuronalinput resistance (IR) of the BLA neurons (RMP and IR were $-$ 67.0± 1.6 mV and 45.5 ± 3.3 M $Omega$ before, and $-$ 66.0 ± 1.3 mV and 45.6± 2.4 M $Omega$ 60 min after the washout of L-CCG) (cf. Neugebauer etal., 1997)

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Figure 1. Concentration-dependent depression of EPSP by L-CCG. A, Application of L-CCG for 10 min resulted in an initial depression of EPSP, which was followed, upon washout of the L-CCG, by LTD. B, Concentration-dependent effects of L-CCG on the initial depression and LTD.

We have shown previously that LFS consistently induced LTD at the LA-BLA synapse but not at the ventral endopyriform nucleus(VEN)-BLA synapse (Wang and Gean, 1999). To test whether L-CCG-inducedLTD is also restricted at the LA-BLA synapse, we performed theexperiments by placing the stimulating electrode on the VEN. Insix neurons tested, L-CCG (10 µM) similarly induced an LTD atthis pathway ( $-$ 30.7 ± 3.6%, 60 min after the washout of L-CCG;n =6).

Block of L-CCG-induced LTD by mGluR II antagonists

MCCG (100 µM), a selective antagonist for mGluR II, by itself did not affect EPSP significantly (97.8 ± 3.5% of control; n= 9; p > 0.1). However, as illustrated in Figure 2A, it blockedthe initial depression as well as the LTD induced by L-CCG. Inthe presence of MCCG, the initial depression and LTD induced byL-CCG were only $-$ 12.4 ± 4.4 (n = 9) and $-$ 9.6 ± 4.9% (n = 9), respectively,which were significantly less than that of without MCCG pretreatment(p < 0.001; unpaired t test for both initial depression and LTD).

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Figure 2. Blockade of L-CCG-induced LTD by mGluR II antagonists. A, Application of L-CCG (10 µM) in the presence of MCCG (100 µM) failed to cause initial depression and LTD. Inset shows superimposed traces taken at the time points indicated. B, Application of EGLU (10 µM) did not affect the EPSP significantly but blocked the effect of L-CCG (10 µM). Inset shows the traces taken at the time points indicated.

Another mGluR II antagonist, EGLU (Jane et al., 1996), was also examined. Consistent with a previous report (Li et al., 1998),superfusion of EGLU (10 µM) did not affect the amplitude of EPSP(101 ± 1% of control; n = 7) but blocked the effect of L-CCG onEPSP (Fig. 2B). In the presence of EGLU, the initial depressionand LTD induced by L-CCG were 2.8 ± 4.1 (n = 7) and 0.1 ± 3.5%(n = 7), respectively, which were considerably less than in controlneurons (p < 0.001 for both initial depression and LTD). Furthermore,the effect of EGLU was not mimicked by the selective mGluR I antagonist7-(hydroxyimino)cyclopropa[b]chromen-1a-carboxylate ethyl ester(CPCCOEt). The initial depression and LTD induced by L-CCG (10µM) in the presence of CPCCOEt (100 µM) were $-$ 39.1 ± 5.2 and $-$ 29.7± 8.8% (n = 3), respectively. Similarly, the group III mGluR antagonist(S)-2-methyl-2-amino-4-phosphonobutyrate (100 µM) itself affectedneither synaptic transmission (107 ± 5%; n = 5) nor the LTD byL-CCG (10 µM) ( $-$ 28.6 ± 5.0%; n = 5). These results confirm themediation of LTD by group IImGluR.

L-CCG-induced LTD is independent of NMDA receptor activation

To determine whether NMDA receptor plays a role in L-CCG-induced LTD, NMDA receptor antagonist D-APV was applied before perfusionof L-CCG. Figure 3A shows that application of L-CCG (10 µM) inD-APV (50 µM) resulted in an initial depression of EPSP, whichmeasured $-$ 58 ± 5% (n = 7), and was followed by an LTD with themagnitude of $-$ 31 ± 6% (n = 7). These values were indistinguishablefrom those observed in the absence of D-APV.

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Figure 3. LTD induced by L-CCG is independent of NMDA receptor activation and is accompanied by an increase in PPF. A, Application of L-CCG (10 µM) in the presence of D-APV (50 µM) induced LTD that was not significantly different from control LTD. B, EPSPs evoked by paired stimuli in control and 60 min after the washout of L-CCG (10 µM). The control EPSP evoked by the first stimulus is scaled to that recorded 60 min after LTD induction. It is clear that there is a greater PPF after L-CCG LTD.

