The M1 Muscarinic Agonist CI-1017 Facilitates Trace Eyeblink Conditioning in Aging Rabbits and Increases the Excitability of CA1 Pyramidal Neurons

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The Journal of Neuroscience, January 15, 2000, 20(2):783-790

The M1 Muscarinic Agonist CI-1017 Facilitates Trace Eyeblink Conditioning in Aging Rabbits and Increases the Excitability of CA1 Pyramidal Neurons
Craig Weiss¹, Alison R. Preston¹, M. Matthew Oh¹, Roy D. Schwarz², Devin Welty², and John F. Disterhoft¹
¹ Department of Cell and Molecular Biology, Northwestern University Medical School, Chicago, Illinois 60611, and ² Parke-Davis Pharmaceutical Research, Ann Arbor, Michigan 48105

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The M1 muscarinic agonist CI-1017 was administered intravenously to aging rabbits on a daily basis before and during hippocampallydependent trace eyeblink conditioning sessions. Circulating levelsof CI-1017 were significantly related to the drug dose. The drugwas found to significantly increase the rate and amount of learningin a dose-dependent manner with no significant effects on theamplitude, area, or latency of conditioned responses. There wasno evidence of pseudoconditioning at the highest drug concentration,and the minimally effective dose produced only mild and temporaryhypersalivation as a side effect. CI-1017 (10 µM) was also foundto increase the excitability of CA1 pyramidal neurons recordedfrom hippocampal slices from young and aging naive rabbits asmeasured by changes in spike-frequency adaptation and the postburstafterhyperpolarization. These biophysical changes were reversedwith either atropine (1 µM) or pirenzepine (1 µM). These resultssuggest that M1 agonists ameliorate age-related learning and memoryimpairments at least in part by reducing the afterhyperpolarizationand spike-frequency adaptation of hippocampal pyramidal neuronsand that M1 agonists may be an effective therapy for reducingthe cognitive deficits that accompany normal aging and/or Alzheimer'sdisease.

Key words: acetylcholine; afterhyperpolarization; Alzheimer's disease; cholinesterase; hippocampus; learning

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alzheimer's disease (AD) is partially characterized by a loss of forebrain cholinergic neurons and depletion of cortical cholinergicaxons (Perry et al., 1978; Bartus et al., 1982; Whitehouse etal., 1982; Whitehouse and Au, 1986; Geula and Mesulam, 1994; Levey,1996; Robinson and Harrell, 1997). These data suggest that therapiesbased on cholinergic pharmacology might be successful at amelioratingbehavioral consequences of AD (Schwarz et al., 1997). Drugs currentlyused to treat AD (Tacrine and Donepezil) inhibit cholinesterasesand rely on the presence of cholinergic neurons, which graduallydie as the disease progresses. A therapy based on agonist replacementmay be more successful in the long term because muscarinic acetylcholinereceptors from postmortem AD brains appear to remain intact (Mashet al., 1985; Pearce and Potter, 1991), although some may be functionallydisabled (Ferrari-DiLeo et al., 1995; Flynn et al., 1995).

Successful therapies would be based on receptor activation for the afferents that are affected by the disease, i.e., the pharmacologicallyidentified M1 receptor (Hulme et al., 1990) and the geneticallyidentified m1 receptor (Bonner et al., 1987). The highest concentrationof M1 receptors is in the dentate gyrus (Messer and Hoss, 1987),and the m1 receptor is highly concentrated in cortex, hippocampus,and striatum. All five receptor types (m1-m5) are coupled to G-proteins,and m1, m3, and m5 receptors activate phospholipase C, which inturn activates diacylglycerase, IP₃, and protein kinase C. Thissequence of events is often associated with increased neural plasticity,including acquisition of trace eyeblink conditioning (EBC) inthe rabbit (Van der Zee et al., 1997). Furthermore, scopolamine(a muscarinic antagonist) disrupts trace EBC (Kaneko and Thompson,1997), and the M1 antagonist pirenzepine disrupts other learningparadigms (Caufield et al., 1983; Hagan et al., 1987; Messer etal., 1987; Bymaster et al., 1993; Ohno et al., 1994).

CI-1017 is a second generation agonist designed to selectively activate the M1 receptor while minimizing peripheral side effects(Tecle et al., 1998). It is an oxime of 1-azabicyclo[2.2.1] heptan-3-onewith a 3-phenylpropargyl analog substituent, and it is identifiedas a relatively m1-selective partial agonist by cell metabolism,cell amplification, and second messenger assays with an overallselectivity of m1 $>=$ m4 >m3 = m5 $>>$ m2 (Jaen et al., 1995).

