Group 1 and 2 Metabotropic Glutamate Receptors Play Differential Roles in Hippocampal Long-Term Depression and Long-Term Potentiation in Freely Moving Rats

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 (111)

Citing Articles via Google Scholar

Google Scholar

Articles by Manahan-Vaughan, D.

Search for Related Content

PubMed

PubMed Citation

Articles by Manahan-Vaughan, D.

Previous Article  |  Next Article

Volume 17, Number 9, Issue of May 1, 1997 pp. 3303-3311
Copyright ©1997 Society for Neuroscience

Group 1 and 2 Metabotropic Glutamate Receptors Play Differential Roles in Hippocampal Long-Term Depression and Long-Term Potentiation in Freely Moving Rats

Denise Manahan-Vaughan
Federal Institute for Neurobiology, Department of Neurophysiology, D-39008 Magdeburg, Germany

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

This study examined the role of metabotropic glutamate receptors (mGluRs) in hippocampal long-term depression (LTD) in vivo.The group 1 mGluR antagonist (S)4-carboxyphenylglycine (4CPG),group 1/2 antagonist (RS)- $alpha$ -methyl-4-carboxyphenylglycine (MCPG),and group 2 antagonists (RS)- $alpha$ -methylserine-O-phos-phate monophenylester (MSOPPE) and (2S)- $alpha$ -ethylglutamic acid (EGLU) were used.The NMDA receptor antagonist D( $-$ )-2-amino-5-phosphonopentanoicacid (AP5) was used to examine the NMDA receptor contributionto the observed LTD. Adult male Wistar rats underwent implantationof stimulating and recording electrodes into the Schaffer collateralsand CA1 stratum radiatum, respectively. After recovery of 5-7d, the field EPSP was measured from freely moving animals. Drugswere applied either before or after 1 Hz low-frequency train (LFT)or 100 Hz stimulation via a cannula implanted in the lateral cerebralventricle. Nine hundred pulses at 1 Hz produced an LTD that wasmarked and long-lasting. This LTD was completely inhibited bypre-LFT application of AP5. MCPG inhibited LTD from 2 hr post-LFT.4CPG partially impaired LTD. MSOPPE and EGLU completely blockedinduction of LTD, although short-term depression remained intact.MSOPPE did not block long-term potentiation (LTP) induced by 100Hz stimulation, whereas 4CPG produced a significant inhibition.When MSOPPE was present, LTD could not be induced either beforeor after LTP induction, whereas LTD could be induced in an identicalprotocol in vehicle-injected animals.
These results suggest a differential role for mGluRs in NMDA receptor-dependent hippocampal LTD in vivo. Group 1 mGluRs mayplay a role in both LTD and LTP, whereas group 2 mGluRs may becritically involved only in LTD induction.
Key words: metabotropic glutamate receptors; long-term depression; long-term potentiation; in vivo; hippocampus; NMDA receptors

INTRODUCTION

Long-term depression (LTD) is a long-lasting nonpathological decrease in synaptic transmission that has been studied mostlyin cerebellum (Ito, 1989; Linden, 1994) but has also been reportedin the hippocampus (Bear and Malenka, 1994). Hippocampal LTD sharescharacteristics with another form of synaptic plasticity, namelylong-term potentiation (LTP) (Bliss and Lomo, 1973), in that itis dependent on calcium entry through NMDA receptor channels (Dudekand Bear, 1992; Mulkey and Malenka, 1992). It has also been postulatedthat LTD represents an inverse form of LTP (Bear and Malenka,1994; Stevens and Wang, 1994).

It has been reported that in the hippocampus, LTD requires activation of metabotropic glutamate receptors (mGluRs) for robustinduction to take place (Bashir et al., 1993; O'Mara et al., 1995),although others have refuted this claim (Selig et al., 1995).As yet, little information exists as to which mGluR subtypes,if any, may participate in this phenomenon. To date, eight mGluRsubtypes (mGluR 1-8) have been identified (Masu et al., 1991;Abe et al., 1992; Tanabe et al., 1992, 1993; Nakajima et al.,1993; Okamoto et al., 1994; Duvoisin et al., 1995). Group 1 mGluRscomprise mGluRs 1 and 5, which are mainly postsynaptically localizedin hippocampus, are coupled to phospholipase C, and are activatedby 1S 3R-1-aminocyclopentane-1,3- dicarboxylic acid (ACPD). Group2 mGluRs include mGluRs 2 and 3, which are also activated by ACPDbut are coupled to adenylate cyclase and localized mainly presynaptically.mGluRs 4, 6, 7, and 8 also couple to adenylate cyclase but sharean agonist preference for L-2-aminophosphono butyrate (L-AP4)and have therefore been classified as group 3 mGluRs.

Group 1 mGluRs seem to play a critical role in LTP induction in vivo (Manahan-Vaughan and Reymann, 1996; Manahan-Vaughan etal., 1996). Furthermore, activation of group 3 mGluRs can bothdepress basal synaptic transmission and inhibit LTP in the CA1region in vivo (Manahan-Vaughan and Reymann, 1995a). To furthercharacterize the involvement of mGluR subtypes in hippocampalsynaptic plasticity, the present study investigated the contributionof group 1 and 2 mGluRs to induction of LTD and LTP in the hippocampalCA1 region of freely moving rats.

MATERIALS AND METHODS
Surgical preparation. Seven-week-old male Wistar rats were prepared as described previously (Manahan-Vaughan and Reymann,1995a). Briefly, under sodium pentobarbitone anesthesia (Nembutal,40 mg/kg, i.p), animals underwent implantation of a monopolarrecording and a bipolar stimulating electrode (made from 0.1 mmdiameter Teflon-coated stainless steel wire). A hole was drilledfor the recording electrode (1 mm diameter, 2.8 mm posterior tobregma, 1.8 mm lateral to the midline), and a second hole (1 mmdiameter, 3.1 mm posterior to bregma, 3.1 mm lateral to the midline)was drilled for the stimulating electrodes [coordinates basedon Paxinos and Watson (1986)]. The dura was pierced through bothholes, and the recording and stimulating electrodes were loweredinto the CA1 stratum radiatum and the Schaffer collaterals, respectively.Recordings of evoked field potentials via the implanted electrodeswere taken throughout surgery. A cannula was implanted in thelateral cerebral ventricle (0.08 mm posterior to bregma, 1.6 mmlateral to the midline). Once verification of the location ofthe electrodes was complete, the entire assembly was sealed andfixed to the skull with dental acrylic (Paladur, Heraeus KulzerGmbH). The animals were allowed between 5 and 7 d to recover fromsurgery before experiments were conducted. During this periodthey were monitored closely for infection or distress and handledregularly. Twenty-four hours before the commencement of the experiments,animals were placed in the recording chamber with full accessto food and water, to allow familiarization to occur. Throughoutthe experiments, the animals could move freely within the recordingchamber (40 cm × 40 cm × 40 cm), because the implanted electrodeswere connected by a flexible cable and swivel connector to thestimulation unit and amplifier. Aside from the insertion of theconnector cable and injection cannula at the start of the experiment,disturbance of the animals was kept to an absolute minimum. Throughoutthe experiments the electroencephalogram of each animal was monitoredcontinuously.

At the end of the study, brains were removed and histological verification of electrode and cannula localization was carriedout. Brain sections (16 µm) were embedded in paraffin, stainedaccording to the Nissl method using 1% toluidine blue (Bock, 1989),and then examined using a light microscope. Brains in which anincorrect electrode or cannula localization was found were discardedfrom the study.

Measurement of evoked potentials. The field EPSP (fEPSP) slope function was used as a measure of excitatory synaptic transmissionin the CA1 region. To obtain these measurements, an evoked responsewas generated in the stratum radiatum by low-frequency (0.025Hz) stimulation with single biphasic square wave pulses of 0.1msec duration per half wave, generated by a constant current isolationunit. For each time point measured during the experiments, fiverecords of evoked responses were averaged. fEPSP was measuredas the maximal slope through the five steepest points obtainedon the first positive deflection of the potential. By means ofinput/output curve determination the maximum fEPSP was found,and during experiments all potentials used as baseline criteriawere evoked at a stimulus intensity that produced 40% of thismaximum.