To localize the site of expression, we explored the effect of L-CCG on PPF, because if L-CCG LTD involves presynaptic mechanisms,then it might be associated with an increase in PPF (Manabe etal., 1993; Schulz et al., 1994). A typical experiment is shownin Figure 3B in which a pair of synaptic responses was elicitedwith an interstimulus interval of 60 msec, and the ratio of PPFwas compared between control and after LTD was induced. The resultof seven experiments revealed that PPF was increased to 122 ±6% (n = 7; p < 0.01) of baseline 60 min after LTDinduction.

L-CCG-induced LTD and LFS-induced LTD are not mutually occluded

LTD induced by LFS requires NMDA receptor activation, whereas L-CCG LTD does not, suggesting different mechanisms of induction.We tested this prediction by performing occlusion experiments.In a first set of experiments, L-CCG LTD was saturated by givinga concentration of 10 µM, which induced the maximal LTD (Fig.1). We then compared the magnitude of LTD induced under this conditionwith that induced without L-CCG pretreatment. A summary of nineexperiments is shown in Figure 4A in which L-CCG elicited an initialdepression of $-$ 51.7 ± 4.8% and an LTD of $-$ 29.6 ± 2.9%. SubsequentLFS produced a further LTD ( $-$ 14.3 ± 3.4%; n = 9; p < 0.01; pairedt test). When the data were renormalized to the 10 min precedingapplication of LFS, responses were calculated to be depressedby 20.3 ± 3.4%. Thus, LFS was still able to elicit LTD, althoughits magnitude was less than that without previous applicationof L-CCG ( $-$ 39.8 ± 8.5%; n = 16; p < 0.05; unpaired t test).

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Figure 4. L-CCG-induced LTD and LFS-induced LTD are not mutually occluded. A, One application of 10 µM L-CCG for 15 min was given to saturate LTD. Sixty minutes after washout of L-CCG, 1 Hz stimulation (900 pulses, 15 min) was delivered. LFS produced a further depression. B, An example of experiments showing that, after LTD was induced to a maximal level by three periods of LFS, subsequent application of L-CCG (10 µM) induced a further LTD.

To further address this question, we performed the reverse occlusion experiment in which LTD was induced by LFS before L-CCGwas applied. An example of these experiments is shown in Figure4B. LTD was induced to a maximal level (~50%) by three epochsof LFS as indicated by a lack of further depression in responseto the final epoch. Subsequent application of L-CCG (10 µM) stillinduced a 12.5% LTD (25% if normalized to pre-L-CCG level) at60 min after washout of L-CCG. In nine neurons, under this condition,L-CCG (10 µM) elicited an average of 18.4 ± 3.1% (n = 8; p < 0.05;paired t test) of LTD, but its magnitude was less than that ofuntreated control slices ( $-$ 31.5 ± 3.0%; n = 12; p < 0.05; unpairedttest).

Requirements of synaptic activity and presynaptic Ca²⁺ entry for L-CCG-induced LTD

To determine whether synaptic activation was required for L-CCG-induced LTD, experiments were performed in which synapticstimulation was ceased both during the application of L-CCG and10 min after the washout, thereby avoiding Ca²⁺ entry into presynaptic boutons during application of L-CCG. Asshown in Figure 5, L-CCG did not induce LTD in the absence ofsynaptic stimulation. At 60 min after washout of L-CCG, the EPSPamplitude measured 91.8 ± 7.4% (n = 8; p > 0.1).

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Figure 5. Induction of L-CCG LTD is dependent on presynaptic activity. Summary of eight experiments showing that L-CCG LTD was blocked when synaptic stimulation was stopped both during the application of L-CCG (10 µM) and 10 min after the washout.

To determine whether a rise in presynaptic Ca²⁺ is required for the action of L-CCG, we buffered intraterminal Ca²⁺ using a membrane-permeant Ca²⁺ chelator, BAPTA-AM. Application of BAPTA-AM (100 µM) reducedthe EPSP amplitude by 38.9 ± 4.6% (n = 8) and, in the presenceof BAPTA-AM, L-CCG (10 µM) no longer induced initial depression(1.4 ± 1.2%; n = 8) or LTD ( $-$ 0.8 ± 5.9%; n = 8) (Fig. 6A). Todifferentiate presynaptic versus postsynaptic sites of action,we loaded the recorded postsynaptic neuron with BAPTA salt. Afterimpalement, the cells were allowed to stabilize for at least 30min to allow the cell to fill with BAPTA, which was manifestedby blockade of slow afterhyperpolarization (Fig. 6B). Baselineresponses were then obtained for an additional 10 min before superfusingL-CCG. As shown in Figure 6C, L-CCG still induced initial depressionand LTD, measured $-$ 55.0 ± 3.5 and $-$ 25.0 ± 3.6% (n = 7), respectively.These values were not significantly different from those recordedwith control electrodes. Collectively, these results suggest thatan activity-mediated change in presynaptic but not postsynapticCa²⁺ level is required for L-CCG-induced LTD.

