Metabotropic Glutamate Receptors Trigger Homosynaptic Protein Synthesis to Prolong Long-Term Potentiation

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The Journal of Neuroscience, February 1, 2000, 20(3):969-976

Metabotropic Glutamate Receptors Trigger Homosynaptic Protein Synthesis to Prolong Long-Term Potentiation
Clarke R. Raymond¹^,³, Vida L. Thompson²^,³, Warren P. Tate²^,³, and Wickliffe C. Abraham¹^,³
Departments of ¹ Psychology and ² Biochemistry and the ³ Neuroscience Research Centre, University of Otago, Dunedin, New Zealand

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We investigated the mechanisms by which previous "priming" activation of group I metabotropic glutamate receptors (mGluRs)facilitates the persistence of long-term potentiation (LTP) inarea CA1 of rat hippocampal slices. Priming of LTP was elicitedby either pharmacological or synaptic activation of mGluRs beforea weak tetanic stimulus that normally produced only a rapidlydecaying phase of LTP that did not involve protein synthesis ormGluRs. Pharmacological priming of LTP persistence by a selectivegroup I mGluR agonist was blocked by an inhibitor of group I mGluRsand by inhibitors of translation, but not by a transcriptionalinhibitor. The same mGluR agonist increased ³⁵S-methionine incorporation into slice proteins. LTP could alsobe facilitated using a synaptic stimulation priming protocol,and this effect was similarly blocked by group I mGluR and proteinsynthesis inhibitors. Furthermore, using a two-pathway protocol,the synaptic priming of LTP was found to be input-specific. Totest for the contribution of group I mGluRs and protein synthesisto LTP in nonprimed slices, a longer duration control tetanizationprotocol was used to elicit a more slowly decaying form of LTPthan did the weak tetanus used in the previous experiments. Thepersistence of the LTP induced by this stronger tetanus was dependenton mGluR activation and protein synthesis but not on transcription.Together, these results suggest that mGluRs couple to nearby proteinsynthesis machinery to homosynaptically regulate an intermediatephase of LTP dependent on new proteins made from pre-existingmRNA.

Key words: LTP; mGluRs; metaplasticity; protein synthesis; synaptic plasticity; hippocampus

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Long-term potentiation (LTP) is an input-specific and persistent increase in the strength of synaptic connections that isthe major model mechanism for information storage in the brain(Bliss and Lømo, 1973; Bliss and Collingridge, 1993). Of criticalimportance for LTP as a memory mechanism is its long-term maintenance.In general, a distinction is made between a rapidly decaying early-phaseLTP involving post-translational modification of proteins (Lovingeret al., 1987; Malinow et al., 1988) and a more persistent late-phaserequiring gene transcription and new protein synthesis (Krug etal., 1984; Nguyen et al., 1994; Frey et al., 1996). However, thereis some evidence for an intermediate phase of LTP dependent ontranslation but not transcription (Otani et al., 1989).

Many studies have reported that activation of metabotropic glutamate receptors (mGluRs) during a tetanus can promote the inductionand, in particular, the persistence of LTP (Behnisch et al., 1991;Bashir et al., 1993). The proposed need for mGluR activation inLTP has been controversial, however, indicating that mGluR activationmay not be necessary in all cases for durable LTP to occur (Chinestraet al., 1993; Thomas and O'Dell, 1995). One intriguing aspectof the mGluR contribution to LTP is that it can occur hours beforea tetanus (Bortolotto et al., 1994). Similarly, we have shownthat previous "priming" activation of group I mGluRs will transforma weak, decaying form of LTP into a more persistent form (Cohenand Abraham, 1996; Cohen et al., 1998). mGluR activation aftertetanic stimulation can also facilitate LTP persistence (Manahan-Vaughanand Reymann, 1996).

The degree of LTP persistence is not directly coupled to the degree of initial potentiation (Abraham et al., 1993), and thuswe have hypothesized that, whatever their contribution to theinduction of LTP, mGluRs may separately regulate the persistenceof LTP by coupling to protein synthesis mechanisms. This suggestionhas a precedent in that mGluR-mediated epileptiform dischargesin hippocampal slices have been shown to require protein synthesis(Merlin et al., 1998). Of particular interest, however, is thefact that protein synthesis machinery is located not only in somalregions of hippocampal neurons but also in dendrites and evendendritic spines (Steward, 1997). Accordingly, mGluRs are wellplaced to trigger transcription-independent de novo protein synthesisin spatially restricted synaptic sites. In confirmation of this,activation of mGluRs can trigger protein synthesis in hippocampalsynaptoneurosome preparations, which contain no transcriptionalmachinery (Weiler and Greenough, 1993; Weiler et al., 1997).