The aim of this study was to determine whether CI-1017 would significantly improve the learning rate of aging rabbits duringtrace EBC. This is an interesting task to examine because it ishippocampally dependent in rabbits (Solomon et al., 1986; Moyeret al., 1990; Kim et al., 1995) and humans (Disterhoft et al.,1996a; McGlinchey-Berroth et al., 1997), and it is significantlyimpaired by aging (Disterhoft et al., 1995; Thompson et al., 1996a)and AD (Woodruff-Pak et al., 1990; Solomon et al., 1991, 1995;Woodruff-Pak and Papka, 1996). Improved acquisition of EBC byaging rabbits (Kronforst-Collins et al., 1997), with concomitantenhancement of neuronal excitability (Oh et al., 1999), was demonstratedpreviously with the cholinesterase inhibitor metrifonate. We nowdemonstrate both facilitation of EBC and increased hippocampalCA1 pyramidal neuron excitability with the muscarinic agonistCI-1017.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects and surgery. Subjects in the behavioral pharmacology experiment were 26 New Zealand White female rabbits that were30 or 36 months of age at the start of the experiment. Surgeryto implant a femoral catheter, vascular access port, and atraumatichead restraint was done using sterile procedures approved by theNorthwestern University Animal Care and Use Committee. Rabbitswere anesthetized with ketamine (45 mg/kg) and xylazine (7.5 mg/kg),and the scalp, back, and groin were shaved and cleaned with alcoholand betadine. A midline incision was made along the back, anda pocket was formed by cutting any subdermal adhesions. A vascularaccess port (GPV-4S-24 or TI200-4S; Access Technologies, Skokie,IL) was filled with heparinized saline, placed within the pocket,and sutured in place to the underlying muscle. An incision wasalso made inside the groin, and a long forceps was used to tunnelunder the skin and lead the catheter attached to the vascularaccess port (venaport) to the femoral region. The wound for thevenaport was cleaned with betadine and sutured shut with 4-0 nylon.The femoral vein was exposed, cleared of adhering tissue, andpunctured with a catheter introducer (#6999; Becton Dickinson,Franklin Lakes, NJ). The catheter was inserted into the vein,advanced ~10 cm, and sutured into place with silk stays and 4-0nylon. The wound was then cleaned and closed with 4-0nylon.

The rabbit was placed within a stereotaxic device to restrain the head. The scalp was cleaned, and a midline incision wasmade to expose bregma and lambda. The periosteum was scraped away,the skull was cleaned with betadine and hydrogen peroxide, andfour holes were made to receive self-tapping stainless steel screws.The screws and skull were covered with dental acrylic, and a restrainingdevice containing four nylon bolts (6-32 × 3/4 inch) was placedwithin the cement. The wound was then cleaned, and the rabbitwas placed on a warming pad to recover. The rabbit was given Buprenex(0.4 mg/kg) for analgesia when it was ambulatory, and it was returnedto its homecage.

The venaport in each rabbit was injected daily with 0.3 ml of heparinized saline to keep the port and catheter patent. Rabbitswere given a minimum recovery time of 1 week and were then broughtto the laboratory for daily eyeblink conditioning sessions. Rabbitswere placed within a cloth bag that was tied at the neck and tail,placed within a Plexiglas box that had a yoke surrounding theneck, and the lids of the right eye were held open with dresshooks and Velcro (Disterhoft et al., 1977). The rabbit was placedwithin a sound attenuating chamber, the nylon restraining boltswere fastened to a rigid support, and an infrared reflective sensorand air puff delivery tube were placed in front of the right eye(Thompson et al., 1994). The rabbits were habituated to the restrainingdevice and conditioning chamber for 2-5 d daily before receivingany conditioningstimuli.

Drug delivery. Rabbits received CI-1017 (which was provided by Parke-Davis, Ann Arbor, MI) or vehicle (0.9% saline) as ofthe first day of conditioning. The rabbits were randomly dividedinto four groups of 5.0, 1.0, 0.5, and 0.0 mg/ml, and the experimenterwas blinded to the dose. The rabbits had a mean weight of 4.15kg (range of 3.2-4.7 kg). Each rabbit was given 0.6 ml of thedrug over the course of 1 min (0.3 ml to flush the catheter ofheparinized saline and a bolus of 0.3 ml to raise the plasma levelof the drug quickly) and then infused with the drug at a rateof 2.7 ml/hr. Conditioning trials began 30 min after the startof the infusion, and the infusion continued for the duration ofeach daily session. The nominal loading dose was thus 0.361, 0.072,0.036, or 0.0 mg/kg, and the nominal maintenance dose was 3.25,0.65, 0.325, or 0.0 mg · kg¹ · hr¹.

