Increased Excitability of Aged Rabbit CA1 Neurons after Trace Eyeblink Conditioning

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The Journal of Neuroscience, July 15, 2000, 20(14):5476-5482

Increased Excitability of Aged Rabbit CA1 Neurons after Trace Eyeblink Conditioning
James R. Moyer Jr, John M. Power, Lucien T. Thompson, and John F. Disterhoft
Department of Cell and Molecular Biology and the Institute for Neurosciences, Northwestern University Medical School, Chicago, Illinois 60611-3008

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cellular properties of CA1 neurons were studied in hippocampal slices 24 hr after acquisition of trace eyeblink conditioningin young adult and aging rabbits. Aging rabbits required significantlymore trials than young rabbits to reach a behavioral criterionof 60% conditioned responses in an 80 trial session. Intracellularrecordings revealed that CA1 neurons from aging control rabbitshad significantly larger, longer lasting postburst afterhyperpolarizations(AHPs) and greater spike frequency adaptation (accommodation)relative to those from young adult control rabbits. After learning,both young and aging CA1 neurons exhibited increased postsynapticexcitability compared with their respective age-matched controlrabbits (naive and rabbits that failed to learn). Thus, afterlearning, CA1 neurons from both age groups had reduced postburstAHPs and reduced accommodation. No learning-related differenceswere seen in resting membrane potential, membrane time constant,neuron input resistance, or action potential characteristics.Furthermore, comparisons between CA1 neurons from trace-conditionedaging and trace-conditioned young adult rabbits revealed no statisticallysignificant differences in postburst AHPs or accommodation, indicatingthat similar levels of postsynaptic excitability were attainedduring successful acquisition of trace eyeblink conditioning,regardless of rabbit age. These data represent the first in vitrodemonstration of learning-related excitability changes in agingrabbit CA1 neurons and provide additional evidence for involvementof changes in postsynaptic excitability of CA1 neurons in bothaging andlearning.

Key words: aging; afterhyperpolarization; spike frequency adaptation; associative learning; hippocampus; in vitro; intracellular

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aged animals, including humans, are impaired in a variety of learning tasks (Zyzak et al., 1995; Thompson et al., 1996). Weadopted the rabbit eyeblink preparation as a model system in whichto study neurobiological correlates of aging and associative learning(Disterhoft et al., 1977; Akase et al., 1989; Moyer et al., 1990;Thompson et al., 1992, 1996a; McEchron and Disterhoft, 1999).Aging rabbits require significantly more trials to learn traceeyeblink conditioning than young adult rabbits (Graves and Solomon,1985; Thompson et al., 1996a). Unlike standard delay conditioning(Akase et al., 1989), trace eyeblink conditioning depends notonly on brainstem-cerebellar circuitry but also on an intact hippocampusfor successful acquisition (Moyer et al., 1990; Kim et al., 1995).Trace eyeblink conditioning deficits exhibited by aging rabbitsparallel the deficits observed in hippocampectomized adult rabbits;both groups are profoundly impaired and show inappropriate timingof the few conditioned responses (CRs) elicited during training(Moyer et al., 1990; Thompson et al., 1996a). These data suggestthat at least part of the deficit exhibited by aging rabbits involvesimpaired hippocampalfunction.

Hippocampal slices are a valuable tool for studying various aspects of cellular neurophysiology. Using intracellular recordings,we previously demonstrated that aging rabbit CA1 neurons had bothlarger postburst afterhyperpolarizations (AHPs) (Moyer et al.,1992) and prolonged calcium action potentials (APs) (Moyer andDisterhoft, 1994) than young adult neurons. These differencesin calcium-mediated processes are similar to those observed inaging rat CA1 neurons (Landfield and Pitler, 1984; Pitler andLandfield, 1990). In addition, calcium-dependent synaptic plasticityis altered in aging hippocampal neurons (Norris et al., 1996,1998; Shankar et al., 1998), suggesting that one of the consequencesof brain aging in mammals may be an impaired ability to modulateintracellular calcium (Landfield, 1987; Disterhoft et al., 1994a;Khachaturian, 1994; Thibault and Landfield, 1996).