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Figure 6. Presynaptic but not postsynaptic Ca²⁺ increase is required for L-CCG LTD. A, Summary of eight experiments showing that the membrane-permeable Ca²⁺ chelator BAPTA-AM (100 µM) suppressed synaptic transmission and blocked L-CCG LTD. B, Superimposed traces taken immediately (1 min) and 30 min after the impalement of cell with a BAPTA-containing electrode to show the block of afterhyperpolarization. Electrode was filled with BAPTA (50 mM) as described in Materials and Methods. C, LFS LTD but not L-CCG LTD was blocked by intracellular BAPTA.

L-CCG-induced LTD can be reversed by isoproterenol-induced LTP

We sought to determine whether chemically depressed synapses could be potentiated by another chemical. After eliciting LTDwith L-CCG, we applied isoproterenol (Iso). Iso was used becauseprevious studies from this laboratory have shown that stimulationof $beta$ -adrenoceptors resulted in long-term enhancement of excitatorysynaptic responses in the BLA neurons (Huang et al., 1996). Asshown in Figure 7A, 20 min after LTD induction ( $-$ 25.8 ± 4.6%;n = 7), application of Iso (15 µM) increased synaptic strengthback to the original control level (107.7 ± 8.2%, measured at60 min after the washout of Iso; n = 7). To further examine whetherIso-induced LTP could be depotentiated by L-CCG, we applied Isoand L-CCG in the reverse order. Figure 7B shows a summary of eightexperiments in which Iso (15 µM) induced LTP that stabilized at138.4 ± 5.6% (n = 8) of baseline level (20 min after Iso; n =8). L-CCG (10 µM) application 20 min after the washout of Isocaused a complete reversion of LTP. The EPSP amplitude was returnedto 88.4 ± 6.5% (n = 8) of the initial control 60 min after L-CCG.

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Figure 7. L-CCG LTD can be potentiated by Iso. A, Application of L-CCG (10 µM) induced an LTD. Twenty minutes after LTD stabilized, Iso (15 µM) was applied, which increased the synaptic strength back to the original level. B, Parallel experiments in which L-CCG and Iso were applied in the reverse order. Application of Iso (15 µM) induced an LTP. L-CCG (10 µM) application 20 min after the washout of Iso caused a complete reversal of LTP.

Involvement of protein kinase A in L-CCG-induced LTD

Mediating through G-proteins of G_i/G_o classes, mGluR II is coupled negatively to adenylyl cyclase and thereby inhibits theformation of cAMP (Pin and Duvoisin, 1995). If mGluR-mediateddecrease in cAMP level is necessary for triggering LTD, then pharmacologicalinhibition of cAMP and cAMP-dependent protein kinase A (PKA) shouldmimic the effect of L-CCG. We tested this possibility by applicationof KT5720, a PKA catalytic site antagonist. Application of KT5720(1 µM) gradually reduced the amplitude of EPSP. The amplitudesof EPSP were 80.6 ± 3.3, 50.4 ± 2.9, and 50.5 ± 4.1% (n = 3) at30, 60, and 90 min after the application ofdrug.

We next addressed the question of whether a decrease in PKA activity is important for L-CCG-induced LTD. To perform theseexperiments, slices were incubated in 1 µM KT 5720 for at least1 hr before being transferred to the recording chamber in whichthe same concentration of KT 5720 was maintained. As shown inFigure 8, L-CCG (10 µM) failed to induce LTD under this condition(100 ± 1% of control, measured at 60 min after the washout ofL-CCG; n = 6). It is noted that L-CCG still caused an initialdepression when PKA activity was inhibited by KT 5720. These resultssuggest that the initial depression of transmitter release elicitedby mGluR activation is not attributable to a decrease in cAMP.This conclusion was supported by the observation that inhibitionof adenylyl cyclase with SQ 22536 (50 µM) completely abolishedthe induction of LTD (5.3 ± 4.3%; n = 6) without blocking theinitial depression of EPSP by 10 µM L-CCG ( $-$ 38.2 ± 4.8%; n = 6).