Blood sampling. Blood samples were taken from the marginal ear vein of all rabbits immediately after training on trainingday 10. The samples were mixed with heparin and centrifuged at3000 rpm for 5 min at 4°C. The plasma was then removed and storedat $-$ 80°C until it was analyzed for circulating levels of CI-1017.

Behavioral training. The conditioning task involved pairing a tone (100 msec, 6 kHz, 90 dB, 5 msec rise-fall time) with anair puff to the eye (150 msec, 3 psi). A 500 msec stimulus-freetrace period separated the tone and air puff to make the taskdependent on the hippocampus (Moyer et al., 1990). A computercontrolled delivery of the stimuli and recording of the behavior(Akase et al., 1994). This frequency of the conditioning stimulus(CS) is optimal for the rabbit auditory system (Martin et al.,1980) and was delivered by headphones to the ear canal via rubbertubing. The unconditioned stimulus (US) was an air puff that wasadequate to evoke extension of the nictitating membrane (NM).The air puff was supplied by compressed air and controlled bya regulator and solenoid valve. Movement of the NM was transducedby an infrared sensor, which converts a change in reflectancefrom the cornea to a change in voltage (Thompson et al., 1994).

Training sessions were conducted while the rabbits were restrained in a cloth bag and Plexiglas box. They received one sessionper day with each session consisting of 80 presentations of thepaired stimuli. Trials were separated by a random intertrial interval(ITI) of 30-60 sec. Conditioned responses (CRs) were defined asextensions of the NM that exceeded the mean baseline amplitudeby 4 SDs for a minimum of 10 msec. Most rabbits were conditionedwith the trace conditioning paradigm for 15 d (3 weeks of 5 d)and then with delay conditioning (750 msec tone, 150 msec coterminatingair puff) for 5 d. Some rabbits were trained for 20 d with traceconditioning and 5 d with delay conditioning. All rabbits weregiven a sixth day of delay conditioning with attenuated tonesto detect their sensitivity to theCS.

Behavioral control sessions (n = 15) were given to an additional 12 rabbits (six with vehicle and six with 5.0 mg/ml) to testfor pseudoconditioning and sensitization. These sessions consistedof 80 trials with tones and 80 trials with air puffs. The twotypes of trials were presented in random order with a 15-30 secITI. These rabbits were then switched to the delay paradigm forfive dailysessions.

Behavioral data analysis. The data were analyzed with ANOVA that used drug dose as a group variable and daily scores as arepeated measure. These scores included the percent of trialswith CRs, the peak amplitude of CRs, the area of CRs (the sumof the amplitudes for each sample during the CS-US period), thelatency to the peak of the CR, and the average amplitude of theunconditioned response (UR). Post hoc tests of significance (p $equal$ 0.05) were performed using Fisher's least significance differencetest. Analyses were performed using StatVIEW 4.1 (SAS Institute,Cary, NC) on a Macintosh PowerPC computer (Apple Computers, Cupertino,CA).

Biophysical recordings. The effects of CI-1017 on the biophysical properties of CA1 pyramidal neurons from hippocampal slicesfrom six young (2-3 months) and seven aging (31-38 months) naiverabbits were examined. The tissue preparation and current-clampintracellular recording techniques have been described previously(Oh et al., 1999). Briefly, rabbits were deeply anesthetized withhalothane, and the brain was extracted within 1 min of death.Hippocampal slices (300 µm) were made using a vibratome and thenplaced in a holding chamber at room temperature (22°C) for atleast 45 min before being transferred to the submersion chamber(Harvard Apparatus, Holliston, MA) forrecording.