Blockade of excess calcium influx has been shown to ameliorate age-related learning deficits. For example, the dihydropyridinecalcium channel antagonist nimodipine facilitates acquisitionof trace eyeblink conditioning in aging rabbits (Deyo et al.,1989; Straube et al., 1990; Kowalska and Disterhoft, 1994). Intravenousadministration of the same dose of nimodipine that facilitateslearning also increases spontaneous firing rates of aging rabbitCA1 neurons in vivo (Thompson et al., 1990). Subsequent in vitrostudies showed that postsynaptic excitability of aging CA1 neuronscan be restored to levels more closely resembling young adultneurons by bath application of nanomolar concentrations of nimodipine(Moyer et al., 1992; Moyer and Disterhoft, 1994). Together, thesedata suggest that reducing calcium influx in aging CA1 neuronsnot only alters their electrophysiological properties but alsofacilitates the ability of aged animals tolearn.

Previous studies have demonstrated that ion channels can be modulated by associative learning (Alkon, 1984; Disterhoft etal., 1986; de Jonge et al., 1990; Woody et al., 1991; Moyer etal., 1996; Thompson et al., 1996b; Saar et al., 1998). For example,learning-specific reductions of the calcium-dependent slow AHPhave been observed in CA1 and CA3 neurons after acquisition ofhippocampally dependent trace eyeblink conditioning (Moyer etal., 1996; Thompson et al., 1996b). Furthermore, the reduced AHPsobserved after learning are transient, decaying back to baselinewithin 5-7 d, a time period appropriate for memory consolidation(Moyer et al., 1996; Thompson et al., 1996b). Similarly, reducedAHPs were observed in layer II pyramidal neurons of rat piriformcortex after acquisition of an odor discrimination task (Saaret al., 1998). To date, no studies have used intracellular recordingsin vitro to evaluate learning-related changes in postsynapticexcitability of CA1 neurons in aging animals. To evaluate whetherlearning-related changes also occur in aging animals, intracellularcurrent-clamp recordings were made from CA1 pyramidal neuronsin slices taken from aging rabbits after acquisition of traceeyeblink conditioning. These data were compared with data obtainedfrom aging control rabbits that did not learn, from aging naiverabbits, and similar data from young adultrabbits.

Parts of this paper have been published previously in abstract form (Disterhoft et al., 1994b).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Behavioral training. New Zealand albino rabbits (Oryctolagus cuniculus) were purchased from Hazelton Rabbitry (Denver, PA)and maintained in accordance with guidelines established by theUnited States Department of Agriculture and approved and managedby the Animal Care Committee of Northwestern University. Rabbitsreceived 500 msec trace eyeblink conditioning as described previously(Moyer et al., 1990; Thompson et al., 1996a). Briefly, rabbitswere fitted with restraining head bolts and trained in pairs inindividual sound-attenuated chambers for daily 80 trial sessions(mean intertrial interval, 45 sec). The CS was a 100 msec, 85dB, 6 kHz tone presented via stereo headphones. The unconditionedstimulus (US) was a 150 msec, 3.5 psi corneal air puff sufficientto elicit reliable extension of the nictitating membrane (NM)(or third eyelid) as the unconditioned response. Because agingrabbits typically fail to acquire this trace eyeblink conditioningtask to our usual criterion of 80% CRs in a training session (Thompsonet al., 1996a), a behavioral criterion of 60% CRs in a trainingsession was used for both age groups (all references to learningin the text refer to acquisition of 60% CRs unless explicitlyindicated otherwise). An NM extension was counted as a CR if itoccurred after CS onset but before US onset. Slow-learning rabbits(<30% CRs after 15 sessions) served as an additional control population(Disterhoft et al., 1988a; Moyer et al., 1996; Thompson et al.,1996b). Only one young adult rabbit was slow-learning (comparedwith five aging slow-learning rabbits), so three additional slow-learningyoung adult rabbits were taken from a simultaneous cohort of behavioralstudies and included in the present study. Learning curves foryoung and aged rabbits were normalized to the mean number of trialsrequired to reach criterion for that group using linear interpolationalgorithms (IgorPro; WaveMetrics, Lake Oswego, OR) (Thompson etal., 1996). Behavioral experiments were controlled by an IBM-PCclone computer using custom hardware and software as describedpreviously (Akase et al., 1994; Thompson et al., 1994).