LTD was induced by a low-frequency train (LFT) of 1 Hz (900 pulses) and a stimulus intensity that was 60-70% of the maximum(determined by means of the input/output curve). The input specificityof the LTD obtained was verified via implantation of a controlstimulating electrode in the contralateral commissural path. Alternatestimulation via the contralateral and ipsilateral stimulatingelectrodes demonstrated that basal synaptic transmission in theCA1 was evoked by low-frequency stimulation (0.025 Hz) throughthe contralateral electrode, whereas LTD was evoked via the ipsilateralelectrode through which LFT had been given (data not shown). LTPwas induced by a high-frequency tetanus (HFT) of 100 Hz (10 burstsof 10 stimuli, 0.1 msec stimulus duration, 10 sec interburst interval)and a stimulus amplitude that was 20% of the maximum (determinedby means of the input/output curve).

Compounds and drug treatment. (RS)- $alpha$ -methyl-4-carboxyphenylglycine (MCPG), (S)-4-carboxyphenylglycine (4-CPG), (2S)- $alpha$ -ethylglutamicacid (EGLU), D( $-$ )-2-amino-5-phosphonopentanoic acid (AP5), and(RS)- $alpha$ -methylserine-O-phosphate monophenyl ester (MSOPPE) wereobtained from Tocris Cookson (Bristol, UK). For injection, alldrugs were first dissolved in 5 µl sodium hydroxide solution (1mM) and then made up to a 100 µl volume with 0.9% sodium chloride.Throughout the experiments, drugs or vehicle were applied intothe lateral cerebral ventricle via an injection cannula that wasinserted through the surgically implanted outer cannula. Drugor vehicle injection occurred either after measurement of thebaseline for 30 min or 5 min after HFT or LFT. The injection cannulawas inserted before the baseline measurements were taken and leftin place for the duration of the experiment so that an artifactin recordings attributable to its insertion or removal would notbe created.

The drugs were injected in a 5 µl volume over a 6 min period via a Hamilton syringe. In LTD and LTP experiments, an HFT orLFT was applied 30 min after drug injection (or 60-90 min afterthe start of the experiment when injections occurred post-HFT/LFT),with measurements then taken at t = 5, 10, and 15 min and thenat subsequent 15 min intervals up to 4 hr. In some cases, an additionalmeasurement was taken 24 hr post-HFT/LFT. In baseline experiments,the same protocol was followed, except that no HFT or LFT wasgiven. To approximate drug concentrations in vivo and to matchthe reported effective concentrations of the drugs in vitro, drugdose calculations were initially based on the assumption thatthe rat brain volume is ~2 ml. Thus for an estimated brain concentrationof 50 µM AP5, 20 mM (100 nmol) in a 5 µl injection volume wasused. Dose-response relationships were subsequently carried outto determine the effective concentration ranges of the drugs used.

Data analysis. The baseline fEPSP data were obtained by averaging the response to stimulation of the Schaffer collaterals,to obtain five sweeps at 40 sec intervals, every 5 min over aperiod of 30 min. Drug or vehicle injections were then appliedand followed by an additional six recordings in a 30 min period.At this point LFT or HFT was given, and three additional measurementsat 5 min intervals were taken, followed by recordings at 15 minintervals for 4 or 24 hr. The data were then expressed as mean%preinjection baseline fEPSP reading ± SEM. Statistical significancewas estimated using ANOVA with repeated measures, followed bypost hoc Student's t tests. The probability levels interpretedas statistically significant were p < 0.001 (***), p < 0.01 (**),p < 0.05 (*).

RESULTS

Hippocampal LTD in freely moving rats is NMDA receptor dependent
The involvement of NMDA receptors in the induction of LTD was examined using the NMDA receptor antagonist AP5. When an LFT(900 pulses at 1 Hz) was applied via the Schaffer collateral-commissuralpathway to the stratum radiatum of the CA1 region, an LTD of thefEPSP (n = 6) was generated that was still present 24 hr afterLFT. No change in the profile of LTD was seen when a vehicle injectionwas applied 30 min before LFT via a cannula implanted in the lateralcerebral ventricle (n = 19) (Fig. 1). The fEPSP 5 min after LFTwas 64 ± 3% of the preinjection fEPSP baseline values. In sixof the experiments, the profile of the depression was followedfor 24 hr; it was found that the fEPSP was 73 ± 5% of preinjectionvalues. This was not different from the degree of depression seenin noninjected LFT animals but was significantly different fromnon-LFT animals (n = 12; ANOVA: F_(1,25) = 6.7; p < 0.001).
Fig. 1. LTD in the CA1 region in vivo is dependent on activation of both NMDA receptors and mGluRs. A, A low-frequency train (LFT)in the presence of a vehicle injection (n = 19) results in a robustLTD that persists for 24 hr. Previous injection of the NMDA receptorantagonist AP5 (20 mM/5 µl; n = 9) completely inhibits the inductionof LTD, from t = 5 min post-LFT. B, Original analog traces showingevoked responses in the CA1 region at three time points: preinjection,t = 5 min, and t = 4 hr post-LFT, in (1) a vehicle-injected animaland (2) an animal injected with MCPG (200 mM/5 µl). C, MCPG (200mM/5 µl; n = 8) significantly inhibits LTD, from t = 120 min post-LFT,compared with vehicle-injected controls (n = 10). *p < 0.05, **p< 0.01, ***p < 0.001. Line breaks (//) indicate change in timescale.
[View Larger Version of this Image (29K GIF file)]

When AP5 was applied before LFT, in a concentration that had previously been found to block LTP in vivo [20 mM (100 nmol)/5µl] (Manahan-Vaughan et al., 1996), a complete inhibition of LTDoccurred (Fig. 1A) (ANOVA: F_(1,25) = 13.3; p < 0.001). Thus, 5min after LFT, the fEPSP in the AP5 group was 94 ± 4% of preinjectionfEPSP baseline values (n = 9; p < 0.01 compared with controls).This significant inhibition of LTD was maintained throughout theduration of the experiment. Therefore, activation of NMDA receptorsduring LFT is essential for initiation of LTD to occur in vivo.

It was shown previously that the same concentration of AP5 (20 mM/5 µl) has no effect on hippocampal basal synaptic transmissionwhen injected into the lateral cerebral ventricle (Manahan-Vaughanet al., 1996). This finding rules out the possibility that a directeffect of AP5 on basal synaptic transmission explains the inhibitionof LTD obtained by AP5.

LTD in vivo requires activation of mGluRs
To investigate the involvement of mGluRs in LTD, the general mGluR antagonist MCPG was used. This compound, in a concentrationof 200 mM (1 µmol)/5 µl, significantly inhibits LTP in vivo, allowingonly short-term potentiation (STP) to occur (Manahan-Vaughan andReymann, 1995a; Manahan-Vaughan et al., 1996). When the same concentrationof MCPG (200 mM/5 µl; n = 8) was administered 30 min before LFT,a significant inhibition of LTD occurred (ANOVA: F_(1,24) = 20.6;p < 0.001). At first, however, a depression appeared that wasnot statistically different from controls (58 ± 7% of preinjectionfEPSP baseline values at 5 min post-LFT in the MCPG-injected animals;61 ± 6% in controls; n = 12) (Fig. 1B,C), but by 120 min post-LFTthe fEPSP values of the MCPG-injected group had recovered significantly,being 92 ± 8% of preinjection values compared with 76 ± 3% incontrols (p < 0.05). By 135 min post-LFT, the fEPSP values inthe MCPG-injected animals had returned to pre-LFT levels (Fig.1C). It was determined previously that this concentration of MCPG(200 mM/5 µl) has no effect on basal synaptic transmission inthe CA1 region when injected into the lateral cerebral ventricle(Manahan-Vaughan and Reymann, 1995b).

Group 1 mGluRs play a role in LTD in vivo
To attempt to dissect the mGluR-mediated component of LTD into the receptor subtypes involved, the group 1 mGluR antagonist4CPG was used. 4CPG has an IC₅₀ value of 4 × 10⁵ M at mGluR 1 and an EC₅₀ value of 5 × 10⁴ M at mGluR 2 and is inactive at mGluR 4 (Hayashi et al., 1994;tested in chinese hamster ovary cells). In addition, it has beenreported that 4CPG inhibits ACPD-stimulated phosphoinositide hydrolysisin cerebrocortical slices (Eaton et al., 1993).

