Evidence for Involvement of Central 5-HT4 Receptors in Cholinergic Function Associated with Cognitive Processes: Behavioral, Electrophysiological, and Neurochemical Studies

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Vol. 296, Issue 3, 676-682, March 2001

Evidence for Involvement of Central 5-HT₄ Receptors in Cholinergic Function Associated with Cognitive Processes: Behavioral, Electrophysiological, and Neurochemical Studies

Machiko Matsumoto, Hiroko Togashi, Kiyoshi Mori, Ken-ichi Ueno, Satoshi Ohashi, Taku Kojima and Mitsuhiro Yoshioka

Departments of Pharmacology (M.M., H.T., K.M., K.-i.U., S.O., M.Y.) and Anesthesiology (T.K.), Hokkaido University School of Medicine, Sapporo, Japan

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

The possible involvement of 5-HT₄ receptors in cognitive function was investigated with a view toward modulating the cholinergicneuronal system. For this purpose, behavioral, electrophysiological,and neurochemical studies were performed in rats. The behavioralstudy, using a passive avoidance test, demonstrated that the 5-HT₄receptor agonist SC 53116 (10 µg/rat i.c.v.) had an ameliorativeeffect on the muscarinic receptor antagonist scopolamine-induced(1 mg/kg i.p.) impairment of learning. The electrophysiologicalstudy showed that SC 53116 (1 and 10 µg/rat i.c.v.) enhanced thepopulation spike amplitude in the hippocampal CA1 field evokedby Schaffer collateral stimulation. SC 53116 (10 µg/rat i.c.v.)also augmented the tetanus-induced long-term potentiation (LTP).This augmented LTP was blocked not only by the selective 5-HT₄receptor antagonist GR 113808 (20 µg/rat i.c.v.) but also by scopolamine(1 mg/kg i.p.). These findings suggest that the functional interactionbetween the serotonergic system mediated via 5-HT₄ receptors andthe cholinergic system associated with cognitive processes existsin vivo. This possibility was further strengthened by neurochemicalstudy using in vivo microdialysis; local administration of SC53116 (10 and 100 µM) concentration-dependently enhanced the extracellularlevels of acetylcholine (ACh) in the hippocampus. SC 53116-induced(10 µM) facilitation of ACh release was prevented by coperfusionof GR 113808 (10 µM). Taken together, the present findings obtainedby these different approaches indicate the possibility that the5-HT₄ receptors are involved in cognitive impairment induced bythe cholinergic neuronalsystem.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Serotonin (5-HT)₄ receptors are widely expressed in the central and peripheral neuronal systems (Hoyer et al., 1994), however,little is known about their physiological roles in the centralnervous system. 5-HT₄ receptors are concentrated in the limbicstructures, including the hippocampus, which plays an essentialrole in memory processes (Waeber et al., 1993; Ullmer et al.,1996). The activation of 5-HT₄ receptors is known to stimulateadenylyl cyclase activity in the hippocampus of rats (Torres etal., 1995; Markstein et al., 1999) and guinea pigs (Bockaert etal., 1990). Furthermore, increasing evidence indicates that cAMPplays an important role in the hippocampal long-term potentiation(LTP), which is thought to be a form of the basic cellular mechanismsunderlying learning and memory (Frey et al., 1993; Abel et al.,1997; Otmakhova et al., 2000). These previous findings suggesta possible involvement of 5-HT₄ receptors in the modulation ofcognitivefunctions.

Indeed, several behavioral studies have shown that 5-HT₄ receptors were associated with learning and memory processes. Forinstance, the mixed 5-HT₄ agonist/5-HT₃ antagonist BIMU 1 showedameliorative effects in the rat olfactory association learningtest (Letty et al., 1997; Marchetti-Gauthier et al., 1997). BIMU1 also improved the scopolamine-induced amnesia in the mouse passiveavoidance test (Galeotti et al., 1998). The 5-HT₄ receptor agonistRS 67333 prevented atropine-induced learning impairment in theMorris water maze test (Fontana et al., 1997). Terry et al. (1998)reported, using a delayed matching-to-sample task, that the 5-HT₄receptor agonist RS 17017 improved memory processes in youngerand older monkeys. They suggested that the 5-HT₄ receptor-mediatedimprovements in older monkeys, in particular, have implicationsfor neurodegenerative conditions such as Alzheimer's disease.Furthermore, a binding study suggested that a marked loss of 5-HT₄receptors was found in the hippocampus of patients with Alzheimer'sdisease (Reynolds et al., 1995). These findings lead us to speculatethat 5-HT₄ receptors partially contributed to the cholinergicfunction associated with cognitive processes. However, to ourknowledge, there is no evidence supporting the presence of thefunctional interaction between the serotonergic neuronal mechanismsmediated via 5-HT₄ receptors and cholinergic function based onbehavioral alterations and physiological changes in these neuronalsystems.