Here, we provide evidence that the priming of LTP persistence in area CA1 of the hippocampus by previous pharmacological orsynaptic activation of mGluRs occurs by a homosynaptic proteinsynthesis-dependent, but transcription-independent, mechanism.Furthermore, we identified a phase of nonprimed LTP that alsoentails mGluR activation and transcription-independent proteinsynthesis. Together, these findings suggest that local proteinsynthesis, triggered by group I mGluRs, allows for a long-lastingand input-specific phase of LTP without complex macromoleculartrafficking.

Parts of this work have been published previously in abstract form (Raymond and Abraham, 1998).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiology. Hippocampal slices (400 µm) were prepared from young adult male (200-300 gm) Sprague Dawley rats, as describedpreviously (Cohen et al., 1998). Slices were submerged in a brainslice chamber and preincubated for at least 2 hr in a continuousflow (2-3 ml/min) of artificial CSF (ACSF) [containing (in mM):124 NaCl, 3.2 KCl, 1.25 NaH₂PO₄, 26 NaHCO₃, 2.5 CaCl₂, 1.3 MgCl₂,and 10 D-glucose, equilibrated with 95% O₂-5% CO₂] at 32.5°C.Extracellular synaptic potentials were recorded from stratum radiatumin area CA1 using glass microelectrodes (1-3 M $Omega$ ) filled with 2M NaCl. Baseline synaptic responses were evoked by stimulationof the Schaffer collateral-commissural pathway at 0.033 Hz (diphasicpulses, 0.1 msec half-wave duration) with a 50 µm tungsten monopolarelectrode. The stimulation intensity was adjusted to elicit fieldEPSPs at population spike threshold as observed in the dendriticfield recording. This corresponded to a field EPSP of approximatelytwo-thirds maximum amplitude (the baseline potential was typicallybetween 1.5 and 2.0 mV in amplitude). In most cases, a singlestimulating electrode was used. In the heterosynaptic primingexperiments, one electrode was placed on either side of, and equidistantfrom, the recording electrode to stimulate independent inputsto the same neuronal population. LTP was induced by theta-burststimulation (TBS), consisting of trains of 10 × 100 Hz bursts(five diphasic pulses per burst) with a 200 msec interburst interval,at the test pulse intensity. Thus, 2 TBS consisted of two trainsof TBS, each train separated by 30 sec, and 0.5 TBS equaled halfa train, or five bursts only. Initial slopes of EPSPs were measuredoff-line and expressed as percentage change from baseline, calculatedas the average of the last 15 min of baseline recordings. Slicesthat had baseline values that varied >10% over the 30 min baselineperiod were discarded from the analysis. Two-tailed Student'st tests were performed to determine significance at the 95% confidencelevel, unless otherwise stated. Data are presented as group means±SEM.

Drugs and reagents. Reagents were obtained from the following vendors: all salts from BDH Chemicals (Poole, UK); (R,S)-3,5-dihydroxyphenylglycine(DHPG) and (R,S)-1-aminoindan-1,5,dicarboxylic acid (AIDA) fromTocris Cookson (Bristol, UK); D-2-amino-phosphonopentanoic acid(AP-5) from Research Biochemicals (Natick, MA); and cycloheximide,actinomycin-D (Act-D), and emetine from Sigma (St. Louis, MO).Drugs were dissolved in 100 mM NaOH (AIDA, D-AP-5), dH₂O (DHPG,emetine, cycloheximide), or DMSO (Act-D) and diluted at least500-fold to their final concentration inASCF.

³⁵S-Methionine incorporation. To measure the extent of ³⁵S-methionine (³⁵S-Met) incorporation into new proteins, four groups of four randomlyassigned hippocampal slices, prepared as above, were placed inculture dishes containing 5 ml of ACSF and preincubated for 1hr in a humidified carbogen atmosphere at 32.5°C. In groups 3and 4, 5 µl of emetine (final concentration of 20 µM) was added.After a 30 min incubation, 67 µl of ³⁵S-methionine (final concentration of 2 µCi/ml) was added to allfour groups. Five minutes later, 5 µl of DHPG (final concentrationof 20 µM) was added to groups 2 and 4. After a final 30 min incubation,100 µl of unlabeled methionine (final concentration of 0.1 mg/ml)was added to each dish to compete out further incorporation ofradiolabel. The four slices in each group were pooled, and theprotein was extracted in 1 ml of 10% TCA-0.1% methionine and centrifuged(12,000 rpm) for 15 min at 4°C. The pellet was washed three timesin 5% TCA-0.05% methionine and centrifuged (12,000 rpm) at 4°Cbetween each wash. The pellet was resolubilized in 1 M NaOH (500µl) and incubated overnight at 37°C. The next day, the extractwas neutralized with 1 M HCl (500 µl), and ³⁵S-met incorporation was measured on an LKB-Wallac (Gaithersburg,MD) Liquid Scintillation Counter in 6 ml of Starscint (Packard,Meridian, CT). This procedure was replicated using five differentbatches of 16slices.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