When 4CPG in a concentration of 2 mM (n = 4), 4 mM (n = 4), or 10 mM/5 µl (n = 4) was applied 30 min before LFT, no significanteffect on LTD was seen (Fig. 2C). When 4CPG (n = 7) was administered30 min before LFT, however, in a concentration that was foundpreviously to be effective in blocking LTP in vivo (20 mM (100nmol)/5 µl), a significant impairment of LTD expression was seencompared with controls (n = 12; ANOVA: F_(1,24) = 21.9; p < 0.001).As was the case with MCPG, application of 4CPG did not affectshort-term depression (Fig. 2A,B). By 120 min post-LFT, however,a recovery of fEPSP values toward preinjection levels had occurred,and a significant difference was evident from this time pointonward compared with LFT controls (88 ± 6% of preinjection fEPSPbaseline values compared with 74 ± 3% in controls; p < 0.05) (Fig.2A,B). A complete recovery back to preinjection fEPSP baselinevalues did not take place in the 4CPG group; rather, the fEPSPvalues showed a significant difference when compared with controlnon-LFT animals (n = 8; ANOVA: F_(1,24) = 3.2; p < 0.001) (Fig.2A,B). Thus, 4CPG seemed to produce a partial but significantblock of LTD.
Fig. 2. LTD in the CA1 region in vivo is modulated by group 1 mGluRs. A, The group 1 mGluR antagonist 4CPG (20 mM/5 µl; n = 7) partiallyimpairs LTD when compared with vehicle-injected controls (n =12), from t = 120 min post-LFT. This effect was significantlydifferent from baseline values. B, Original analog traces showingevoked responses in the CA1 region at three time points: preinjection,t = 5 min, and t = 4 hr post-LFT, in an animal injected with 4CPG(20 mM/5 µl). C, Dose-response curve for the antagonist effectof 4CPG (2-40 mM/5 µl) on LTD in the CA1 region. The values representthe magnitude of LTD observed at 4 hr post-LFT. D, Applicationof 4CPG (20 mM/5 µl; n = 5) 5 min after LFT results in a significantinhibition of LTD, from t = 135 min post-HFT compared with vehicle-injectedcontrols (n = 5). *p < 0.05. Line breaks (//) indicate changein time scale.
[View Larger Version of this Image (31K GIF file)]

When basal synaptic transmission was monitored for 4 hr in the presence of 4CPG (20 mM/5 µl), no effect on synaptic transmissionwas observed (n = 4). In addition, when the higher concentrationof 40 mM 4CPG/5 µl was applied 30 min before LFT, no further inhibitionof LTD was seen compared with the 20 mM/5 µl concentration (Fig.2C).

To examine whether 4CPG modulates LTD by influencing its initiation, experiments were carried out in which the compound wasapplied 5 min after the termination of LFT (n = 5). In this casean impairment of LTD was obtained similar to that seen when 4CPGwas applied before LFT (ANOVA: F_(1,25) = 15.2; p < 0.001). Thus,no difference in the degree of depression was seen initially whencompared with controls (n = 6) (Fig. 2D). From 135 min post-LFT,however, the magnitude of depression of fEPSP in the 4CPG grouphad reduced (85 ± 2% of preinjection values compared with 67 ±6% in controls; p < 0.05) (Fig. 2D), and a significant differenceoccurred from this time point onward until the end of the experiment.A complete recovery back to preinjection fEPSP baseline valuesdid not occur in the 4CPG group; rather, the values showed a significantdifference when compared with control non-LFT animals (n = 8;ANOVA: p < 0.001).

These data indicate that group 1 mGluRs do not modulate LTD through an interaction with NMDA receptors during LTD initiation,for example, but rather seem to modulate the maintenance phaseof LTD.

Group 1 mGluR activation is necessary for persistent LTP in vivo
When a vehicle injection (n = 6) was applied 30 min before an HFT, LTP was induced that persisted for >24 hr (Fig. 3A). Thispotentiation was statistically significant from control (nontetanized),from t = 5 min post-HFT onward. When 4CPG (n = 5) in a concentrationof 20 mM (100 nmol)/5 µl was administered 30 min before HFT, asignificant difference between 4CPG- and vehicle-treated animalswas seen (ANOVA: F_(1,25) = 24.2; p < 0.001). Thus, although STPremained intact, by 60 min post-HFT, fEPSP values had declinedto 126 ± 10% in the 4CPG group compared with 155 ± 6% in controls.At 24 hr post-LFT, the control group was still potentiated, whereasin the 4CPG group fEPSP values returned to pre-HFT baseline levelsby 90 min. Therefore, a concentration of 4CPG that significantlyinhibits LTD also successfully inhibits LTP. This finding supportsa role for group 1 mGluRs in bidirectional modulation of synapticplasticity.
Fig. 3. LTP in the CA1 region in vivo is modulated by group 1 mGluRs. A, 4CPG (20 mM/5 µl; n = 5) significantly inhibits LTP, fromt = 60 min after a high-frequency tetanus (HFT) compared withvehicle-injected controls (n = 6). B, Application of 4CPG (20mM/5 µl; n = 5) 5 min after HFT results in a significant inhibitionof LTP, from t = 45 min post-HFT compared with vehicle-injectedcontrols (n = 5). *p < 0.05, **p < 0.01, ***p < 0.001. Line breaks(//) indicate change in time scale.
[View Larger Version of this Image (32K GIF file)]

To investigate whether 4CPG inhibits the initiation or maintenance phases of LTP, the compound was applied 5 min after LTP.It was found that an inhibition of LTP occurred (ANOVA: F_(1,25)= 34.3; p < 0.001) similar to that seen when the drug was appliedbefore HFT. At 5 min post-HFT, the amplitude of LTP was 151 ±4% of preinjection fEPSP baseline levels (n = 5) compared with161 ± 5% in controls (n = 5). By 45 min post-HFT, a significantreduction in the degree of potentiation was seen in the 4CPG groupwhen compared with controls (p < 0.05), and by 120 min post-HFT,fEPSP values had returned to preinjection levels (Fig. 3B). Thus,group 1 mGluRs seem to contribute to the maintenance rather thanthe initiation of LTP.

Group 2 mGluR activation is required for persistent LTD in vivo
MSOPPE is a selective group 2 mGluR antagonist (Jane et al., 1996a; Thomas et al.,1996a) that shows a preference for group2 mGluRs over group 3 mGluRs. When MSOPPE in a concentration of4 mM (n = 4), 10 mM (n = 4), or 20 mM/5 µl (n = 4) was applied30 min before LFT, no effect on LTD was seen (Fig. 4C). When theconcentration was raised to 40 mM (200 nmol)/5 µl, a significantinhibition of LTD was observed (ANOVA: F_(1,24) = 43.8; p < 0.001)(Fig. 4A,B). Although the degree of LTD immediately after LFTwas not significantly different in drug (n = 12) and control (n= 12) groups, by 90 min post-LFT a significant inhibition of LTDhad occurred in the MSOPPE group compared with controls (94 ±6% compared with 75 ± 4% in controls; p < 0.05) (Fig. 4A). Inthe MSOPPE group the evoked potentials returned to pre-LFT valuesby 165 min post-LFT, whereas in the control group values werestill depressed at 4 hr post-LFT.
Fig. 4. LTD in the CA1 region in vivo critically involves group 2 mGluRs. A, The group 2 mGluR antagonist MSOPPE (40 mM/5 µl; n =12) completely blocks LTD, from t = 90 min post-LFT when comparedwith vehicle-injected controls (n = 12). B, Original analog tracesshowing evoked responses in the CA1 region at three time points:preinjection, t = 5 min, and t = 4 hr post-LFT, in an animal injectedwith MSOPPE (40 mM/5 µl). C, Dose-response curve for the antagonisteffect of MSOPPE (4-80 mM/5 µl) on LTD in the CA1 region. Thevalues represent the magnitude of LTD observed at 4 hr post-LFT.D, The group 2 mGluR antagonist EGLU (n = 6) completely blocksLTD, from t = 75 min post-LFT when compared with vehicle-injectedcontrols (n = 11). *p < 0.05, **p < 0.01, ***p < 0.001. Line breaks(//) indicate change in time scale.
[View Larger Version of this Image (32K GIF file)]

When basal synaptic transmission was monitored for 4 hr in the presence of MSOPPE (40 mM/5 µl; n = 8), no effect on synaptictransmission was seen compared with controls (n = 8). When thehigher concentrations of 60 mM (n = 4) and 80 mM MSOPPE/5 µl (n= 4) were applied 30 min before LFT, no improvement in the degreeof inhibition of LTD obtained was seen compared with the 40 mM/5µl dose (Fig. 4C).