The present study was undertaken to elucidate the functional role of 5-HT₄ receptors with a view toward modulating the cholinergicneuronal system. For this purpose, behavioral, electrophysiological,and neurochemical studies were performed in rats. The behavioralstudy was carried out to evaluate the memory and learning functionusing a passive avoidance task. The electrophysiological approachwas performed to examine the synaptic transmission by measuringthe population spike amplitude in the hippocampal CA1 field. Neurochemically,an in vivo microdialysis method was used to elucidate the dynamicchanges in hippocampal cholinergic neuronal activity by determiningacetylcholine (ACh) release. Based on these differential paradigms,the physiological function of central 5-HT₄ receptors wasinvestigated.

	Materials and Methods

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General Procedures. Male Wistar strain rats (11-14 weeks old) were used. Rats were housed in a room with a 12-h light (7:00 AM to 7:00 PM)/dark(7:00 PM to 7:00 AM) cycle under a constant temperature (21 ±2°C). All handling of animals was performed in accordance withguidelines for the Care and Use of Laboratory Animals of the AnimalResearch Committee of the Hokkaido University School of Medicine.Drugs were administered intraperitoneally (i.p.) or intracerebroventricularly(i.c.v.) or perfused locally via a dialysis probe. A probe fori.c.v. injection was inserted at the following coordinates relativeto bregma and dural surface, i.e., caudal, 0.8 mm; lateral, 1.4mm; ventral, 3.3 mm through the guide cannula, and 10 µl of drugwas administered at a flow rate of 2 µl/min. As controls, saline(0.9% NaCl) or artificial cerebrospinal fluid (in mM: KCl 2.7,NaCl 140, CaCl₂ 1.2, MgCl₂ 1.0, NaH₂PO₄ 0.3, Na₂HPO₄ 1.7) wasadministered i.p. or i.c.v.,respectively.

Behavioral Study. The passive avoidance test was performed according to the step-through method (Jarvik and Kopp, 1967). The apparatus consistedof a light compartment connected to a dark box by a dividing wallcontaining a guillotine door. In the training session, an acquisitiontrial was performed as follows; rats were acclimated in the lightcompartment for 2 min, then the guillotine door was opened. Threeseconds later, when the rats crossed over into the dark box, aninescapable electrical shock (0.8 mA, 3 s) was delivered. Thistrial was repeated until acquisition was established. Acquisitionwas regarded as being established when rats eventually remainedin the light compartment for more than 300 s to avoid enteringthe dark box. The number of entries into the dark box to learnthe "information for electrical shock" was counted until acquisitionwas established. After 24 h, the retention test was conducted:rats were placed in the light compartment and the time taken toenter the dark box, the latency time (seconds), was measured upto a maximum of 600 s. In this experiment, drugs were administeredfollowing three protocols: in protocol 1, the muscarinic receptorantagonist scopolamine was administered after acquisition. Inprotocol 2, scopolamine was injected before the training session,and the 5-HT₄ receptor agonist SC 53116 (Flynn et al., 1992) wasadministered after acquisition. In protocol 3, scopolamine andSC 53116 were administered before the trainingsession.