DHPG primes LTP through de novo protein synthesis from existing mRNA

We have shown previously that LTP induction and persistence can be primed by previous activation of group I mGluRs by theselective agonist DHPG (Cohen et al., 1998). To replicate thisfinding in the present experiments, slices were administered DHPG(20 µM) in the bathing medium for a 10 min period, beginning 30min before a weak tetanus, i.e., 0.5 TBS. DHPG treatment by itselfproduced a mild long-lasting synaptic depression that persistedafter drug washout, as has been reported previously (Palmer etal., 1997; Cohen et al., 1998). More importantly, DHPG increasedthe induction and persistence of subsequent LTP (40 ± 6%; n =7; measured 60 min after tetanus) relative to untreated controlslices (19 ± 1%; n = 6; p < 0.05) (Fig. 1A).

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Figure 1. Mechanisms of DHPG-induced priming of LTP in CA1 slices. A, After 1 hr of baseline recording, control slices were administered 0.5 TBS (arrow), which induced a decaying form of LTP. A 10 min priming application of DHPG (20 µM; dark bar) mildly depressed synaptic transmission but significantly enhanced the persistence of subsequent LTP. B, Delivery of either emetine (20 µM, 20 min; Emet) or cycloheximide (60 µM, 20 min; CXM, striped bar) before and during the DHPG priming period (dark bar) prevented the enhancement of LTP persistence. C, Emetine (20 µM, 20 min; striped bar) given immediately after 0.5 TBS had no effect on primed LTP (compare with B). D, Actinomycin-D (40 µM, 30 min; Act-D, striped bar), given before and during the DHPG priming period (dark bar), had no effect on the enhancement of LTP by DHPG. The slices presented in this figure were run in an interleaved manner.

The use of the priming paradigm provides the ability to temporally separate mGluR activation from tetanic stimulation, thusfacilitating investigations of the mechanisms downstream of mGluRactivation that may be important for LTP. Because we hypothesizedthat mGluR activation primes LTP at least in part by triggeringde novo protein synthesis, we tested the effects of two proteinsynthesis inhibitors on this phenomenon. Inhibition of proteinsynthesis by emetine (20 µM) or cycloheximide (60 µM), given for10 min before and during the mGluR priming period, did not affectthe initial induction of subsequent LTP but caused it to decayrapidly to control levels within 1 hr after tetanus (emetine,17 ± 9%; n = 4; p < 0.05; cycloheximide, 22 ± 4%; n = 4; p < 0.05)(Fig. 1B). Neither drug had any effect on the nonprimed LTP inducedby 0.5 TBS (data not shown). To assess whether DHPG acted by triggeringde novo protein synthesis rather than simply priming translationmechanisms engaged by the subsequent tetanus, emetine was addedat one of two times after DHPG priming. When emetine was appliedbeginning 10 min before, during, and for 10 min after the tetanus,the priming of LTP was again blocked (16 ± 3%; n = 4; p < 0.05;data not shown). However, when the timing of emetine applicationwas further delayed so as to occur for the 20 min immediatelyafter LTP induction, it had no effect on the maintenance of primedLTP (Fig. 1C). This stands in contrast to its effectiveness aftera stronger (nonprimed) tetanus that produces a more persistentform of LTP than the 0.5 TBS used here (compare with Fig. 4C).This time course over which emetine blocks the priming effectsuggests that DHPG triggers a rapid synthesis of proteins beforethe induction of LTP that then interacts with events triggeredby the tetanus to promote the persistence of the inducedLTP.

In contrast to the ability of protein synthesis inhibitors to block the DHPG-induced priming of LTP persistence, the transcriptionalinhibitor actinomycin-D, delivered for 20 min before and duringDHPG application at a dose (40 µM) and previously used to blockthe late phase of LTP (Nguyen et al., 1994; Nguyen and Kandel,1997), had no effect on the priming of LTP (41 ± 4%; n = 5) (Fig.1D). This result indicates that DHPG was triggering de novo synthesisof critical proteins from existing mRNA rather than from newtranscripts.