EGLU is a highly selective antagonist for group 2 mGluRs that exhibits a potency at group 2 mGluRs similar to that of MSOPPEbut has no antagonist action at group 3 mGluRs (Jane et al., 1996b).Thus, EGLU was used to examine whether the blockade of LTD seenwith MSOPPE can be explained via antagonism of group 2 mGluRs.When EGLU was applied in concentrations of either 5 or 10 mM/5µl before LFT (n = 4 and n = 5, respectively), no inhibition ofLTD was observed. A significant inhibition of LTD, however, wasobtained when EGLU in a concentration of 20 mM (100 nmol)/5 µlwas applied before LFT (Fig. 5D) (ANOVA: F_(1,25) = 23.8; p < 0.001).
Fig. 5. Group 1 and 2 mGluRs contribute to maintenance rather than initiation of LTD. A, Application of MSOPPE (40 mM/5 µl; n = 5)5 min after LFT results in a significant inhibition of LTD, fromt = 105 min post-LFT compared with vehicle-injected controls (n= 5). B, Application of a subthreshold concentration of MSOPPE(20 mM/5 µl) in conjunction with 4CPG (20 mM/5 µl; n = 5) 5 minpost-LFT results in a complete block of the 4CPG-resistant fractionof LTD, from t = 105 min compared with vehicle-injected controls(n = 5).
[View Larger Version of this Image (33K GIF file)]

Although the magnitude of LTD immediately after LFT was not significantly different in drug (n = 6) and control (n = 11) groups,by 75 min post-LFT a significant inhibition of LTD had occurredin the EGLU group compared with controls (93 ± 7% compared with75 ± 3% in controls; p < 0.05) (Fig. 4D). In the EGLU group theevoked potentials returned to preinjection values by 90 min post-LFT,whereas in the control group fEPSP values were still depressedat 24 hr post-LFT. When EGLU (20 mM/5 µl; n = 6) was administeredand basal synaptic transmission was monitored for 4 hr subsequently,no effect on synaptic transmission was seen compared with controls(n = 8). In addition, no further improvement in the degree ofinhibition of LTD was seen when a 40 mM concentration of EGLUwas applied before LFT (n = 6).

Both group 1 and 2 mGluRs contribute to LTD maintenance in vivo
To examine whether MSOPPE inhibits LTD through prevention of initiation rather than maintenance of LTD, experiments were carriedout in which the compound (40 mM/5µl) was applied 5 min afterthe termination of LFT. In this case, a profile of response wasobtained similar to that seen when MSOPPE was applied before LFT(Fig. 5A) (ANOVA: F_(1,25) = 13.2; p < 0.001). Thus, although short-termdepression was unaffected, MSOPPE (n = 5) produced an inhibitionof LTD that became evident from 105 min post-LFT (100 ± 5% ofpreinjection fEPSP baseline values compared with 76 ± 5% in vehicle-injectedcontrols; n = 5; p < 0.05).

In addition, when EGLU (20 mM/5 µl; n = 6) was applied 5 min after LFT, a significant inhibition of LTD occurred (ANOVA: F_(1,25)= 11.7; p < 0.001), and a profile of LTD inhibition was seen similarto that obtained when EGLU was applied before LFT. The magnitudeof LTD 5 min after LFT was not significantly different in drug(n = 6) and control (n = 6) groups (54 ± 9% of preinjection valuescompared with 57 ± 6% in controls). By 105 min post-LFT a significantinhibition of LTD had occurred in the EGLU group compared withcontrols (93 ± 7% compared with 73 ± 4% in controls; p < 0.05).In the EGLU group the evoked potentials returned to preinjectionvalues by 120 min post-LFT, whereas in the control group valueswere still depressed at 24 hr post-LFT.

Taken together, these data further support the possibility that group 2 mGluRs are critically involved in the maintenancephase of LTD.

As a partial inhibition of LTD was obtained with 4CPG, we investigated whether application of MSOPPE could inhibit the 4CPG-resistantfraction of LTD. MSOPPE dose-dependently inhibits LTD, with amaximal effect at a concentration of 40 mM/5 µl (Fig. 4C). A concentrationof MSOPPE that was subthreshold for significant inhibition ofLTD (20 mM (100 nmol)/5 µl) was used therefore in conjunctionwith 4CPG (20 mM/5 µl). When LFT was applied in the presence ofthese compounds, a significant inhibition of LTD occurred (ANOVA:F_(1,25) = 18.6; p < 0.001). In brief, when MSOPPE and 4CPG wereapplied together 5 min post-LFT, initially no difference betweenthe drug (n = 5) and control groups (n = 5) was seen (Fig. 5B).By 105 min post-LFT, however, a significant inhibition of LTDdeveloped. At this time point the fEPSP was 89 ± 4% of preinjectionfEPSP baseline values in the MSOPPE/4CPG group and 72 ± 4% incontrols. By 135 min post-LFT, fEPSP values had returned to preinjectionfEPSP baseline levels in the drug group (Fig. 5B). The effectof MSOPPE/4CPG on LTD was significantly different from the effectof MSOPPE (20 mM/5 µl; n = 4) when injected alone (ANOVA: F_(1,25)= 7.0; p < 0.001) and was significantly different compared withLTD evoked from animals in which 4CPG (20 mM/5 µl; n = 5) wasapplied 5 min after LFT (ANOVA: F_(1,25) = 15.1; p < 0.001). Thesedata indicate that activation of both group 1 and group 2 mGluRscontributes to LTD maintenance.

Group 2 mGluR activation is not necessary for LTP in vivo
When a vehicle injection (n = 6) was applied 30 min before HFT, LTP was induced that persisted for >24 hr (Fig. 6A). Thispotentiation was statistically significant from control (nontetanized),from t = 5 min post-HFT onward. When MSOPPE (n = 7) in a concentrationof 40 mM (200 nmol)/5 µl was administered 30 min before an HFTwas applied, LTP was induced that was not statistically significantfrom the vehicle-injected LTP group (Fig. 6A,B). Thus, a concentrationof MSOPPE that inhibits the induction of LTD has no effect onLTP.
Fig. 6. LTP induction does not depend on activation of group 2 mGluRs. A, The group 2 mGluR antagonist MSOPPE (n = 7) does not inhibitLTP in the CA1 region when compared with vehicle-injected controls(n = 6). B, Original analog traces showing evoked responses inthe CA1 region at three time points: preinjection, t = 5 min,and t = 4 hr post-HFT, in an animal injected with MSOPPE (40 mM/5µl). Line breaks (//) indicate change in time scale.
[View Larger Version of this Image (22K GIF file)]

Group 2 mGluRs may play a differential role in hippocampal synaptic plasticity in vivo
To further investigate whether group 2 mGluRs may play a critical role in LTD as opposed to LTP, an experiment was carriedout in which LFT was applied 1 hr after induction of LTP. Whena vehicle injection (n = 5) was applied into the lateral cerebralventricle and followed 30 min later by HFT, LTP occurred (Fig.7A) that was not statistically different from the previous controlgroup (Fig. 6A). When LFT was given 1 hr after HFT, fEPSP valuesreturned to pre-HFT baseline levels. When MSOPPE [40 mM (200 nmol)/5µl; n = 5] was applied before HFT, a potentiation occurred similarto that seen in the control group. When LFT was given 1 hr later,no significant reduction in the magnitude of LTP was elicited.Thus, although LTD could follow LTP in the control animals, itwas not possible to evoke LTD after LTP in the MSOPPE group (ANOVA:F_(1,30) = 9.7; p < 0.001).
Fig. 7. LTD but not LTP depends on activation of group 2 mGluRs. A, HFT in the presence of a vehicle injection (n = 5) results ina marked potentiation of fEPSP. LFT applied 1 hr after HFT causesevoked potentials to return to baseline values. MSOPPE (n = 5)applied before an identical protocol results in an LTP that cannotbe reversed by application of LFT. B, Original analog traces showingevoked responses in the CA1 region at three time points: preinjection,t = 60 min, and t = 4 hr post-tetanus, in (1) an animal injectedwith MSOPPE (40 mM/5 µl) in which HFT is followed 1 hr later byLFT, and (2) an animal injected with MSOPPE (40 mM/5 µl) in whichLFT is followed 1.5 hr later by HFT. C, Vehicle injection (n =6) before LFT results in a marked depression of fEPSP. HFT applied1.5 hr after LFT results in a reversal of depression to approximatelypre-LFT values. MSOPPE (n = 6) applied before LFT results in adepression of LFT that recovers gradually. Application of HFT1.5 hr after LFT produces a marked potentiation of fEPSP to LTPlevels. Line breaks (//) indicate change in time scale.
[View Larger Version of this Image (36K GIF file)]

To examine whether LTD could be followed by LTP, an experiment was performed in which LFT was applied before HFT. In the controlgroup (n = 6), vehicle injection was followed 30 min later byLFT. A marked LTD was immediately noted, which was still presentafter 90 min. When HFT was then applied after stabilization ofLTD (90 min post-LFT), a complete reversal of LTD to pre-LFT valueswas obtained (Fig. 7B). When MSOPPE (n = 6) was applied and followed30 min later by LFT, an initial depression of synaptic transmissionoccurred, which by 90 min had recovered to pre-LFT values. WhenHFT was then applied, a marked potentiation of fEPSP occurred(Fig. 7B), which was similar in profile to the "HFT only" group(Fig. 6A,B). This potentiation was still present after 24 hr.Thus, although antagonism of group 2 mGluRs impairs LTD in vivo,LTP is not affected (ANOVA: F_(1,32) = 48.3; p < 0.001). Theseobservations support a differential role for group 2 mGluRs indistinct forms of hippocampal synaptic plasticity.