Electrophysiological Study. The efficacy of synaptic transmission was evaluated by monitoring the population spike amplitude in the hippocampal CA1 field.Rats anesthetized with 1% halothane in a mixture of 20% O₂ and80% N₂ were fixed in a stereotaxic frame according to bregma andlambda in the same horizontal plane. A bipolar stainless steelelectrode was used to stimulate Schaffer collaterals (3.0 mm posterior,1.5 mm lateral to the bregma, 2.8 mm ventral to the dura). A monopolarglass-coated recording electrode was placed in the ipsilateralpyramidal cell layer of CA1 (5.0 mm posterior, 3.0 mm lateralto the bregma, approximately 2.3 mm ventral to the dura). Theevoked potential by test stimulation (frequency 0.1 Hz, pulseduration 250 µs, stimulus interval 30 s) was amplified and monitoredwith an oscilloscope. The integrated population spike amplitudeobtained from five successive stimuli was recorded every 5 minwith a data-analyzing system (ATAC-450, Nihon Kohden, Japan).The intensity of the test stimulation was adjusted for each ratto elicit a population spike amplitude of approximately 50% maximumamplitude. LTP, which is suggested as the electrophysiologicalmodel for learning and memory (Bliss and Collingridge, 1993),was induced by tetanic stimulation (5 trains at 1 Hz each, composedof eight pulses at 400 Hz) at the same intensity as the test stimulus.Tetanic stimulation was given 20 min after the drugadministration.

Neurochemical Study. In vivo microdialysis technique was used to estimate the cholinergic neuronal activity in the hippocampus of freely movingrats. Rats were anesthetized with ketamine (100 mg/kg i.p.) anda 3-mm concentric guide cannula was stereotaxically implantedinto the hippocampus (5.8 mm posterior, 4.8 mm lateral to thebregma, 4.0 mm ventral to the dura). Two days after surgery, adialysis probe was inserted through the guide cannula and perfusedat a flow rate of 1 µl/min with Ringer's solution (KCl 2.7, NaCl147, CaCl₂ 2.3 mM) containing 10 µM physostigmine. Perfusion wasperformed to obtain the stable baseline for 120 to 180 min, andsuccessive 20-µl samples were collected at 20-min intervals. Drugswere administered into the hippocampus via the dialysis probe.The extracellular levels of ACh were measured using high performanceliquid chromatography (HPLC) with an electrochemical detector(Acetylcholine Analytical System, Eicom, Co. Ltd., Japan), asdescribed previously (Hirokami et al., 1994). Briefly, ACh andcholine were separated using an AC-Gel column attached to theenzyme reactor containing acetylcholinesterase and choline oxidase.ACh was assayed using the HPLC-electrochemical detector followingits conversion to hydrogen peroxide, which was electrochemicallydetected at a platinum working electrode at 450 mV versus theAg/AgCl reference electrode. The mobile phase contained 0.1 Msodium phosphate buffer (pH 8.5), 0.6 mM tetramethylammonium chloride,and 0.8 mM sodium 1-decanesulfonate. The HPLC separation and enzymaticreactions were performed at 33°C.

Drugs. SC 53116 (1-(S)-1-exo-4-amino-5-chloro-N-[(hexahydro-1H-pyrrolizin-1-yl)methyl]-2-methoxybenzamide, hydrocholoride, monohydrate)was donated by G.D. Searle and Co. Ltd (Chicago, IL). GR 113808(1-[2-(methylsulphonylamino)ethyl]-4-piperidinyl]methyl-1-methyl-1H-indole-3-carboxylate,maleate salt was donated by Glaxo Wellcome Co. Ltd. (Greedfold,UK). Scopolamine hydrobromide was purchased from Sigma (St. Louis,MO).