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Figure 8. L-CCG LTD is blocked by adenylyl cyclase and PKA inhibitors. A, Slices were incubated for at least 1 hr in 1 µM KT 5720 or 20 min in 50 µM SQ 22536 before being transferred to the recording chamber in which the same concentration of drug was maintained. L-CCG LTD normally observed in control slices was blocked in the KT 5720- or SQ 22536-treated slices. Inset shows the representative traces taken before and 60 min after the washout of L-CCG. Calibration: 10 mV, 40 msec. B, Block of L-CCG-induced initial depression by PMA. Slices were incubated for at least 1 hr in KT 5720 (1 µM) plus PMA (1 µM). Inset shows the representative traces taken before and 60 min after the washout of L-CCG. Calibration: 10 mV, 40 msec.

Several G-protein-coupled receptors, such as mGluR II, GABA_B, and adenosine A₁ receptors, exert inhibitory action on the synaptictransmission. Activation of these receptors also depresses voltage-dependentCa²⁺ channels. Both G-protein-coupled receptor-mediated presynapticinhibition and Ca²⁺ channel depression could be disrupted by phorbol esters (Swartzet al., 1993), the protein kinase C (PKC) activators, suggestingthat PKC may phosphorylate and consequently inactivate some classesof G-protein mediating these actions. We therefore tested whetherPKC activation can influence mGluR II-mediated synaptic depression.In these experiments, slices were incubated for at least 1 hrin 1 µM KT 5720 to eliminate L-CCG LTD. As illustrated in Figure8B, L-CCG-induced transient depression was blocked by the pretreatmentof slices with the PKC activator PMA (1 µM).

Endogenous activation of mGluR II

It has been suggested that neurotransmitters uptake into neurons and glial cells is the major mechanism by which synapticallyreleased neurotransmitter is removed from the extracellular space.To investigate whether synaptically released glutamate is capableof diffusing to presynaptic terminals and inducing LTD by activatingat mGluR II, glutamate release is increased by HFS (100 Hz, 1sec) and by blocking glutamate uptake (Scanziani et al., 1997).In these experiments, the slices were perfused with D-APV (50µM) to prevent NMDA receptor-dependent LTP and LTD. In the initialexperiments, HFS elicited a post-tetanic potentiation, which wasfollowed by an LTD in only 6 of 15 neurons tested. If mGluR activationdepends on the spread of glutamate, the activation of these receptorsshould be enhanced by blocking the uptake of glutamate. Indeed,when the glutamate uptake blocker L-trans-pyrrolidine-2,4-dicarboxylicacid (trans-PDC) (100 µM) was applied, HFS induced an LTD in allseven neurons tested ( $-$ 29.4 ± 3.6, 60 min after the stimulation;n = 7). We next tested whether mGluR II was involved in EPSP depressionby applying MCCG (100 µM). In the presence of this mGluR II antagonist,HFS-induced LTD was blocked ( $-$ 4.8 ± 2.9%, 60 min after the stimulation;n = 6), providing evidence that EPSP depression was caused bymGluR activation (Fig. 9).

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Figure 9. Glutamate release by brief titanic stimulation activates presynaptic mGluR II and induces LTD. In the presence of D-APV (50 µM) and the glutamate uptake inhibitor trans-PDC (100 µM), brief titanic stimulation (100 Hz, 1 sec) evoked an LTD that was completely blocked by MCCG (100 µM). Inset shows the representative traces taken before and 60 min after the stimulation. Calibration: 10 mV, 40 msec.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present results, in combination with previous work, clearly show that there are two forms of LTD that coexist at the samesynapses of the rat amygdala. Both induction and expression mechanismsappear to be completely different; one induced by a mGluR II agonistrequires Ca²⁺ influx into presynaptic terminals and is expressed by an enhancedtransmitter release, and the other triggered by prolonged LFSis NMDA receptor-dependent and expressed postsynaptically. Importantly,like electrically induced synaptic plasticity, the same synapsesthat had undergone chemical-induced LTD could subsequently bepotentiated by another chemical. Moreover, we have provided thefirst evidence that, when glutamate concentration is increasedby high-frequency activity and by blocking glutamate uptake, mGluRsbecome activated, leading to an LTD of synaptic transmission.The use-dependent activation of presynaptic mGluRs that we describehere thus may have important physiological functions related tothe amygdala, such as fear conditioning and kindlingepileptogenesis.