Biophysical measurements [postburst afterhyperpolarization (AHP), spike-frequency adaptation (accommodation), input resistance,and resting membrane potential] were recorded. A burst of fouraction potentials was used to examine the AHP, and an 800 msecpulse at the same current was used to examine accommodation. CA1neurons were included in the study if the neurons had little spontaneousactivity at rest, a stable resting membrane potential less than $-$ 60 mV, an action potential duration >1.2 msec from rise thresholdto recrossing the resting potential, an input resistance >20 M $Omega$ ,and an action potential amplitude >80 mV from rest. Biophysicalproperties were measured at least 5 min after the initial impalement.The neurons were held near $-$ 70 mV (using less than ±0.2 nA) toensure that any effects were not attributable to voltage-dependentmembrane properties (Oh et al., 1999). The following sequenceof biophysical recordings was used: (1) baseline measurementsrecorded in artificial CSF (aCSF); (2) measurements in aCSF containing10 µM CI-1017; and (3) measurements in aCSF containing 10 µM CI-1017and either 1 µM atropine (to test for reversal of a cholinergiceffect; Sigma, St. Louis, MO) or 1 µM pirenzepine (a specificM1 antagonist; Sigma). The neurons were allowed to stabilize for10 min at $-$ 75 mV (or at rest if the membrane potential was lessthan $-$ 75 mV) during each change in perfusate. Data from the biophysicalmeasurements were analyzed with a repeated-measures ANOVA andFisher's PLSD test. The mean ± SE values of the measures arereported.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Behavior

The behavioral results are based on data from 23 conditioned rabbits and 12 control rabbits. There were three other conditionedrabbits that were excluded from the analyses: one did not exhibitany startle responses, indicating it was deaf, and two failedto show CRs even during simple delay conditioning, which suggesteda generalized functional impairment including the cerebellum andassociated brainstem circuitry. There were four, seven, five,and seven rabbits that completed at least 15 d of trace conditioningin the 0.0, 0.5, 1.0, and 5.0 mg/ml groups, respectively. All12 control rabbits completed the study and exhibited CRs afterthey were switched to a delay conditioningparadigm.

An ANOVA for the percent of trials with CRs during 15 d of conditioning indicated that there was a significant effect of dose(F_(3,19) = 4.92; p = 0.011), a significant increase in CRs acrossdays of training (F_(14,266) = 26.27; p < 0.0001), and a significantinteraction between the two factors (F_(42,266) = 1.78; p = 0.004).A graph of these results is shown in Figure 1A. The 5.0 mg/mlgroup exhibited the greatest level of conditioning (66.8 ± 8.2%on day 10) and attained this level more quickly than the othergroups attained their peak level of CRs. The vehicle control rabbitsdid not exhibit their maximum of 44 ± 8.8% CRs until day 15.

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Figure 1. A, A graph of the percent of trials with CRs across 15 daily training sessions as a function of drug dose. B, The two higher doses (5 and 1 mg/ml) exhibited significantly more CRs than the two lower doses (0 and 0.5 mg/ml). Data are means ± SE. Error bars are omitted from A for clarity.

Post hoc tests indicated that the high-dose set (1.0 and 5.0 mg/ml groups) exhibited significantly more CRs than the low-doseset (0.0 and 0.5 mg/ml groups), and there was no significant differencebetween each of the two groups within the high- or low-dose sets.Figure 1B presents the increase in percent CRs as a function ofhigh- or low-dose sets to show the effect of the drug more clearly.The interaction of dose and sessions appears to be due to themore rapid increase in the percent of trials with CRs for thehigh-dose set compared with the low-dose set. This increase persistedfor the duration of the experiment so that the high-dose set consistentlyoutperformed the low-dose set (Fig. 1B). The two sets of rabbitswere significantly different from each other on the first dayof conditioning and on all subsequent days, except days 2 and6.

Some of the rabbits (19 of 23) were conditioned for 20 d instead of 15 d. An ANOVA for this group of rabbits produced thesame set of significant results as presented above. The resultsalso indicated that the performance of the 5.0 mg/ml group continuedto improve beyond day 15 (day 19, 77.8 ± 7.2% CRs), whereas theperformance of the 1.0 mg/ml group plateaued between days 15 and17 and then decreased to a level about that of day 10 (day 20,46.6 ± 11.2%CRs).

The CRs of the conditioned rabbits improved in quality, as well as in frequency of occurrence. An ANOVA for the peak amplitudeof the CR (on trials in which there was a CR) indicated a significantincrease in amplitude over the course of training (F_(14,266) =2.64; p = 0.001). There was no significant difference among thedose groups and no significant interaction of dose and session.A graph of the increase in the peak CR amplitude is shown in Figure2A.

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Figure 2. A, A graph of the peak amplitude of response during the CS-US period on trials in which there was a CR. B, A graph of the area of response during the CS-US interval on trials in which there was a CR. C, A graph of the mean amplitude of response during the UR period. There was a significant increase in all three measures across sessions, but no significant differences among the groups and no significant interaction of dose and session were found. A comparison of these data with those in Figure 1 indicate that the high-dose rabbits showed more CRs, rather than CRs with different characteristics. The y-axis is shown in integrated units.