Statistics. All experimental results were represented as mean ± S.E.M. Values obtained by neurochemical studies using in vivo microdialysisand electrophysiological techniques were expressed as a percentageof the baseline levels before drug administration. For comparisonwith the experimental groups, Student's unpaired t test or Dunnett'stest was conducted after assessment by analysis of variance (ANOVA).Probability values less than 5% were consideredsignificant.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Behavioral Study: Effects of SC 53116 on Cholinergic Function in the Passive Avoidance Test. To evaluate the involvement of 5-HT₄ receptors in the cholinergic function of cognitive processes, the muscarinic receptorantagonist, scopolamine was used as an amnesic agent. Scopolamine(0.3 and 1 mg/kg i.p.), when administered before the trainingsession, reduced the latency for entering the dark box duringthe retention test in a dose-dependent manner. Scopolamine-induced(1 mg/kg i.p.) amnesic effects, however, were not observed whenadministered immediately after acquisition (Fig. 1). The 5-HT₄receptor agonist, SC 53116 (10 µg/rat i.c.v.) tended to amelioratethe scopolamine-induced (1 mg/kg i.p.) reduction of entrance latency,but not significantly. SC 53116 (10 µg/rat i.c.v.), when administeredalone, showed no influence on the latency during the retentiontest compared with controls (Fig. 2). Scopolamine (1 mg/kg i.p.),administered before the training session significantly increasedthe total number of entries into the dark box for acquisition.Co-administration of SC 53116 (10 µg/rat i.c.v) significantlyattenuated increases in the number of entries induced by scopolamine(Fig. 3). Thus, SC 53116 improved the scopolamine-induced deficitin the learning processes. SC 53116 (10 µg/rat i.c.v.) by itselfdid not alter the entrance counts compared with controls (Fig.3).

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Fig. 1. Effects of scopolamine on entrance latency in the retention of the passive avoidance test. Experiments were performed as follows: protocol 1; scopolamine (1 mg/kg i.p.) was administered immediately after acquisition of the training session. Protocol 2; scopolamine (0.3 and 1 mg/kg i.p.) was injected 30 min before the training session. The number of rats is shown inside each column. Values represent the mean ± S.E.M. *p < 0.05 versus saline-treated controls.

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Fig. 2. Effects of SC 53116 on scopolamine-induced entrance latency in the retention of the passive avoidance test. Experiments were performed as follows. Protocol 2: scopolamine (1 mg/kg i.p.) was injected 30 min before the training session. SC 53116 (10 µg/rat i.c.v.) was administered immediately after the acquisition of the training session. Protocol 3: scopolamine (1 mg/kg i.p.) and SC 53116 (10 µg/rat i.c.v.) were administered 30 and 20 min, respectively, before the training session. The number of rats is shown inside each column. Values represents the mean ± S.E.M. *p < 0.05 versus saline-treated controls.

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Fig. 3. Effects of SC 53116 on the scopolamine-induced number of entries (counts) during the training session of the passive avoidance test. Scopolamine (1 mg/kg i.p.) and SC 53116 (10 µg/rat i.c.v.) were administered 30 and 20 min, respectively, before the training session (protocol 3). The number of rats is shown inside each column. Values represent the mean ± S.E.M. *p < 0.05 and ^#p < 0.05 versus saline-treated controls and scopolamine-administered rats, respectively.

Electrophysiological Study: Effects of SC 53116 on Synaptic Transmission in the Hippocampal CA1 Field. The efficacy of synaptic transmission was estimated by monitoring the population spike amplitude in the CA1 field. SC 53116(1 and 10 µg/rat i.c.v.) enhanced the population spike amplitudeevoked by test stimulation of Schaffer collaterals in a concentration-dependentmanner (Fig. 4A). SC 53116-induced (10 µg/rat i.c.v.) facilitationwas significantly prevented by pretreatment with the selective5-HT₄ receptor antagonist GR 113808 (20 µg/rat i.c.v.). GR 113808alone did not affect the synaptic transmission (Fig. 4B). As shownin Fig. 5, tetanic stimulation evoked long-lasting increases inthe population spike amplitude with a maximum effect of 210%,i.e., LTP was induced. Application of SC 53116 (10 µg/rat i.c.v.)caused an enhanced amplitude of LTP (maximum effect; 307.0 ± 27.8%,n = 6). SC 53116-induced augmentation of LTP was significantlyprevented by scopolamine (1 mg/kg i.p.). Scopolamine (1 mg/kgi.p.), when administered alone, significantly suppressed LTP formationcompared with controls (Fig. 5). SC 53116-induced (10 µg/rat i.c.v.)enhancement of LTP was also abolished by pretreatment with GR113808 (20 µg/rat i.c.v.) (maximum effects; 172.1 ± 23.4%, n =4, p < 0.05).