Characteristics of L-CCG LTD

In this study, we have demonstrated that LTD can be induced in the basolateral nucleus of the rat amygdala by L-CCG, a selectivemGluR II agonist. The effect of L-CCG is concentration-dependentwith a maximal depression of ~30%. The blockade of L-CCG-inducedLTD by the selective mGluR II antagonists MCCG and EGLU confirmsthe mediation by mGluR II. LTD was not caused by a slow washoutof L-CCG because application of MCCG during the washing perioddid not affect the magnitude of LTD (our unpublished observation).Furthermore, potentiation consistently did occur in response toIso after induction of LTD, which argues strongly against excitotoxicityas a mechanism for the observed synapticdepression.

Group II mGluRs are located both presynaptically and postsynaptically, and their involvement in the induction of LTD has beendescribed at the hippocampal mossy fiber-CA3 (Yokoi et al., 1996;Domenici et al., 1998; Tzounopoulos et al., 1998), medial perforantpath-dentate gyrus (Huang et al., 1999), and the perirhinal cortex(Cho et al., 2000). In these studies, the locus of mGluR II responsiblefor LTD induction is not consistent; some studies favored a postsynapticmechanism for mGluR II-mediated LTD (Huang et al., 1999; Cho etal., 2000), whereas others suggested a presynaptic mGluR II-mediatedlong-lasting depression of transmitter release (Tzounopoulos etal., 1998; Kobayashi et al., 1999). We have reported previouslythat LTD could be reliably induced in the amygdala by LFS, whichrequires activation of both NMDA and mGluRs, and depends on postsynapticCa²⁺ increases and phosphatase activity. The precise mechanisms underlyingthe synergy between NMDA and mGluRs in the LTD induction remainto be identified. However, as described recently for LFS LTD inthe perirhinal cortex (Cho et al., 2000), it is possible thatmGluR II facilitates mGluR I-mediated increases in intracellularCa²⁺. This facilitation plus NMDA receptor activation may be necessaryfor LTD induction at resting membrane potentials. Thus, in theamygdala, mGluR II may play an important role in both presynapticand postsynaptic forms ofLTD.

The lack of effect of loading postsynaptic cells with Ca²⁺ chelator to impede L-CCG LTD strongly suggests that this form ofLTD is independent of postsynaptic Ca²⁺ influx. This finding, together with the blockade of LTD by extracellularperfusion of membrane-permeable Ca²⁺ chelator, indicates that an elevation of presynaptic Ca²⁺ is crucial for L-CCG-induced LTD in the amygdala. The resultsalso show that L-CCG LTD is dependent on presynaptic activitybut is not dependent on NMDA receptor activation. This reinforcesthe notion that postsynaptic mechanisms may not be involved because,in pathways in which postsynaptic mechanism is important, LTDinduction is usually blocked by NMDA receptor antagonists (Dudekand Bear, 1992; Mulkey and Malenka, 1992) and is not dependenton presynaptic activity. In addition, an increase in PPF duringL-CCG LTD provides further evidence that not only the inductionbut also the expression is presynaptic and caused by a decreasein transmitter release. The selective PKA inhibitor KT 5720 onits own caused a depression of synaptic transmission and blockedL-CCG LTD, presumably by mimicking and thereby occluding any furtherdepression. Therefore, one potential mechanism by which presynapticCa²⁺ entry could be linked to LTD induction is mGluR II-mediated decreasein Ca²⁺-sensitive adenylyl cyclase activity, which leads to a decreasein cAMP formation and the activity of PKA, resulting in a long-lastingdecrease in transmitter release. These data, combined with previouswork on Iso-induced LTP (Huang et al., 1996), provides evidencethat synaptic plasticity in the amygdala neurons is at least partiallycontrolled by the presynaptic cAMP-PKA signalingpathway.

In the presence of KT 5720 or SQ 22536, L-CCG is no longer able to induce an LTD but is still capable of causing an initialdepression of synaptic transmission. These results suggest thatL-CCG has effects on the initial depression and LTD may be mediatedthrough different mechanisms. One type of inhibitory pathway couplingneurotransmitter receptors to voltage-dependent Ca²⁺ channels involves G-proteins and is membrane delimited (Hille,1994). This inhibitory pathway is generally thought to be responsiblefor neurotransmitter-mediated inhibition of Ca²⁺ channels and synaptic transmission and could be disrupted byactivation of PKC (Thompson and Gahwiler, 1992; Swartz et al.,1993; Kamiya and Yamamoto, 1997). In the present study, the L-CCG-inducedinitial depression is markedly reduced by PMA, implicating thatit is likely attributable to a block of presynaptic voltage-dependentCa²⁺ channels. These results, coupled with the observation that L-CCGLTD was absent in rab3A-deficient mice in the mossy fiber-CA3synapse (Tzounopoulos et al., 1998), suggesting that L-CCG-inducedsynaptic depression may have two components: the initial depressionthat involves modulation of presynaptic voltage-dependent Ca²⁺ channels and LTD, which may affect a rab3A-dependent vesicleexocytosis. Future experiments to simultaneously record nerveterminal Ca²⁺ currents and postsynaptic responses should be able to clarifythisissue.