DISCUSSION

Initiation of LTD in the CA1 region in vivo is NMDA receptor dependent
It has been shown previously that administration of 900 pulses at 1 Hz will reliably produce robust input-specific LTD invitro (Dudek and Bear, 1992; Mulkey and Malenka, 1992) and inanesthetized rats in vivo (Heynen et al., 1996). In this study,a similar stimulation protocol produced a persistent and markedLTD in freely moving rats. When the NMDA receptor antagonist AP5was applied before LFT, however, a complete block of LTD occurred.This finding is in agreement with the reports of others that blockadeof the NMDA receptor prevents homosynaptic LTD in the CA1 regionin vitro (Dudek and Bear, 1992; Mulkey and Malenka, 1992) andsupports the possibility that initiation of LTD in the hippocampalCA1 region in vivo is dependent on activation of NMDA receptors.

Induction of robust LTD in vivo is mGluR dependent
It has been reported that MCPG blocks LTD in the CA1 region (Bashir et al., 1993; Bolshakov and Siegelbaum, 1994), dentategyrus (O'Mara et al., 1995), visual cortex (Haruta et al., 1994),and cerebellum (Hartell, 1994) of the rat in vitro, although othersclaim that MCPG has no effect on hippocampal LTD in vitro (Seliget al., 1995). MCPG remains a controversial compound however,because although some researchers have found it to be a competitiveantagonist of both PLC and cAMP-coupled mGluRs (Eaton et al.,1993; Jane et al., 1993; Watkins and Collingridge, 1994), othershave found no effect of this compound at these receptors (Chinestraet al., 1993; Saugstad et al., 1994). In previous work it wasfound that MCPG consistently blocks hippocampal LTP in freelymoving rats (Manahan-Vaughan and Reymann, 1995a,b) and antagonizesthe action of group 1 mGluRs (Manahan-Vaughan and Reymann, 1996;Manahan-Vaughan et al., 1996). Thus, it may be the case that theaction of this compound may be strongly influenced by the conditionsunder which its efficacy is tested.

Other evidence to support the involvement of mGluRs in LTD has been provided using the group 1 and 2 mGluR agonist ACPD, whichinduces LTD in the cerebellum (Daniel et al., 1992) and dentategyrus in vitro (O'Mara et al., 1995). Furthermore, in the presentstudy a marked blockade of hippocampal LTD in vivo in the presenceof MCPG was found. The effect became evident >1 hr after LFT wasgiven, suggesting that, as is the case with LTP in vivo (Manahan-Vaughanand Reymann, 1995b; Manahan-Vaughan et al., 1996), mGluRs arecritically involved in the induction of stable LTD downstreamof the NMDA-dependent "early" component. Thus, the early phaseof LTD, which depends on NMDA receptor activation, was present,but in the absence of mGluR activation LTD did not persist longerthan ~1 hr. This finding is in agreement with previous reportsfrom in vitro studies, which suggest that mGluRs are cruciallyinvolved in the maintenance of robust hippocampal LTD.

Group 1 mGluRs contribute to the stable induction of both LTD and LTP in vivo
To identify the subtype of mGluR that may be responsible for LTD induction, an investigation of the effect of the group 1mGluR antagonist 4CPG (Birse et al., 1993; Hayashi et al., 1994;Watkins and Collingridge, 1994) on LTD was conducted. This drughas an IC₅₀ value of 4 × 10⁵ M at mGluR 1 and an EC₅₀ value of 5 × 10⁴ M at mGluR 2 and is inactive at mGluR 4 (Hayashi et al., 1994;tested in chinese hamster ovary cells). In addition it has beenreported that 4CPG competitively inhibits ACPD-stimulated phosphoinositidehydrolysis in cerebrocortical slices (Birse et al., 1993; Eatonet al., 1993). Although its selective potency at mGluR 1 has beenconfirmed by others, it has been claimed that this compound isfar less potent at mGluR 5 compared with mGluR 1 (Brabet et al.,1995). In the present study, it was found that although an impairmentin the magnitude of LTD occurred in the presence of 4CPG, theremaining depression was still significantly different from controlvalues, implying that only a partial inhibition of LTD took place.Others have reported that blockade of mGluR 1 in cultured Purkinjecells using antibodies (Shigemoto et al., 1994) and "knockout"of mGluR 1 in mouse cerebellum (Aiba et al., 1994a) result inan impairment of LTD. The data presented in this study also suggesta role for group 1 mGluRs in hippocampal LTD in vivo. The observation,however, that the partial blockade of LTD could not be improvedon application of higher concentrations of 4CPG indicates thatgroup 1 mGluRs are capable of modulating the degree of LTD butare not critical for hippocampal LTD induction.

The observation that 4CPG inhibits LTP in exactly the same concentration that impairs LTD is an interesting finding. Togetherwith the observation that the compound is still effective whenapplied after induction of LTP or LTD, these data suggest thatgroup 1 mGluRs are involved in the maintenance rather than theinitiation of these forms of synaptic plasticity. Furthermore,these data indicate that group 1 mGluRs are capable of bidirectionalmodulation of synaptic plasticity. One possibility is that differentialdegrees of activation of group 1 mGluRs can determine which formof synaptic plasticity is expressed. This may occur perhaps throughgroup 1 mGluR-mediated modulation of the level of activation ofprotein kinase C (Stanton, 1995). This bidirectional capabilityof group 1 GluRs could have an important significance in termsof the regulation of synaptic plasticity.

Group 2 mGluRs are critically involved in the stable induction of LTD but not LTP
The involvement of group 2 mGluRs in LTD and LTP was investigated by means of the selective group 2 mGluR antagonists MSOPPE(Jane et al., 1996a; Thomas et al., 1996a) and EGLU (Jane et al.,1996b; Thomas et al., 1996b). Both MSOPPE and EGLU exhibit a selectivepreference for group 2 mGluRs. Their K_D values for antagonismof ACPD-induced depression of dorsal root-evoked monosynapticexcitation have been determined as 73 and 63 µM, respectively,at presynaptic (group 2) mGluRs. The K_D values of MSOPPE for antagonismof L-AP4-induced depression of dorsal root-evoked monosynapticexcitation is 221 µM at presynaptic (group 3) mGluRs (Jane etal., 1996a), whereas EGLU has no detectable actions at group 3mGluRs (Jane et al., 1996b; Thomas et al., 1996b). One cannotcompletely rule out, however, the possibility that group 3 mGluRsmay be influenced by the concentration of MSOPPE used in the presentstudy. In addition, the characterization of EGLU antagonism ofpresynaptic mGluRs was conducted using rat spinal cord preparations,in which the complement of group 3 mGluRs may not be identicalto that of hippocampal group 3 mGluRs. Thus it may be the casethat antagonism of group 3 mGluRs may contribute to the inhibitionof LTD seen with MSOPPE and EGLU.

In the present study, a dose-dependent inhibition of LTD was obtained with MSOPPE. A similar block of LTD was obtained withEGLU, which is reported to be a more selective antagonist of group2 mGluRs than MSOPPE (Jane et al., 1996b; Thomas et al., 1996b).Both MSOPPE and EGLU also effectively blocked the induction ofLTD when applied 5 min post-HFT, which suggests that activationof group 2 mGluRs contributes to the maintenance or stabilizationof LTD. Interestingly, neither MSOPPE nor EGLU had an effect onthe induction or expression of LTP in vivo. The observation thatboth MSOPPE and EGLU can fully inhibit LTD but have no effecton LTP implies that activation of group 2 mGluRs may be criticallyrequired for LTD but unnecessary for LTP.