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Fig. 4. Effects of SC 53116 on the population spike amplitude evoked by the test stimulation in the hippocampal CA1 field of anesthetized rats. A, time course responses of the population spike amplitude after SC 53116 (1 and 10 µg/rat i.c.v.) administration. Specimen recordings show superimposed traces of the population spike amplitude before and after SC 53116 (10 µg/rat i.c.v.) administration. Data were expressed as a percentage of the baseline levels before SC 53116 administration. B, maximum response of SC 53116-induced (10 µg/rat i.c.v.) changes in the population spike amplitude in the presence or absence of GR 113808 (20 µg/rat i.c.v.). GR 113808 was injected i.c.v. 10 min before SC 53116 administration. The number of rats is shown inside each column. Values represent the mean ± S.E.M. *p < 0.05 and ^#p < 0.05 versus controls and SC 53116-administered rats, respectively.

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Fig. 5. Effects of SC 53116 on the population spike amplitude evoked by tetanic stimulation in the hippocampal CA1 field of anesthetized rats. A, specimen recordings show superimposed traces of the population spike amplitude before and after tetanic stimulation in the presence of SC 53116 (10 µg/rat i.c.v.). Time course responses (A) and maximum responses (B) of LTP induced by SC 53116 (10 µg/rat i.c.v.) in the presence or absence of scopolamine (1 mg/kg i.p.). Scopolamine (1 mg/kg i.p.) was injected 10 min before SC 53116 administration. Data were expressed as a percentage of the baseline levels before SC 53116 administration. The number of rats is shown inside each column. Values represent the mean ± S.E.M. *p < 0.05 and ^#p < 0.05 versus controls and SC 53116-administered rats, respectively.

Neurochemical Studies: Effects of SC 53116 on ACh Release in the Rat Hippocampus. To evaluate the dynamic changes of cholinergic neuronal activity, in vivo microdialysis was used by determining ACh releasefrom the hippocampus. Extracellular levels of ACh were significantlyand concentration-dependently increased by local application ofSC 53116 (10 and 100 µM). SC 53116 (1 µM) did not affect the AChrelease (Fig. 6). SC 53116-induced (10 µM) increases in ACh releasewere significantly abolished by coperfusion with GR 113808 (10µM). GR 113808 (10 µM), when perfused alone, did not influencethe ACh levels (Fig. 7). The mean basal level of ACh was 2.5 ±0.2 pmol/sample (n = 25). There were no significant differencesin the basal ACh levels among the groups.

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Fig. 6. Effects of SC 53116 on the extracellular levels of ACh in the hippocampus of freely moving rats. Time course responses (A) and maximum responses (B) of SC 53116-induced (1, 10, and 100 µM) changes in ACh release. SC 53116 was administered locally via dialysis probe over a period of 60 min. Data were expressed as the percentage of baseline levels before SC 53116 perfusion. Basal levels, determined immediately before perfusion of SC 53116, were 1 µM, 2.04 ± 0.20 pmol/20 min; 10 µM, 2.69 ± 0.38 pmol/20 min; 100 µM, 2.11± 0.48 pmol/20 min. These values did not differ significantly from that of controls (2.61 ± 0.27 pmol/20 min). The number of rats is shown inside each column. Values represent the mean ± S.E.M. *p < 0.05 versus controls.

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Fig. 7. Effects of GR 113808 on SC 53116-induced changes in ACh release in the hippocampus of freely moving rats. Time course responses (A) and maximum responses (B) of SC 53116-induced (10 µM) changes in ACh release in the presence or absence of GR 113808 (10 µM). GR 113808 (10 µM) was administered locally via dialysis probe over a period of 60 min and coperfused with SC 53116 (10 µM). Data were expressed as a percentage of the baseline levels before GR 113808 perfusion. Basal levels, determined immediately before perfusion of drugs, were SC 53116 (10 µM), 2.69 ± 0.38 pmol/20 min; SC 53116 (10 µM) + GR 113808 (10 µM), 2.51 ± 0.19 pmol/20 min; and GR 113808 (10 µM), 2.11 ± 0.24 pmol/20 min. The number of rats is shown inside each column. Values represent the mean ± S.E.M. *p < 0.05 and ^#p < 0.05 versus controls and SC 53116-treated rats, respectively.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Based on the findings using the behavioral tests and electrochemical techniques, the present study demonstrated that the 5-HT₄receptors were involved in the modulation of the cholinergic functionassociated with learning and memory. This physiological interactionbetween the serotonergic system mediated via 5-HT₄ receptors andthe cholinergic system was further confirmed by neurochemicalevidence, i.e., hippocampal ACh release was enhanced by activationof 5-HT₄receptors.