As a more direct test for mGluR-triggered protein synthesis, we performed experiments that measured the incorporation of radiolabeled³⁵S-Met into newly synthesized protein in hippocampal slices, asdescribed in Materials and Methods. DHPG caused a small but significantincrease in total ³⁵S-Met incorporation measured 30 min after drug application (17± 3%; n = 5 pooled samples of four slices each; p < 0.05; pairedt test) (Fig. 2). Preincubation of slices with emetine reducedthe increase in ³⁵S-Met incorporation by 78 ± 15% (n = 5).

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Figure 2. Summary histogram of ³⁵S-methionine incorporation into hippocampal slice proteins. A 30 min incubation with DHPG (20 µM) caused a significant increase in ³⁵S-methionine incorporation measured by scintillation counting. Preincubation of slices with emetine (20 µM, 30 min; Emet) reduced incorporation by 78%, confirming the efficacy of emetine in blocking protein synthesis, and blocked the DHPG-induced increase. Each of the five replications involved four pooled slices (randomly assigned) per treatment group. (*p < 0.05, significant difference from control; paired t test).

Mechanism of LTP priming by mGluRs activated by synaptically released glutamate

Can LTP be primed by mGluRs activated by synaptically released glutamate? To test this, we primed slices by synaptically activatingmGluRs through the delivery of 2 TBS but in the presence of theNMDA receptor antagonist AP-5 (50 µM) to prevent LTP induction.The AP-5 was then washed out for 20 min before the delivery ofa weak LTP-inducing stimulus (1 TBS). Despite the AP-5 treatment,the priming tetanus caused a small, slowly developing potentiationthat probably reflects an NMDA receptor-independent form of LTP(Grover and Teyler, 1990). As predicted, however, synapticallypriming in this way significantly enhanced subsequent LTP comparedwith AP-5-treated controls given the same weaker tetanus (control,14 ± 5% measured 60 min after tetanus; n = 5; primed, 36 ± 7%;n = 5; p < 0.05) (Fig. 3A). To determine whether this primingeffect relied on the activation of mGluRs and protein synthesis,either the group I mGluR antagonist AIDA (500 µM) (Moroni et al.,1997), which we have shown previously to block the DHPG-inducedpriming of LTP (Cohen et al., 1998), or emetine was applied beforeand during the priming stimulation. Neither drug affected thesmall NMDA receptor-independent potentiation elicited by the primingstimulation in the presence of AP-5, suggesting a lack of effecton voltage-dependent calcium channel function. However, AIDA completelyblocked the enhancement of subsequent LTP (13 ± 3%; n = 4; p <0.05) (Fig. 3B), as did 20 µM emetine (15 ± 3%; n = 4; p < 0.05)(Fig. 3C). These results support the hypothesis that synapticpriming is mediated by group I mGluR activation and that, as forpharmacologically primed LTP, protein synthesis is critical forthis enhancement of LTP.

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Figure 3. Synaptically released glutamate primes LTP by an mGluR-mediated mechanism. A, In controls, 1 TBS (light arrow) delivered 20 min after AP-5 (50 µM, 10 min; dark bar) wash induced a decaying form of LTP. Priming stimulation consisting of 2 TBS (dark arrow) in the presence of AP-5 resulted in a small, NMDA receptor-independent LTP that stabilized during AP-5 washout. LTP induced by 1 TBS subsequent to the priming stimulation was significantly enhanced. B, The group I mGluR antagonist AIDA (500 µM; dark bar), in combination with AP-5 during the priming stimulation, prevented the facilitation of LTP. C, Application of emetine (20 µM; Emet, striped bar) during the priming stimulation blocked the priming of LTP. D, To test for synapse specificity of the priming effect, two independent pathways to the same population of pyramidal cells were used. Path 1 (data not shown) received the 2 TBS priming stimulation (dark arrow) in the presence of AP-5 (dark bar). When 1 TBS was delivered to path 2 20 min later (light arrow), there was only a mild facilitation of the initial induction of LTP, which rapidly decayed to control levels. The control data from A are presented for comparison. These data demonstrate the input-specific nature of the mGluR and protein synthesis regulation of LTP. The slices A-C were run in an interleaved manner.