Comparison of two forms of LTD in the amygdala

Previously, we have reported that LTD could be reliably induced by LFS in the amygdala (Wang and Gean, 1999). Although L-CCGLTD described here is phenomenologically similar to that of LFSLTD, the underlying cellular mechanisms appear to be quite different.LFS LTD in the amygdala requires activation of the NMDA receptors,depends on postsynaptic Ca²⁺ increases and phosphatase activity (Wang and Gean, 1999), andis independent of the presynaptic phenomenon of paired-pulse facilitation.Therefore, the mechanism of LFS LTD in the amygdala is qualitativelysimilar to those of hippocampal CA1 neurons and several othersynapses in the brain in which a dependence on postsynaptic Ca²⁺ increases is evident (Dudek and Bear, 1992; Mulkey and Malenka,1992).

In contrast, L-CCG LTD is NMDA receptor-independent and is not blocked by loading the postsynaptic cell with BAPTA salt. Itis prevented by BAPTA-AM, suggesting that Ca²⁺ increases in the presynaptic terminals are necessary for itsinduction. Although LFS after induction of L-CCG LTD was unableto depress the responses to the same degree as in naïve synapses,depression consistently did occur. The inability to fully depressthe synapses in these experiments is not surprising, giving thewell documented "metaplastic" effects of previously reduced activitythat would slide the modification threshold, $theta$ _m, to a lower value,making it more difficult to further depress synapses (Abrahamand Bear, 1996; Holland and Wagner, 1998). Thus, saturation ofone form of LTD did not occlude the other. Paired-pulse experimentsrevealed that PPF ratio was increased in L-CCG LTD, suggestingthat the maintenance is likely to occur at presynaptic sites.In these respects, L-CCG LTD in the amygdala closely resemblesthat recently described at hippocampal mossy fiber-CA3 synapsein which LTD requires presynaptic Ca²⁺ increases and is expressed at the presynaptic sites (Tzounopouloset al., 1998; Kobayashi et al., 1999).

Functional implications

As stated in the introductory remarks, drugs that produce LTD in the amygdala may exhibit anxiolytic effect on patients withpost-traumatic stress disorders. The other pathophysiology involvingthe amygdala is kindling phenomenon, which refers to the progressivedevelopment of partial and generalized seizures as a result ofrepeated subconvulsive stimuli (Goddard et al., 1969; McNamara,1986). Kindling has been regarded as a chronic model of humantemporal lobe epilepsy, and the amygdala is one of the most sensitivesites to induce kindling (Loscher et al., 1995). Electrophysiologicalrecordings have demonstrated that kindling is expressed by a sustainedenhancement of excitatory synaptic responses in the amygdala (Geanet al., 1989; Rainnie et al., 1992). In addition, clinical studieshave reported that patients with complex partial seizures of temporallobe origin may experience behavioral disorders, such as depressiveand anxiety-related symptoms (Adamec, 1990). The finding of L-CCGLTD in the amygdala suggests that mGluR II agonists may be potentialanticonvulsants in certain forms of seizure disorders. Indeed,group II mGluR agonists have been shown to attenuate epileptiformbursting observed in kindled rats (Neugebauer et al., 1997; Keeleet al., 1999) and suppressed bicuculline-induced bursts in corticalneurons (Burke and Hablitz, 1995).

  FOOTNOTES

Received May 22, 2000; revised July 31, 2000; accepted Sept. 27, 2000.

This study was supported by National Science Council Grant NSC89-2320-B006-011 and Academic Excellence Program of the Ministryof Education Grant 89-B-FA08-1-4 of Taiwan, Republic ofChina.
Correspondence should be addressed to Dr. Po-Wu Gean, Department of Pharmacology, College of Medicine, National Cheng-KungUniversity, Tainan, Taiwan 701. E-mail: powu{at}mail.ncku.edu.tw.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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