Group 2 mGluRs may play an exclusive role in LTD
The observation that MSOPPE inhibits LTD but not LTP in vivo provokes the interesting implication that the involvement ofmGluRs in these two forms of synaptic plasticity is not simplydependent on the relative levels of activation of these receptors.This possibility is reinforced by the finding that it is possiblein vivo to induce LTP and LTD in series, as has been reportedin vitro (Mulkey and Malenka, 1992; Dudek and Bear, 1993), butit is not possible to follow LTP with LTD, or to follow LTD withLTP, when MSOPPE is present. This suggests that distinct mGluRsubtypes may be critically involved in one form of synaptic plasticityas opposed to another. With regard to LTP, this question was addressedpreviously, and it was found that group 1 mGluRs seem to be thecritical mGluR class involved, whereas group 3 mGluRs may playmerely a modulatory role in this phenomenon (Manahan-Vaughan andReymann, 1995a, 1996; Manahan-Vaughan et al., 1996). The requirementof group 1 mGluRs for LTP has also been demonstrated in mGluR1knockout mice (Aiba et al., 1994b). Furthermore, the observationsof the present study offer strong evidence to support the theorythat group 2 mGluRs are critically involved in the maintenanceof LTD but not LTP.

This finding, combined with the observation that group 1 mGluRs contribute to LTD maintenance, implies that both a presynaptic(group 2 mGluR) and a postsynaptic (group 1 mGluR) locus for LTDexpression exists. It has been shown that induction of hippocampalLTD requires Ca²⁺ release from distinct pre- and postsynaptic stores (Reyes andStanton, 1996). Perhaps group 1 mGluRs contribute to LTD by stimulatingrelease of Ca²⁺ from postsynaptic inositol trisphosphate-gated intracellularCa²⁺ stores, whereas group 2 mGluRs influence release of Ca²⁺ from the presynaptic ryanodine-sensitive Ca²⁺ stores identified by Reyes and Stanton (1996).

Conclusion
The results of this study comprise a number of interesting observations about LTD in vivo. Namely, (1) it is possible to obtaina robust LTD in the CA1 region of freely moving rats; (2) thisLTD is dependent on activation of NMDA receptors; (3) in addition,activation of mGluRs is required for a persistent form of LTDto occur; (4) although group 1 mGluRs seem to modulate the degreeof LTD, group 2 mGluR activation may be a critical factor forLTD maintenance; and (5) it seems that group 2 mGluRs are involvedin LTD but not LTP induction, whereas group 1 mGluRs are involvedin the induction or modulation of both phenomena.

Taken together, the observations of this study demonstrate an intriguing involvement of mGluRs in synaptic plasticity andsuggest that bidirectional modulation of hippocampal synaptictransmission by distinct mGluR subtypes can occur. Furthermore,it may be the case that certain mGluR subtypes modulate distinctforms of plasticity only. Thus, mGluR involvement in LTD and LTPmay correspond to an important system by which the efficacy ofsynaptic transmission is regulated within the hippocampus.

FOOTNOTES

Received Dec. 20, 1996; revised Feb. 7, 1997; accepted Feb. 13, 1997.

I am very grateful to Ms. Silvia Vieweg for expert technical assistance and to Professor Klaus Reymann and Dr. Ritchie Brownfor valuable discussion of this manuscript.

Correspondence should be addressed to Dr. Denise Manahan-Vaughan, Federal Institute for Neurobiology, Department of Neurophysiology,Brenneckestrasse 6, P.O. Box 1860, D-39008 Magdeburg, Germany.