It was notable in these synaptic priming experiments that there was a stronger facilitation of LTP at early time points afterthe induction of LTP than that observed for the pharmacologicalpriming paradigm (compare Figs. 3A, 1A). This may reflect therelease of other neurotransmitters in addition to glutamate, suchas noradrenaline, which is capable of priming the initial LTPinduction but not its persistence (as opposed to mGluRs, whichprime both features of LTP) (Cohen et al., 1999). Such releaseof other neuromodulators may account for the residual early facilitationstill remaining in the AIDA-treated slices (Fig. 3B) comparedwith control values (Fig. 3A).

In the experiments above, the synaptic priming protocol was used to facilitate the induction of LTP homosynaptically, i.e.,for the same synapses that were primed. The critical proteins,however, could in principle have been either synthesized at, ortransported to, nonprimed synapses and thus been capable of modifyingLTP heterosynaptically (Frey and Morris, 1997). To address thisquestion, we delivered 2 TBS plus AP-5 to one pathway and, aftera 20 min wash, induced LTP on a second, independent pathway terminatingin the same dendritic zone using the weaker 1 TBS protocol. Althoughthe initial induction of LTP on the second pathway was facilitatedcompared with controls, its persistence was not (16 ± 6%; n =4) (Fig. 3D). These data are consistent with the interpretationthat the proteins synthesized in response to the priming protocolare active only at the primed synapses. This finding, togetherwith the rapidity of the priming effect (<20 min), suggests thatthese proteins are synthesized by polyribosomes located closeto the synaptically activatedmGluRs.

Contributions by mGluRs and protein synthesis to nonprimed LTP

We were interested in determining whether mGluR-triggered protein synthesis might also play a role in conventional, nonprimedLTP. As mentioned in the introductory remarks, it has been controversialwhether mGluRs play any vital role in the induction or persistenceof nonprimed LTP. The necessity of mGluR activation for LTP, however,may depend on the nature of the tetanic stimulus (Wilsch et al.,1998). Accordingly, we chose to use for these experiments thesame tetanic stimulus (2 TBS) that successfully primed LTP abovebut without concurrent application of AP-5. The 2 TBS protocolproduced an LTP that was nearly identical in magnitude to thatobserved after 0.5 TBS in DHPG-primed slices over 2 hr after tetanus(Fig. 4A), confirming that it may be a suitable stimulus for activatingmGluRs and triggering protein synthesis.

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Figure 4. Role of mGluR-triggered protein synthesis in nonprimed LTP. A, The delivery of 2 TBS (arrow) in nonprimed slices (open circles) gave a moderate degree of LTP induction and persistence similar to that observed previously in DHPG-primed slices (data from Fig. 1A replotted for comparison purposes; filled circles). B, The control level of LTP for 120 min after 2 TBS is plotted (open circles; same slices as in A). Note that LTP is still decremental. Block of group I mGluRs with AIDA (500 µM, 10 min before and during the tetanus; dark bar) significantly reduced the persistence of LTP. C, Emetine (20 µM, 20 min; Emet, striped bar), applied immediately after TBS to avoid any possible effects on the initial induction mechanisms of LTP, also caused a more rapid decay of LTP over the 2 hr period. D, In contrast to emetine, actinomycin-D (40 µM; Act-D, striped bar) applied for 20 min before and after 2 TBS had no effect on LTP persistence. The slices used for this figure were run in an interleaved manner.

The LTP induced by 2 TBS was robust yet slowly decaying (25 ± 3% at 2 hr after TBS; n = 6) (Fig. 4B). The persistence of thisLTP over 2 hr was dependent on mGluR activation because AIDA,delivered for 10 min before and during the TBS, caused the LTPto decay significantly more rapidly (12 ± 2%; n = 4; p < 0.05)(Fig. 4B). Consistent with previous studies of late-phase LTPafter TBS (Nguyen and Kandel, 1997), the persistence of LTP inducedby 2 TBS was dependent on the synthesis of new proteins. Thus,emetine (20 µM), when applied for 20 min beginning immediatelyafter tetanus, caused LTP to decay more rapidly than controls(14 ± 4%; n = 8; p < 0.05) (Fig. 4C). However, unlike the latephase of LTP induced by stronger, repeated trains of stimulation,the maintenance of 2 TBS-induced LTP was not affected by 40 µMactinomycin-D given before, during, and after the tetanus (25± 5%; n = 5) (Fig. 4D). These results show that de novo proteinsynthesis, triggered apparently by group I mGluR activation, isrequired to maintain the nonprimed LTP induced by a moderate stimulusand that such synthesis is programmed from pre-existingmRNA.