An ANOVA of the area of response on trials in which there was a CR indicated that there was a significant increase over thecourse of training (F_(14,266) = 4.12; p < 0.001). There was nosignificant difference among the dose groups and no significantinteraction of dose and session. A graph of the increase in thearea of response is shown in Figure 2B.

An ANOVA of the latency to the peak of the response during the CS-US period on trials in which there was a CR indicated thatthere was a significant interaction of dose and session (F_(42,266)= 2.22; p < 0.0001). The interaction was apparently caused byshorter latencies for the control group during the first threesessions (170 msec). There were no significant main effects ofdose or session. The mean latency to the peak of the CR duringsessions 11-15 for all groups combined was 454.3 msec (air puffonset was at 600 msec). There were no significant differencesrevealed by an ANOVA when the groups were combined into two groupsof high and lowdose.

The UR was also examined for changes in amplitude. An ANOVA indicated that there was a significant increase in the mean amplitudeof response across sessions during the UR period (F_(14,42) = 3.73;p < 0.0001). This increase is shown in Figure 2C and most likelyreflects the presence of reflex facilitation and/or long-durationCRs that added to the UR (see Discussion). There was no significanteffect of dose and no significant interaction of dose and session.In fact, there was no significant difference between the two dosesets on any day of conditioning, including the first day whenthere was the least chance of contamination by a CR. The UR wasalso examined on air puff alone trials (during the last day oftraining with attenuated tones) to avoid contamination by theCR. A t test for the effect of the drug indicated no significantdifference in the peak amplitude of the UR between the high- andlow-dose sets (1409 ± 223 integrated units vs 1834 ± 130 integratedunits,respectively).

Pseudoconditioning controls

The possibility of pseudoconditioning or sensitization was examined among the behavioral control rabbits with an ANOVA usingdose as a grouping variable and percent of trials with CRs ontone alone trials as a repeated measure. The results indicatedthat there was no significant change in percent CRs across trainingsessions, and there was no significant difference between rabbitsthat received either vehicle or the highest dose of CI-1017 (5mg/ml). The behavioral control rabbits had a mean of 13.9 ± 0.88%CRs for all rabbits combined. These results are shown in Figure3A.

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Figure 3. A, CI-1017 had no significant effect on the percent of trials with apparent CRs during 15 behavioral control sessions that presented unpaired tones and air puffs, i.e., there was no pseudoconditioning. B, CI-1017 had no significant effect on the rate of learning when the same rabbits were subsequently switched to the delay conditioning paradigm for five daily sessions. D, Drug at 5 mg/ml; V, vehicle control.

An ANOVA on the mean amplitude of the UR also failed to show either a significant difference between the drug and vehiclegroups or a significant interaction between the group effect anddays of training. There was a significant increase in the UR amplitudeacross days (F_(14,140) = 3.5), but this effect appeared to bedue to the increase in UR amplitude from day 1 to day 2. The effectwas no longer significant when day 1 was excluded from theanalysis.

The control rabbits were then switched to a delay conditioning paradigm for 5 training days by extending the duration of theCS until it coterminated with the US, i.e., a 750 msec CS. AnANOVA of drug group by training session indicated that there wasa significant increase in CRs across sessions (F_(4,40) = 9.0;p < 0.0001) but no significant difference between the controland CI-1017 groups. These data are shown in Figure 3B. The largestdifference between the groups occurred on the first day of delaytraining; the control rabbits had 26 ± 12% CRs and the CI-1017rabbits had 13 ± 4% CRs. The mean maximum daily percent CRs was59.8 ± 13.8% for the control rabbits and 60.2 ± 10.6% for therabbits receiving 5 mg/ml CI-1017.

Side effects

Notable side effects of the drug were observed in the highest dose group (5 mg/ml). This group demonstrated considerable andpersistent salivation, increased likelihood of defecation, andan increase in arousal to occasional noises in the laboratory.Salivation in the highest dose group prevented the experimenterfrom being completely blind to this dosing group. It was persistentduring and across sessions and began soon after the loading bolusinjection. The salivation effect was more variable in the 1.0mg/ml group and nonexistent in the two lower dose groups. Defecation(which was apparently related to the training sessions) only occurredin rabbits on the highest dose (5 mg/kg). It was noted in fourof seven rabbits on the first day, and it persisted throughoutthe experiment for two of the fourrabbits.