REFERENCES

Abe T, Sugihara H, Nawa H, Shigemoto R, Mizuno N, Nakanishi S (1992) Molecular characterization of a novel metabotropic glutamate receptor mGluR 5 coupled to inositol phosphate/Ca²⁺ signal transduction. J Biol Chem 267:13361-13368[Abstract/Free Full Text].
Aiba A, Kano M, Chen C, Stanton ME, Fox GD, Herrup K, Zwingman TA, Tonegawa S (1994a) Deficient cerebellar long-term depression and impaired motor learning in mGluR1 mutant mice. Cell 79:377-388[Web of Science][Medline].
Aiba A, Chen C, Herrup K, Rosenmund C, Stevens CF, Tonegawa S (1994b) Reduced hippocampal long-term potentiation and context-specific deficit in associative learning in mGluR 1 mutant mice. Cell 79:365-375[Web of Science][Medline].
Bashir ZI, Jane DE, Sunter DC, Watkins JC, Collingridge GL (1993) Metabotropic glutamate receptors contribute to the induction of long-term depression in the CA1 region of the hippocampus. Eur J Pharmacol 239:265-266[Web of Science][Medline].
Bear MF, Malenka RC (1994) Synaptic plasticity: LTP and LTD. Curr Opin Neurobiol 4:389-399[Medline].
Birse EF, Eaton SA, Jane DE, St J, Jones PL, Porter RHP, Pook PC-K, Sunter DC, Udvarhelyi PM, Wharton B, Roberts PJ, Salt TE, Watkins JC (1993) Phenylglycine derivatives as new pharmacological tools for investigating the role of metabotropic glutamate receptors in the central nervous system. Neuroscience 52:481-488[Web of Science][Medline].
Bliss TVP, Lomo T (1973) Long-lasting potentiation of synaptic transmission in the dentate area of the unanesthetized rabbit following stimulation of the perforant path. J Physiol (Lond) 232:357-373[Abstract/Free Full Text].
Bock P (1989) In: Romeis Mikroskopische Technik. pp 575-576. München: Urban and Schwarzenberg.
Bolshakov VY, Siegelbaum SA (1994) Post-synaptic induction and presynaptic expression of hippocampal long-term depression. Science 264:1148-1152[Abstract/Free Full Text].
Brabet I, Mary S, Bockaert J, Pin JP (1995) Phenylglycine derivatives discriminate between mGluR1- and mGluR 5-mediated responses. Neuropharmacology 34:895-903[Web of Science][Medline].
Chinestra P, Aniksztejn L, Diabira D, Ben Ari Y (1993) (RS)- $alpha$ -methyl-4-carboxyphenylglycine neither prevents induction of LTP nor antagonises metabotropic glutamate receptors in CA1 hippocampal neurons. J Neurophysiol 70:2684-2689[Abstract/Free Full Text].
Daniel H, Hemart N, Jaillard D, Crepel F (1992) Co-activation of metabotropic glutamate receptors and of voltage-gated calcium channels induces long-term depression in cerebellar Purkinje cells in vitro. Exp Brain Res 90:327-331[Web of Science][Medline].
Dudek SM, Bear MF (1992) Homosynaptic long-term depression in area CA1 of hippocampus and the effects of NMDA receptor blockade. Proc Natl Acad Sci USA 89:4363-4367[Abstract/Free Full Text].
Dudek SM, Bear MF (1993) Bidirectional long-term modification of synaptic effectiveness in the adult and immature hippocampus. J Neurosci 13:2910-2918[Abstract].
Duvoisin RM, Zhang C, Ramonell K (1995) A novel metabotropic glutamate receptor expressed in the retina and olfactory bulb. J Neurosci 15:3075-3083[Abstract].
Eaton SA, Jane DE, St J, Jones PL, Porter RHP, Pook PC-K, Sunter DC, Udvarhelyi PM, Roberts PJ, Salt TE, Watkins JC (1993) Competitive antagonism at metabotropic glutamate receptors (S)-4-carboxyphenylglycine (CPG) and (RS) $alpha$ -methyl-4- carboxyphenylglycine (MCPG). Eur J Pharmacol Mol Pharmacol 244:195-197[Web of Science][Medline].
Hartell NA (1994) Induction of cerebellar long-term depression requires activation of glutamate metabotropic receptors. NeuroReport 5:913-916[Web of Science][Medline].
Haruta H, Kamishita T, Hicks TP, Takahashi MP, Tsumoto T (1994) Induction of LTD but not LTP through metabotropic glutamate receptors in visual cortex. NeuroReport 5:1829-1832[Web of Science][Medline].
Hayashi Y, Sekiyama N, Nakanishi S, Jane DE, Sunter DC, Birse EB, Udvarhelyi PM, Watkins JC (1994) Analysis of agonist and antagonist activities of phenylglycine derivatives for different cloned metabotropic glutamate receptor subtypes. J Neurosci 14:3370-3377[Abstract].
Heynen AJ, Abraham WJ, Bear MF (1996) Bidirectional modification of CA1 synapses in the adult hippocampus in vivo. Nature 381:163-166[Medline].
Ito M (1989) Long-term depression. Annu Rev Neurosci 12:85-102[Web of Science][Medline].
Jane DE, St J Jones PL, Pook P C-K, Salt TE, Sunter DC, Watkins JC (1993) Stereospecific antagonism by (+)- $alpha$ -methyl-4-carboxyphenylglycine (MCPG) of (1S, 3R)-ACPD-induced effects in neonatal rat motoneurones and rat thalamic neurones. Neuropharmacology 32:725-727[Web of Science][Medline].
Jane DE, Pittaway D, Sunter DC, Thomas NK, Tse H-K (1996a) Phosphono substituted amino acids as selective metabotropic glutamate receptor antagonists. Phosphorous Sulfur Silicon 109-110:313-316.
Jane DE, Thomas NK, Tse H-W, Watkins JC (1996b) Potent antagonists at the L-AP4 and (1S, 3S)-ACPD-sensitive presynaptic metabotropic glutamate receptors in the neonatal rat spinal cord. Neuropharmacology 35:1029-1035[Web of Science][Medline].
Linden DJ (1994) Long-term synaptic depression in the mammalian brain. Neuron 12:457-472[Web of Science][Medline].
Manahan-Vaughan D, Reymann KG (1995a) Regional and developmental profile of modulation of hippocampal synaptic transmission and LTP by AP4-sensitive mGluRs in vivo. Neuropharmacology 34:991-1001[Web of Science][Medline].
Manahan-Vaughan D, Reymann KG (1995b) 1S, 3R- ACPD dose-dependently induces a slow onset potentiation in the dentate gyrus in vivo. Eur J Pharmacol 294:497-503[Web of Science][Medline].
Manahan-Vaughan D, Reymann KG (1996) Metabotropic glutamate receptor subtype agonists facilitate LTP within a distinct time window in the dentate gyrus in vivo. Neuroscience 74:723-731[Web of Science][Medline].
Manahan-Vaughan D, Reiser M, Pin JP, Wilsch V, Reymann KG, Riedel G (1996) Physiological and pharmacological profile of trans-azetidine 2,4-dicarboxylic acid: metabotropic glutamate receptor agonism and effects on long-term potentiation. Neuroscience 72:999-1008[Web of Science][Medline].
Masu M, Tanabe Y, Tsuchida K, Shigemoto R, Nakanishi S (1991) Sequence and expression of a metabotropic glutamate receptor. Nature 349:760-765[Medline].
Mulkey RM, Malenka RC (1992) Mechanisms underlying induction of homosynaptic long-term depression in area CA1 of the hippocampus. Neuron 9:967-975[Web of Science][Medline].
Nakajima Y, Iwakabe H, Akazawa C, Nawa H, Shigemoto R, Mizuno N, Nakanishi S (1993) Molecular characterization of a novel retinal metabotropic glutamate receptor mGluR6 with a high agonist selectivity for L-amino-4-phosphonobutyrate. J Biol Chem 268:11868-11873[Abstract/Free Full Text].
O'Mara SM, Rowan MJ, Anwyl RA (1995) Metabotropic glutamate receptor-induced homosynaptic long-term depression and depotentiation in the dentate gyrus of the rat hippocampus in vitro. Neuropharmacology 34:983-989[Web of Science][Medline].
Okamoto N, Hori S, Akazawa C, Hayashi Y, Shigemoto R, Mizuno N, Nakanishi S (1994) Molecular characterization of a new metabotropic glutamate receptor mGluR7 coupled to inhibitory cyclic AMP signal transduction. J Biol Chem 269:1231-1236[Abstract/Free Full Text].
Paxinos G, Watson C (1986) In: The rat brain in stereotaxic coordinates, 2nd ed. New York: Academic.
Reyes M, Stanton PK (1996) Induction of hippocampal long-term depression requires release of Ca²⁺ from separate presynaptic and postsynaptic intracellular stores. J Neurosci 16:5951-5960[Abstract/Free Full Text].
Saugstad JA, Kinzie JN, Mulvihill ER, Segerson TP, Westbrook G (1994) Cloning and expression of a new member of the L-2-amino-4- phosphonobutyric acid-sensitive class of metabotropic glutamate receptors. Mol Pharmacol 45:367-372[Abstract].
Selig DK, Lee H-K, Bear M, Malenka RC (1995) Reexamination of the effects of MCPG on hippocampal LTP, LTD and depotentiation. J Neurophysiol 74:1075-1082[Abstract/Free Full Text].
Shigemoto R, Takaaki A, Nomura S, Nakanishi S, Hirano T (1994) Antibodies inactivating mGluR 1 metabotropic glutamate receptor block long-term depression in cultured Purkinje cells. Neuron 12:1245-1255[Web of Science][Medline].
Stanton PK (1995) Transient protein kinase C activation primes long-term depression and suppresses long-term potentiation of synaptic transmission in hippocampus. Proc Natl Acad Sci USA 92:1724-1728[Abstract/Free Full Text].
Stevens CF, Wang Y (1994) Changes in reliability of synaptic function as a mechanism for plasticity. Nature 371:704-707[Medline].
Tanabe Y, Masu M, Ishii T, Shigemoto R, Nakanishi S (1992) A family of metabotropic glutamate receptors. Neuron 8:169-179[Web of Science][Medline].
Tanabe Y, Nomura A, Masu M, Shigemoto R, Mizuno N, Nakanishi S (1993) Signal transduction, pharmacological properties, and expression patterns of two rat metabotropic glutamate receptors, mGluR3 and mGluR4. J Neurosci 13:1372-1378[Abstract].
Thomas NK, Jane DE, Tse HW, Watkins JC (1996a) $alpha$ -methyl derivatives of serine-O-phosphate as novel selective competitive metabotropic glutamate receptor antagonists. Neuropharmacology 35:637-642[Web of Science][Medline].
Thomas NK, Jane DE, Tse HW, Watkins JC (1996b) (S)- $alpha$ -ethylglutamic acid and (RS)- $alpha$ -cyclopropyl-4-phosphonophenylglycine as antagonists of L-AP4 and (1S,3S)-ACPD-induced depression of monosynaptic excitation of neonatal rat motoneurones. Br J Pharmacol 117:70P.
Watkins JC, Collingridge GL (1994) Phenylglycine derivatives as antagonists of metabotropic glutamate receptors. Trends Pharmacol 15:333-342[Medline].

Copyright ©1997 Society for Neuroscience   0270-6474/1997/173303-09$05.00/0

This article has been cited by other articles:

N. Lemon, S. Aydin-Abidin, K. Funke, and D. Manahan-Vaughan
Locus Coeruleus Activation Facilitates Memory Encoding and Induces Hippocampal LTD that Depends on {beta}-Adrenergic Receptor Activation
Cereb Cortex, May 11, 2009; (2009) bhp065v1.
[Abstract] [Full Text] [PDF]

A. Kemp and D. Manahan-Vaughan
{beta}-Adrenoreceptors Comprise a Critical Element in Learning-Facilitated Long-Term Plasticity
Cereb Cortex, June 1, 2008; 18(6): 1326 - 1334.
[Abstract] [Full Text] [PDF]

J. Klausnitzer and D. Manahan-Vaughan
Frequency Facilitation at Mossy Fiber-CA3 Synapses of Freely Behaving Rats Is Regulated by Adenosine A1 Receptors
J. Neurosci., April 30, 2008; 28(18): 4836 - 4840.
[Abstract] [Full Text] [PDF]

N. Lemon and D. Manahan-Vaughan
Dopamine D1/D5 Receptors Gate the Acquisition of Novel Information through Hippocampal Long-Term Potentiation and Long-Term Depression
J. Neurosci., July 19, 2006; 26(29): 7723 - 7729.
[Abstract] [Full Text] [PDF]

D. Manahan-Vaughan and K.-H. Braunewell
The Metabotropic Glutamate Receptor, mGluR5, is a Key Determinant of Good and Bad Spatial Learning Performance and Hippocampal Synaptic Plasticity
Cereb Cortex, November 1, 2005; 15(11): 1703 - 1713.
[Abstract] [Full Text] [PDF]

B. Poschel, B. Wroblewska, U. Heinemann, and D. Manahan-Vaughan
The Metabotropic Glutamate Receptor mGluR3 is Critically Required for Hippocampal Long-term Depression and Modulates Long-term Potentiation in the Dentate Gyrus of Freely Moving Rats
Cereb Cortex, September 1, 2005; 15(9): 1414 - 1423.
[Abstract] [Full Text] [PDF]