Comparison of drug effects across different LTP paradigms

Figure 5A summarizes and compares the profile of drug effects on LTP, measured at the end of the 1-2 hr post-tetanus recordingperiod, across three experimental paradigms described above. Thedegree of LTP for each drug group is expressed as a percent ofthe control LTP to normalize for different levels of LTP inductionacross the three paradigms. LTP induced by 0.5 TBS was not affectedby either AIDA, emetine, or actinomycin-D. These findings arein contrast to those for DHPG-primed LTP (0.5 TBS) and nonprimed2 TBS-induced LTP, which shared identical response profiles toeach drug; namely, AIDA and emetine both inhibited LTP persistence,whereas actinomycin-D had no effect.

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Figure 5. Summary histogram showing the effects of inhibiting transcription, translation, and group I mGluR activation on three LTP paradigms. A, The degree of LTP is represented as a percentage of their respective paradigm controls, measured at a fixed time after tetanus (1 hr time point for the 0.5 TBS groups, and 2 hr after tetanus for the 2 TBS groups). LTP induced by 0.5 TBS was unaffected by any of the drug treatments, thus reflecting the early protein synthesis-independent phase of LTP dependent on post-translational modifications. In contrast, both DHPG-primed LTP and LTP induced by 2 TBS were reduced by emetine and AIDA. Thus, both of these groups appear to engage similar mechanisms that govern the persistence of LTP, i.e., transcription-independent protein synthesis triggered by group I mGluRs. B, To control for differences in the level of induction, the persistence of LTP was taken as the rate constant of decay for the second, slower exponential function used in a double-exponential fit to the post-LTP data (Cohen and Abraham, 1996). Although statistics were performed on the rate constant data, for clarity reasons the data are plotted as the time constant of decay in minutes (i.e., the inverse of the rate constant). The drug profile of effects on decay rate for each tetanization condition was similar to that observed for LTP measured at a fixed value, as shown in A. These data confirm a role for mGluRs and protein synthesis in LTP persistence mechanisms, independent of any effects on LTP induction. (*p < 0.05, significant difference from control; Student's t test). Act-D, Actinomycin-D; Emet, emetine.

The above data represent snapshots of LTP, taken at a particular time after tetanization. Because such values depend on theinitial degree of LTP induction, even assuming a constant rateof decay, some of the drug effects may relate to altered LTP inductionrather than its persistence. To obtain a more complete pictureof LTP persistence, the post-tetanization data points for eachslice presented in Figure 5A were fit with the sum of two negativeexponentials, and the rate constant of decay for the second, slowerexponential was obtained and used as a measure of LTP persistence(Cohen and Abraham, 1996). Data from two slices were discardedbecause fits could not be made. The remaining rate constant valuesfor each drug group were then compared statistically with theirrespective control values. For clarity, the inverse of the meanrate constant for each group was calculated and plotted in Figure5B as the decay time constant, expressed in minutes. In accordwith the data presented in Figure 5A, none of drugs affected LTPpersistence in the 0.5 TBS condition, with all groups showingtime constants of decay of ~100 min. The two control groups giveneither DHPG priming plus 0.5 TBS or nonprimed 2 TBS both showeda more persistent form of LTP than that after 0.5 TBS, with atime constant of decay close to 200 min. In both of these experimentalparadigms, LTP persistence was significantly reduced by AIDA andemetine back to the level seen in those slices given 0.5 TBS alone.Actinomycin-D, however, had no significant effect on LTP persistencein theseexperiments.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present data are consistent with the hypothesis that activation of group I mGluRs triggers de novo protein synthesis fromexisting mRNA and thereby promotes the persistence of LTP. Interestingly,this protein synthesis can be initiated well before the tetanusand still affect LTP. Thus, the activated synapses can lie inan LTP-primed state, without significant overt evidence of thepriming event. This effect is a classic example of "metaplasticity"(Abraham and Bear, 1996; Abraham and Tate, 1997), in that theLTP response to a weak tetanus by primed synapses is much different(in this case, more persistent) than it otherwise would havebeen.