Rabbits were examined for their auditory sensitivity on the last day of training (day 6 of delay conditioning) to systematicallytest for an increase in auditory-mediated arousal. They were giventwo sets of five trial blocks with paired presentations of theCS and US in which the tone was attenuated between 0 and 30 dBin 5 dB steps (two blocks of air puff alone trials were also given).Data from the rabbits that were originally trained with traceconditioning were analyzed with an ANOVA for the percent of trialswith CRs by dose (high or low) and the amount of attenuation.The results indicate a significant effect of dose (F_(1,14) = 12.52;p = 0.003) and attenuation (F_(6,84) = 20.04; p < 0.0001) but nosignificant interaction. Rabbits in the high-dose set had significantlymore CRs than those in the low-dose set just as they did duringtrace EBC training sessions. Both groups showed equivalent declinesin responding as the CS amplitude was attenuated, as indicatedby the lack of interaction in the ANOVA. The results for rabbitsthat started as behavioral controls for pseudoconditioning alsoindicate that the vehicle group had significantly fewer CRs thanthose receiving 5 mg/ml (F_(1,10) = 7.7; p = 0.02) and that bothgroups combined had a significant decline in percent CRs withincreasing attenuation (F_(6,60) = 7.1; p < 0.0001). There wasno significant interaction of the drug and attenuation for thisgroup of rabbits either. In fact, the rate of decline with increasingattenuation was quite similar between the high- and low-dose druggroups.

Blood analysis for CI-1017

Approximately 1 ml of blood was collected from the marginal ear vein immediately after the session on day 10. The plasma wastaken and analyzed for circulating levels of CI-1017. The resultsindicate a high correlation of delivery dose and plasma concentrationof CI-1017 (r² = 0.92) for the conditioned rabbits. Furthermore, an ANOVA indicateda significant effect of dose on plasma concentration (F_(3,19)= 100.1; p < 0.0001) with the 5 mg/ml dose having significantlygreater levels of CI-1017 than the 1.0 and 0.5 mg/ml groups (622± 46 vs 102 ± 16 and 58 ± 7 ng/ml). There were no significantdifferences among the other doses. The analysis also indicatedthat the behavioral control rabbits receiving 5 mg/ml had a meanof 623 ± 79 ng/ml.

The day 10 plasma concentration of CI-1017 was then compared with the percent of trials with CRs on day 10 for the high- andlow-dose sets of conditioned rabbits. The results indicate thatthe low-dose set had a mean CI-1017 plasma level of 46.4 ± 7.2ng/ml and a mean of 25.1 ± 5.8% CRs. The high-dose set of rabbitshad a mean CI-1017 plasma level of 405.2 ± 81.8 ng/ml and a meanof 54.9 ± 6.4% CRs. A regression analysis of the combined data(high- and low-dose sets) indicated that the data could be fitwith a second-order polynomial. That equation indicated a correlationcoefficient of 0.69 (r² = 0.48), a Y intercept of 20.0% CRs, and a peak effect that wouldoccur at 67.4% CRs and 595.3 ng/ml.

In vitro physiology

The effects of CI-1017 were examined in eight CA1 hippocampal neurons from five young naive rabbits, and in 12 neurons fromseven aging naive rabbits. A repeated-measures ANOVA (with posthoc PLSD tests) indicated that bath application of the drug (10µM) significantly reduced both the mean amplitude of the postburstAHP (F_(1,18) = 51.0; p < 0.0001) and spike-frequency accommodation(F_(1,17) = 58.8; p < 0.0001). The area (F_(1,18) = 32.3; p < 0.0001)and duration (F_(1,18) = 42.4; p < 0.0001) of the AHP were alsosignificantly reduced by CI-1017 (data not shown). There was nosignificant effect of age on the AHP, in contrast with our previousreports (Moyer et al., 1992; Disterhoft et al., 1996b; Oh et al.,1999) apparently because of the small sample size in this study.There also was no significant interaction of age with applicationof thedrug.

The effect of CI-1017 on the mean amplitude of the AHP and on accommodation is shown in Figure 4. These effects were reversedby the addition of the general muscarinic antagonist atropine(1 µM; in four young cells) or the specific M1 antagonist pirenzepine(1 µM; in nine aging cells). Fisher's PLSD test for the 13 cellscombined revealed that the AHP (p = 0.0003), accommodation (p< 0.0001), AHP area (p = 0.0005), and AHP duration (p < 0.0001)were all significantly reversed by the muscarinic antagonists.Examples of the effect of CI-1017 on a single hippocampal neuronare shown in Figure 5. Reversal of the effects by atropine indicatesthat CI-1017 acts primarily by enhancing the effect of muscariniccholinergic neurotransmission.