A previous study using in vivo microdialysis reported that i.c.v. injection of the nonselective 5-HT₄ receptor agonist, BIMU1, caused enhanced ACh release in the rat frontal cortex, butits facilitation did not appear in the hippocampus (Consolo etal., 1994). In the present study, ACh release was increased bylocal application of the 5-HT₄ receptor agonist, SC 53116, andthis facilitation was blocked by the selective 5-HT₄ receptorantagonist GR 113808. These findings strongly indicate that the5-HT₄ receptor-mediated regulation of cholinergic neurons existsnot only in the frontal cortex (Consolo et al., 1994; Yamaguchiet al., 1997) but also in the hippocampus. In agreement with theobservation in the frontal cortex (Consolo et al., 1994), GR 113808alone showed no effect on the ACh release, suggesting that the5-HT₄ receptors did not tonically influence the cholinergic neuronalsystem in the rathippocampus.

It is conceivable that 5-HT₄ receptors are located on cholinergic nerve terminals in the hippocampus as well as in the entericnervous system (Tonini et al., 1991) and thus stimulate ACh release.Although the precise mechanisms of the neuronal interactions areunclear, one possibility is that the reduction in slow afterhyperpolarization,mediated by 5-HT₄ receptors, causes neuronal excitability (Torreset al., 1996) and ultimately contributes to the facilitation ofACh release. This assumption was strengthened by the present electrophysiologicalfindings that the synaptic transmission was facilitated by thestimulation of 5-HT₄ receptors: SC 53116 enhanced the populationspike amplitude in the hippocampal CA1 field. Furthermore, SC53116 potentiated the population spike amplitude not only by thetest stimulation but also by tetanization. It could not be excludedthat the tetanus-induced LTP was augmented by activation of 5-HT₄receptors, however, this facilitation appears to reflect the increasedsynaptic transmission, i.e., LTP-like effects produced by SC 53116alone. The augmentation of LTP formation induced by SC 53116,on the other hand, was prevented not only by GR 113808 but alsoby scopolamine. These findings suggest that LTP formation mediatedby 5-HT₄ receptors was, in part, regulated by muscarinic receptors.In turn, the cooperative mechanism via 5-HT₄ receptors and muscarinicreceptors may contribute to LTPinduction.

The regulation of synaptic plasticity is considered to involve the long-term modulation of ion-channel activity, therefore,the stimulation of 5-HT₄ receptors may initiate this process byactivation of adenylyl cyclase. Thus, accumulated cAMP formationstimulated by 5-HT₄ receptors leads to modulation of the activityof protein kinase A and results in closure of the potassium channels(Fagni et al., 1992). These signaling mechanisms contribute tostimulate ACh release and may result in induction of LTP. Indeed,several lines of evidence indicate that the cholinergic neuronalsystem plays an important role in plastic changes in the CA1 fieldin accordance with memory and learning. For instance, the cholinergicagonist carbachol caused a long-lasting increase in the efficacyof synaptic transmission (Blitzer et al., 1990). The cholinesteraseinhibitor physostigmine, which prevents the degradation of endogenousACh, enhanced the magnitude of LTP (Ito et al., 1987). Consistentwith previous studies (Ito et al., 1987; Hirotsu et al., 1989),the scopolamine-induced attenuation of LTP was observed in thisstudy. These findings indicate that the cholinergic system mayplay a significant role in the mechanism for the induction oflong-lasting synaptic enhancement, i.e., LTPformation.

In the present study, pretreatment with SC 53116 tended to enhance the magnitude of LTP inhibited by scopolamine, but notsignificantly. Although no correlation was established betweensynaptic plasticity and behavioral alteration, these phenomenasuggest that the stimulation of 5-HT₄ receptors are not contributedto improve the memory deficit induced by scopolamine. Indeed,the passive avoidance test showed that SC 53116 ameliorated thescopolamine-induced impairment in the training session, however,this drug failed to improve the amnesic effects induced by scopolaminein the retention test. These findings suggest that the 5-HT₄ receptorsmay participate in the learning processes when cholinergic functionwas impaired, but these receptors may have little influence onthe memory processes. The present findings did not always agreewith previous findings, which showed that BIMU 1 and BIMU 8 improvethe scopolamine-induced amnesic effect in the mouse passive avoidancetest (Galeotti et al., 1998). We cannot sufficiently explain thisdiscrepancy, however, it may be related to the differences inspecies or the selectivity of the drugsused.