Local protein synthesis and LTP

The new proteins important for the mGluR-mediated enhancement of LTP appear to have been synthesized near the activated synapses,although we cannot completely rule out a role for somal translation.First, the effects were blocked by translational but not transcriptionalinhibitors, and the translational inhibitor was effective onlywithin a relatively narrow time window after mGluR stimulation.More importantly, however, the newly synthesized proteins promotedLTP stability in an input-specific manner, as demonstrated bythe synaptic priming experiments (Fig. 4). In combination, thesecharacteristics suggest that at least some of the necessary proteinsare synthesized in close proximity to the sites of mGluR activation.These conclusions are in accord with the finding that proteinsynthesis is stimulated by group I mGluRs in synaptoneurosomes(Weiler and Greenough, 1993). The input specificity of the presenteffect contrasts markedly with the robust heterosynaptic interactionsthat characterize the "synaptic tag" mechanism underlying thelate phase of LTP (Frey and Morris, 1997, 1998). In this lattercase, tetanized synapses are able to sequester proteins translatedelsewhere in the neuron, allowing an otherwise decremental potentiationto be stabilized by heterosynapticactivity.

There is considerable evidence that dendritic protein synthesis does occur in hippocampal neurons (Steward, 1994, 1997). Earlyindications for local protein synthesis of proteins came fromvisualization of synapse-associated polyribosomes in the dendritesof dentate granule cells (Steward and Levy, 1982). Subsequently,both morphological and biochemical studies have revealed a fullcomplement of functional protein synthesis machinery in the dendritesof many different neuronal types (Tiedge and Brosius, 1996; Torreand Steward, 1996; Gardiol et al., 1999). The other importantfinding has been the localization of mRNA in neurites of culturedhippocampal neurons (Bruckenstein et al., 1990; Kleiman et al.,1993) and, more importantly, at the base of dendritic spines inrat hippocampus (Martone et al., 1996). To date, mRNAs encodingover 20 proteins have been isolated near dendritic spines, includingsome with known or inferred roles in LTP, such as $alpha$ CaMkinase II( $alpha$ CaMKII), growth-associated protein 43, tyrosine receptor kinaseB, cAMP response element-binding protein, activity-related cytoskeletalprotein, and several glutamate receptor subunits (Steward, 1997;Tongiorgi et al., 1997; Gao, 1998).

A role for synaptically located protein synthesis has already been proposed to underlie various forms of synaptic plasticity,such as neurotrophin-induced synaptic potentiation in the hippocampus(Kang and Schuman, 1996), long-term facilitation at the Aplysiasensory to motor neuron synapse (Ghirardi et al., 1995), and long-termdepression at cerebellar synapses (Linden, 1996). In addition,our laboratory has shown previously that a phase of dentate gyrusLTP in anesthetized rats may involve transcription-independentprotein synthesis (Otani et al., 1989). Thus, protein synthesisin localized dendritic or synaptic areas may be a general featureof long-term synaptic plasticity. Because the hippocampal LTPexperiments have not been performed in reduced synaptic preparations(Linden, 1996), the possibility remains that the critical proteinsare translated from existing somal mRNA and transported down thedendrites to activated synaptic sites. In this latter model, however,the issue of how newly synthesized proteins can be targeted tothe correct synaptic sites in so short a time frame is highlyproblematic (Schuman, 1997). Locally synthesized proteins, incontrast, provide a means for rapid synapse-specific stabilizationof LTP, without requiring complex macromoleculartrafficking.

mGluRs and LTP

There has been considerable controversy surrounding the extent to which mGluRs play a role in hippocampal LTP. It is clearfrom a number of studies that mGluRs are not always essentialfor normal LTP induction and persistence (Selig et al., 1995;Thomas and O'Dell, 1995), raising the possibility that they playa more modulatory role (Ben-Ari and Anikstejn, 1995). In accordwith this concept, we and others have observed that mGluRs contributeto LTP only for certain tetanization conditions. For example,in the present experiments, AIDA did not affect the decrementalLTP elicited by a weak tetanus (0.5 TBS). We interpret this findingas reflecting a relatively poor activation of mGluRs by synapticallyreleased glutamate. It has been shown for mossy fiber synapsesin CA3, for example, that activation of mGluRs is use-dependent,being considerably magnified during the course of high-frequencystimulation (Scanziani et al., 1997). This is probably becauseof a use-dependent increase in glutamate concentration in thesynaptic cleft. Thus, we consider it likely that an insufficientglutamate concentration is established during 0.5 TBS in the presentexperiments to activate group I mGluRs, which are located peripherallyon the postsynaptic density (Lujan et al., 1996). This can berectified if the mGluRs are activated pharmacologically by DHPGor if the glutamate concentration is raised by using longer durationtetanic stimulation (2TBS).