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Figure 4. CI-1017 increased the excitability of both young and aging hippocampal pyramidal neurons by significantly reducing the amplitude of the AHP and spike-frequency adaptation. A, CI-1017 (10 µM) significantly reduced the mean amplitude of the AHP in neurons from aging rabbits, and the effect was significantly reversed after application of the m1-specific antagonist pirenzepine (1 µM). B, CI-1017 significantly reduced the spike-frequency adaptation of neurons from aging rabbits after application of the drug (10 µM) to the bath; the effect was significantly reversed by the addition of pirenzepine (1 µM). C, CI-1017 (10 µM) reduced the mean amplitude of the AHP in neurons from young rabbits; the effect was reversed after application of the cholinergic antagonist atropine (1 µM). D, CI-1017 (10 µM) significantly reduced the spike-frequency adaptation of neurons from young rabbits; the effect was significantly reversed by the addition of atropine (1 µM).

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Figure 5. Typical examples of the effects of CI-1017 on biophysical properties from a single hippocampal CA1 pyramidal neuron from a young naive rabbit. An 800 msec pulse was used to examine accommodation after a burst of four action potentials. A, Accommodation of the neuron in aCSF. B, Accommodation is reduced by the addition of CI-1017, i.e., the cell is more excitable. C, The excitability change due to CI-1017 is reversed by the addition of the muscarinic antagonist atropine. D, Examples of the postburst AHP during control (aCSF), drug (CI-1017), and reversal (CI-1017 plus atropine) conditions.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The M1 agonist CI-1017 significantly increased the learning rate of aging rabbits during hippocampally dependent trace eyeblinkconditioning. The increase was seen at an intravenous dose aslow as 1.0 mg/ml, and rabbits that received 5.0 mg/ml did notshow significantly better learning than rabbits in the 1.0 mg/mlgroup (although the 5 mg/ml group reached their maximum more quicklythan the 1 mg/ml group). The increase in the percentage of CRsfor the two highest dose groups occurred without significant changesin the quality of the CR, i.e., there was no significant effectof dose on amplitude, area, or latency of the conditioned response.These parameters did improve over the course of training sessionsas rabbits acquired the task, but dose was not a significant factor,and there was no significant interaction of dose and session.Furthermore, there was no evidence of pseudoconditioning. Thus,these data suggest that CI-1017 acts on associative sites to increasethe probability of evoking a CR and not on unconditioned reflexsites. These effects are similar to those observed in aging rabbitstreated with the cholinesterase inhibitor metrifonate (Kronforst-Collinset al., 1997). A previous study had demonstrated that rabbitsreceiving oral doses of CI-1017 (Kronforst-Collins, 1998) didnot exhibit a significant increase in CRs relative to controls.Thus, oral administration of the drug appears not to be idealinrabbits.

The amplitude of the UR was found to increase during paired trials across sessions. This was likely to be due to either increasedreflex facilitation produced by the combined presentation of theCS and US as the CS gained increased salience across trainingsessions (Harvey et al., 1985; Weisz and LoTurco, 1988) or toan increase in the duration of the CRs. We cannot be certain whethereither, or both, effects were occurring because neither air puffalone trials nor tone alone trials were presented during the dailysessions. However, the results from air puff alone trials presentedon the last day of training indicated that there was no significanteffect of the drug on the UR. This, and the lack of pseudoconditioning,suggests that direct activation of the UR pathway was not significantlycontributing to the increase inCRs.

The effects of CI-1017 should be generalized to other learning paradigms if it is acting at M1/m1 cholinergic synapses throughoutthe brain. CI-1017 has in fact been shown to improve learningin other tasks in rodents and nonhuman primates. At an oral doseof 1.0 mg/kg (p.o.), it significantly shortened the latency ofC57BL/10SnJ mice to find a hidden platform in the Morris watermaze (Symons et al., 1988; Schwarz et al., 1997). These mice havesmall hippocampi and decreased numbers of pyramidal neurons. Thedrug (0.1 mg/kg, p.o.) also improved water maze performance inrats with ibotenic acid lesions of forebrain cholinergic neuronswhen compared with sham-lesioned controls, and it improved theperformance of adult rhesus monkeys (0.32 mg/kg, i.m.) on a continuousperformance task after the administration of scopolamine (Schwarzet al., 1997). Another M1 agonist, AF102B, has also been shownto be effective in a single-blind placebo-controlled study usingpatients with probable AD (Fisher et al., 1996).