Interestingly, scopolamine did not cause amnesia when administered after acquisition. These findings were in agreement witha previous study (Flrod and Buccafusco, 1988). Farr et al. (2000)also reported that intrahippocampal infusion of scopolamine followingfootshock avoidance training in a T-maze did not impair retention.In the present electrophysiological study, the suppression ofLTP induced by scopolamine was not observed when this drug wasadministered after tetanization (data not shown). An in vitrostudy using the rat hippocamal slices also showed that scopolamine,when applied for 20 min before and during the tetanus, causedsuppression of LTP, whereas LTP was induced when scopolamine appliedafter tetanus stimulation (Hirotsu et al., 1989). These findingsindicate that the memory formation and LTP induction may be associatedwith a common neuronal mechanism, at least in the cholinergicneuronal system. Indeed, Auerbach and Segal (1994) provided evidenceof a linkage between the cholinergic neuronal system and synapticplasticity in the hippocampus: the carbachol-induced slow onsetand long-lasting increases in the synaptic transmission in theCA1 hippocampal cells, which was named muscarinic long-term potentiation(LTPm), was blocked by atropine when administered before and duringapplication of carbachol. Atropine, when added after LTPm hasalready been induced, did not affect the population spikes. Thus,the activation of a muscarinic receptor may be necessary for theinduction of LTPm but not for the expression of this synapticplasticity. In addition, they proposed that LTPm shared severalproperties with tetanic-stimulated LTP and was an important linkbetween the cholinergic action and hippocampal function (Segaland Auerbach, 1997). In other words, the cholinergic neuronalsystem may play an important role in LTP induction but may beof little importance in the maintenance of LTP.

In summary, the findings of the present study revealed that 5-HT₄ receptors played a significant role in the physiologicalrelationship between the serotonergic and cholinergic systemsassociated with learning and memory. Thus, the functional roleof 5-HT₄ receptors in cognitive processes appears to require interactionwith cholinergic neurotransmission. The 5-HT₄ receptor agonists,therefore, could be useful in the treatment of cognitive deficitsby enhancement of cholinergicneurotransmission.

	Acknowledgments

We thank K. Kato and H. Hashimoto for technicalassistance.

	Footnotes

Accepted for publication November 2, 2000.

Received for publication August 8, 2000.

Send reprint requests to: Dr. Machiko Matsumoto, Department of Pharmacology, Hokkaido University School of Medicine, Kita-15, Nishi-7, Kita-ku, Sapporo 060-8638, Japan. E-mail: mbird{at}med.hokudai.ac.jp

	Abbreviations

5-HT, serotonin; SC 53116, 1-(S)-1-exo-4-amino-5-chloro-N-[(hexahydro-1H-pyrrolizin-1-yl)methyl]-2-methoxybenzamide; GR 113808, [1-[2-(methylsulphonylamino)ethyl]-4-piperidinyl]methyl-1-methyl-1H-indole-3-carboxylate; BIMU 1, endo-N-(8-methyl-8-azabicyclo[3.2.1]-oct-yl)-2,3-dihydro-3-ethyl-2-oxo-1H-benzimidazol-1 carboxamine; BIMU 8, endo-N-(8-methyl-8-azabicyclo[3.2.1]-oct-3-yl)-2,3-dihydro-(1-methyl)ethyl-2-oxo-1H-benzimidalol-1 carboxamide; RS 67333, 1-(4-amino-5-chloro-2-methoxyphenyl)-3-(1-n-butyl-4-piperidinyl)-1-propanone; RS 17017, 1-(4-amino-5-chloro-2-methoxyphenyl)-5-(piperidin-1-yl)-1-pentanone; ACh, acetylcholine; LTP, long-term potentiation; LTPm, muscarinic long-term potentiation.

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