A separate study has shown that too strong a tetanus reduces the dependency of LTP on mGluR activation (Wilsch et al., 1998).This result was interpreted as reflecting activation of alternativemechanisms that elevate calcium postsynaptically, thus occludingany contribution made by mGluRs. Alternatively, this may reflectredundant mechanisms for triggering the necessary synthesis ofproteins. Together, these studies indicate that mGluRs play acritical role in LTP formation only under certain conditions.We propose that one major contribution made by mGluRs under conditionsof moderate activation is the triggering of dendritic proteinsynthesis, perhaps through protein kinase C (PKC)-mediated phosphorylationof translation initiation factors, such as the eIF4E subunit ofthe mRNA cap binding complex eIF4F (Sonenburg, 1996). In accordwith this hypothesis, we have observed that PKC inhibitors blockthe priming of LTP by DHPG (C. R. Raymond and W. C. Abraham, unpublishedobservations).

An mGluR-dependent intermediate phase of LTP

Typically, LTP persistence is divided into two distinct phases, referred to as early LTP and late LTP. In this model, earlyLTP is solely dependent on post-translational modifications, whereaslate LTP is dependent on both new transcription and translation,respectively (Matthies, 1989, Nguyen et al., 1994). On the otherhand, an analysis of dentate gyrus LTP persistence in freely movinganimals revealed three families of exponential decay curves [termedLTP1, 2, and 3 (Abraham and Otani, 1991 after Racine et al., 1983)],and the suggestion was made that there may be a protein synthesis-dependent,but transcription-independent, intermediate phase of LTP (i.e.,LTP2). This hypothesis was supported by the observations thata form of LTP in anesthetized animals was blocked by anisomycinbut not actinomycin-D (Otani et al., 1989) and that the intermediatephase of LTP persistence was associated with little or no activationof immediate early genes (Abraham et al., 1993).

The present study demonstrates that such an intermediate stage of LTP also exists in CA1 slices. The dependence of this phaseon protein synthesis stands in contrast to another recently describedintermediate form of LTP that is independent of protein synthesisbut regulated by protein kinase A and calcineurin (Winder et al.,1998). Both forms of intermediate LTP, however, appear to be maskedwhen a full-blown transcription-dependent late phase of LTP isinduced. In the mGluR- and protein synthesis-dependent intermediatephase, this occlusion could be attributable to a similarity inthe proteins being made from the new and existing mRNA or, alternatively,an inhibition of the mGluR-stimulated cascade when a strongertetanization is used and a greater calcium concentration is established.Protein synthesis in some systems can be inhibited by the calcium-dependentphosphorylation of the $alpha$ -subunit of initiation factor eIF2 (Rowlandset al., 1988). This process would be expected to compete withthe PKC-dependent facilitation of protein synthesis describedabove.

Conclusions

Overall, our data provide firm evidence for an intermediate phase of LTP in area CA1 of the hippocampus that is dependenton mGluR-triggered protein synthesis from pre-existing mRNA. Theinvolvement of transcription-independent protein synthesis inthis phase of LTP suggests that mRNAs constitutively present inthe dendrites encode proteins that promote moderate duration LTP.For example, an increase in the sensitivity of AMPA receptorsby $alpha$ CaMKII phosphorylation has been proposed as one of the mechanismsof early LTP expression (Bliss and Collingridge, 1993). The mRNAfor $alpha$ CaMKII is constitutively present in dendrites (Steward, 1997;Gao, 1998), and its local translation is subject to activity-dependentcontrol (Wu et al., 1998). Newly synthesized $alpha$ CaMKII may thusact to augment and prolong the action of the constitutively expressedkinase, or it may act at a different subsynaptic location. Onthe other hand, the synthesis of proteins required for longer-termmaintenance of LTP (requiring, for example, structural modifications)is transcriptionally controlled, hence the critical requirementfor a period of transcription to express this latephase.

  FOOTNOTES

Received June 21, 1999; revised Nov. 12, 1999; accepted Nov. 18, 1999.

This research was supported by the New Zealand Health Research Council. We thank Dr. B. Mockett for assistance with some ofthe experiments and Drs. C. M. Coussens and M. F. Bear for helpfulcomments on previous versions of thismanuscript.
Correspondence should be addressed to Prof. Wickliffe C. Abraham, Department of Psychology, Box 56, Dunedin, New Zealand.E-mail: cabraham{at}psy.otago.ac.nz.

Dr. Raymond's present address: John Curtin School of Medical Research, Division of Neurosciences, The Australian NationalUniversity, Canberra, ACT 2601,Australia.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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