In contrast to the facilitating effects of CI-1017 on learning, the M1 antagonist pirenzepine has been shown to have disruptiveeffects. It was found to impair acquisition of inhibitory avoidancein mice (Caufield et al., 1983), increase the water maze escapelatency in rats after intracerebroventricular injections (Haganet al., 1987; Hunter and Roberts, 1988), disrupt representationalmemory in rats (Messer and Hoss, 1987; Messer et al., 1987, 1990),and impair working memory in rats given 1 µg/side intrahippocampally(Ohno et al., 1994). Pirenzepine was also very effective in blockingthe effects of CI-1017 on the AHP and spike-frequency accommodationof hippocampal pyramidalneurons.

The mechanism of action for CI-1017 is believed to involve M1/m1 receptors at central cholinergic synapses, particularly withinthe cortex and hippocampus. This was directly tested here by makingintracellular recordings from CA1 pyramidal neurons in hippocampalslices from young and aging naive rabbits. The results indicatethat CI-1017 significantly increased the excitability of CA1 hippocampalneurons, i.e., it reduced spike-frequency adaptation and the postburstAHP. The effect was very robust at a concentration of 10 µM andreached statistical significance when evaluated in relativelyfew cells. The effect was present but less pronounced at a concentrationof 1 µM (data not shown), and it was reversed by the additionof atropine or pirenzepine to 10 µM CI-1017, indicating the expectedmuscarinic mode ofaction.

Several in vitro experiments have demonstrated that application of ACh, muscarinic agonists, or anticholinesterases increaseneuronal excitability (reduced AHP and accommodation) of hippocampalpyramidal neurons (Benardo and Prince, 1981, 1982; Cole and Nicoll,1983, 1984a,b; Madison and Nicoll, 1984; Halliwell, 1990; Pedarzaniand Storm, 1996; Oh et al., 1999). Furthermore, both the AHP andaccommodation were reduced in CA1 neurons from young and agingrabbits that acquired eyeblink conditioning but not in trainedrabbits that did not learn (Disterhoft et al., 1986, 1988, 1996b;Coulter et al., 1989; de Jonge et al., 1990; Moyer et al., 1992,1996; Thompson et al., 1996b). Both the AHP and accommodationare greater in CA1 neurons from aging rabbits (Moyer et al., 1992;Oh et al., 1999) and rats (Landfield and Pitler, 1984; Potieret al., 1992) compared with those from young animals. We haveshown previously that two drugs that increase conditioning ratein aging rabbits, nimodipine (Deyo et al., 1989; Kowalska andDisterhoft, 1994) and metrifonate (Kronforst-Collins et al., 1997),both enhance CA1 neuronal excitability when applied in vitro (Moyeret al., 1992; Oh et al., 1999). These findings, along with thosesummarized here, suggest that aging rabbits may learn better ifhippocampal neuronal excitability is enhanced to become similarto that of neurons from young rabbits as a result of drugapplication.

Although metrifonate (a cholinesterase inhibitor) and CI-1017 (an M1 agonist) produced similar results during eyeblink conditioningin aging rabbits, the mechanism of action for CI-1017 appearstheoretically more favorable for the treatment of AD because ofits specificity for M1 receptors. The secondary consequences ofactivating m1 and m3 receptors are also more positive in lightof the relationship of $beta$ amyloid deposition and AD (Robinson andHarrell, 1997), i.e., activation of cell surface receptors thatare positively coupled to phospholipase C, including m1 and m3,results in increased release of soluble amyloid precursor protein(Nitsch et al., 1992; Hung et al., 1993) and a reduction in $beta$ amyloid peptide observed in vitro (Buxbaum et al., 1992; Nitschet al., 1992; Hung et al., 1993). This suggests that, in additionto alleviating cognitive symptoms of the disease, m1 receptoractivation may interfere with $beta$ amyloid formation, the ratio ofsoluble to amyloidogenic fragments produced in the brain, andslow the disease processitself.

  FOOTNOTES

Received Feb. 4, 1999; revised Oct. 21, 1999; accepted Oct. 21, 1999.

This work was supported by Parke-Davis Pharmaceutical Research and National Institutes of Health Grants R37 AG08796 and 1F31MH11737. We thank Sarah Gardiner, Mark Crowe (Access Technologies),Elke Lipka, Karen Boszor, and MatthewWeiss.
Correspondence should be addressed to Dr. Craig Weiss, Department of Cell and Molecular Biology, W129, Searle Building, Room4-445, Northwestern University Medical School, Chicago, IL 60611.E-mail: cweiss{at}nwu.edu.

A.R.P.'s present address: Department of Psychology, Stanford University, Stanford, CA94305.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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