A. Kemp and D. Manahan-Vaughan
The 5-Hydroxytryptamine4 Receptor Exhibits Frequency-dependent Properties in Synaptic Plasticity and Behavioural Metaplasticity in the Hippocampal CA1 Region In vivo
Cereb Cortex, July 1, 2005; 15(7): 1037 - 1043.
[Abstract] [Full Text] [PDF]

D. J. Froc and R. J. Racine
Interactions Between LTP- and LTD-Inducing Stimulation in the Sensorimotor Cortex of the Awake Freely Moving Rat
J Neurophysiol, January 1, 2005; 93(1): 548 - 556.
[Abstract] [Full Text] [PDF]

A. Kemp and D. Manahan-Vaughan
Hippocampal long-term depression and long-term potentiation encode different aspects of novelty acquisition
PNAS, May 25, 2004; 101(21): 8192 - 8197.
[Abstract] [Full Text] [PDF]

S. M. Gallagher, C. A. Daly, M. F. Bear, and K. M. Huber
Extracellular Signal-Regulated Protein Kinase Activation Is Required for Metabotropic Glutamate Receptor-Dependent Long-Term Depression in Hippocampal Area CA1
J. Neurosci., May 19, 2004; 24(20): 4859 - 4864.
[Abstract] [Full Text] [PDF]

K. Naie and D. Manahan-Vaughan
Regulation by Metabotropic Glutamate Receptor 5 of LTP in the Dentate Gyrus of Freely Moving Rats: Relevance for Learning and Memory Formation
Cereb Cortex, February 1, 2004; 14(2): 189 - 198.
[Abstract] [Full Text] [PDF]

M. A. LYNCH
Long-Term Potentiation and Memory
Physiol Rev, January 1, 2004; 84(1): 87 - 136.
[Abstract] [Full Text] [PDF]

D. Manahan-Vaughan and A. Kulla
Regulation of Depotentiation and Long-term Potentiation in the Dentate Gyrus of Freely Moving Rats by Dopamine D2-like Receptors
Cereb Cortex, February 1, 2003; 13(2): 123 - 135.
[Abstract] [Full Text] [PDF]

J. L. Berkeley and A. I. Levey
Cell-Specific Extracellular Signal-Regulated Kinase Activation by Multiple G Protein-Coupled Receptor Families in Hippocampus
Mol. Pharmacol., January 1, 2003; 63(1): 128 - 135.
[Abstract] [Full Text] [PDF]

S.-T. Li, K. Kato, K. Tomizawa, M. Matsushita, A. Moriwaki, H. Matsui, and K. Mikoshiba
Calcineurin Plays Different Roles in Group II Metabotropic Glutamate Receptor- and NMDA Receptor-Dependent Long-Term Depression
J. Neurosci., June 15, 2002; 22(12): 5034 - 5041.
[Abstract] [Full Text] [PDF]

S. Otani, H. Daniel, M. Takita, and F. Crepel
Long-Term Depression Induced by Postsynaptic Group II Metabotropic Glutamate Receptors Linked to Phospholipase C and Intracellular Calcium Rises in Rat Prefrontal Cortex
J. Neurosci., May 1, 2002; 22(9): 3434 - 3444.
[Abstract] [Full Text] [PDF]

T. Kleppisch, V. Voigt, R. Allmann, and S. Offermanns
G{alpha}q-Deficient Mice Lack Metabotropic Glutamate Receptor-Dependent Long-Term Depression But Show Normal Long-Term Potentiation in the Hippocampal CA1 Region
J. Neurosci., July 15, 2001; 21(14): 4943 - 4948.
[Abstract] [Full Text] [PDF]

J.-H. Kim, R. Anwyl, Y.-H. Suh, M. B. A. Djamgoz, and M. J. Rowan
Use-Dependent Effects of Amyloidogenic Fragments of {beta}-Amyloid Precursor Protein on Synaptic Plasticity in Rat Hippocampus In Vivo
J. Neurosci., February 15, 2001; 21(4): 1327 - 1333.
[Abstract] [Full Text] [PDF]

D. Manahan-Vaughan, A. Kulla, and J. U. Frey
Requirement of Translation But Not Transcription for the Maintenance of Long-Term Depression in the CA1 Region of Freely Moving Rats
J. Neurosci., November 15, 2000; 20(22): 8572 - 8576.
[Abstract] [Full Text] [PDF]

D. Manahan-Vaughan
Long-term Depression in Freely Moving Rats is Dependent upon Strain Variation, Induction Protocol and Behavioral State
Cereb Cortex, May 1, 2000; 10(5): 482 - 487.
[Abstract] [Full Text] [PDF]

A. Ngezahayo, M. Schachner, and A. Artola
Synaptic Activity Modulates the Induction of Bidirectional Synaptic Changes in Adult Mouse Hippocampus
J. Neurosci., April 1, 2000; 20(7): 2451 - 2458.
[Abstract] [Full Text] [PDF]

D. J. Froc, C. A. Chapman, C. Trepel, and R. J. Racine
Long-Term Depression and Depotentiation in the Sensorimotor Cortex of the Freely Moving Rat
J. Neurosci., January 1, 2000; 20(1): 438 - 445.
[Abstract] [Full Text] [PDF]

L. M. Grover and C. Yan
Evidence for Involvement of Group II/III Metabotropic Glutamate Receptors in NMDA Receptor-Independent Long-Term Potentiation in Area CA1 of Rat Hippocampus
J Neurophysiol, December 1, 1999; 82(6): 2956 - 2969.
[Abstract] [Full Text] [PDF]

U. Staubli and J. Scafidi
Time-Dependent Reversal of Long-Term Potentiation in Area CA1 of the Freely Moving Rat Induced by Theta Pulse Stimulation
J. Neurosci., October 1, 1999; 19(19): 8712 - 8719.
[Abstract] [Full Text] [PDF]

M. F. Bear
Homosynaptic long-term depression: A mechanism for memory?
PNAS, August 17, 1999; 96(17): 9457 - 9458.
[Full Text] [PDF]

D. Manahan-Vaughan and K.-H. Braunewell
Novelty acquisition is associated with induction of hippocampal long-term depression
PNAS, July 20, 1999; 96(15): 8739 - 8744.
[Abstract] [Full Text] [PDF]

C. J. Beaver, Q.-H. Ji, and N. W. Daw
Effect of the Group II Metabotropic Glutamate Agonist, 2R,4R-APDC, Varies With Age, Layer, and Visual Experience in the Visual Cortex
J Neurophysiol, July 1, 1999; 82(1): 86 - 93.
[Abstract] [Full Text] [PDF]

D. Balschun, D. Manahan-Vaughan, T. Wagner, T. Behnisch, K. G. Reymann, and W. Wetzel
A Specific Role for Group I mGluRs in Hippocampal LTP and Hippocampus-Dependent Spatial Learning
Learn. Mem., March 1, 1999; 6(2): 138 - 152.
[Abstract] [Full Text]

N. A. Breakwell, M. J. Rowan, and R. Anwyl
(+)-MCPG Blocks Induction of LTP in CA1 of Rat Hippocampus via Agonist Action at an mGluR Group II Receptor
J Neurophysiol, March 1, 1998; 79(3): 1270 - 1276.
[Abstract] [Full Text] [PDF]

H. Li, S. R. B. Weiss, D.-M. Chuang, R. M. Post, and M. A. Rogawski
Bidirectional Synaptic Plasticity in the Rat Basolateral Amygdala: Characterization of an Activity-Dependent Switch Sensitive to the Presynaptic Metabotropic Glutamate Receptor Antagonist 2S-alpha -Ethylglutamic Acid
J. Neurosci., March 1, 1998; 18(5): 1662 - 1670.
[Abstract] [Full Text] [PDF]

L. L. Holland and J. J. Wagner
Primed Facilitation of Homosynaptic Long-Term Depression and Depotentiation in Rat Hippocampus
J. Neurosci., February 1, 1998; 18(3): 887 - 894.
[Abstract] [Full Text] [PDF]

T. Heinbockel and H.-C. Pape
Input-Specific Long-Term Depression in the Lateral Amygdala Evoked by Theta Frequency Stimulation
J. Neurosci., April 1, 2000; 20(7): RC68 - RC68.
[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 (111)

Citing Articles via Google Scholar

Google Scholar

Articles by Manahan-Vaughan, D.

Search for Related Content

PubMed

PubMed Citation

Articles by Manahan-Vaughan, D.