Slice preparation. Twenty-four hours after the last training session, rabbits were deeply anesthetized with halothane, and400 µm hippocampal slices were cut on a vibratome as describedpreviously (Moyer et al., 1996; Thompson et al., 1996a). For thisstudy, 17 young adult rabbits (mean age, 2.2 ± 0.1 months) and19 aging rabbits (mean age, 42.3 ± 1.3 months) were used. Hippocampalslices were maintained in a holding chamber filled with oxygenated,artificial CSF (aCSF) (in mM: 124 NaCl, 3 KCl, 1.3 MgSO₄, 1.24NaH₂PO₄, 2.4 CaCl₂, 26 NaHCO₃, and 10 D-glucose, gassed with 95%O₂-5% CO₂ at pH 7.4) at room temperature (~23°C) for at least45 min. For recording, slices were individually transferred toa submersion chamber (Medical Systems, Greenvale, NY) and continuouslyperfused with oxygenated aCSF at 31°C.

Electrophysiological recordings and data analysis. Intracellular recordings were made from 97 CA1 pyramidal neurons (50 young,47 aging) using an Axoclamp 2A amplifier (Axon Instruments, FosterCity, CA) and thin-walled microelectrodes filled with 3 M KCl(20-50 M $Omega$ ) as described previously (Moyer et al., 1996). All CA1pyramidal neurons included in this study exhibited little spontaneousactivity at rest, had action potential amplitudes >80 mV fromthreshold, had action potential durations >1.2 msec from risethreshold to recrossing of the resting potential, had input resistances $>=$ 25 M $Omega$ , and had stable resting membrane potentials more negativethan $-$ 60 mV. Cells were studied at membrane potentials near $-$ 65mV (using $<=$ 0.2 nA constant current injection, if necessary) tominimize the influence of voltage-dependent changes on membraneconductances. The protocols used to study the properties of CA1neurons and the analyses of all intracellular data were identicalwith previously published methods (Moyer et al., 1996). Briefly,current-voltage relationships were constructed using 400 mseccurrent injections (range, $-$ 1.0 to +0.2 nA). Postburst AHPs wereevaluated using a 100 msec depolarizing current injection sufficientto elicit a burst of four action potentials. Spike frequency adaptation(referred to as accommodation in the present study) was evaluatedby injecting the same amount of depolarizing current used to studythe AHP but for an 800 msec duration. The number of action potentialswere counted and recorded. To evaluate the distribution of changeswithin a population, individual cells were classified as havingbeen "changed by conditioning" if its data fell beyond 2 SDs fromthe mean of the population of naive neurons studied in the particularage group (for details, see Moyer et al., 1996).

All reported values are the mean ± SEM. Statistical analyses were done using unpaired t tests or ANOVA with the significancelevel set at 0.05. Post hoc comparisons were made using Fisher'sPLSD only if a significant main effect wasobserved.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aging rabbits are impaired in acquisition of trace eyeblink conditioning

Aging rabbits required 1405 ± 246 trials to reach the behavioral criterion of 60% CRs within an 80 trial trace conditioningsession compared with 733 ± 138 trials for young adult rabbits(t₁₁ = 2.276; p < 0.05) (Fig. 1A). Comparisons between trace-conditionedyoung and aging rabbits revealed no statistically significantdifferences in percent CRs on the first (young, 7.5 ± 1.9; aging,4.1 ± 1.9; t₁₁ = $-$ 1.27; p = 0.23) or the last (young, 69.8 ± 2.6;aging, 68.6 ± 1.4; t₁₁ = $-$ 0.439; p = 0.67) day of training. Learningcurves constructed from the slow-learning (<30% CRs after 15 sessions)and trace-conditioned rabbits clearly illustrate the poor performanceof the slow-learning rabbits from both groups (Fig. 1C, open symbols)compared with rabbits that learned the task (Fig. 1C, filled symbols).Previous studies have shown that slow-learning rabbits serve asan excellent control group indistinguishable from pseudoconditioningrabbits (Disterhoft et al., 1988b; Moyer et al., 1996). The learningcurves clearly show that, although the aging rabbits were ultimatelyable to achieve a similar level of performance, throughout trainingthey showed fewer CRs, and they took nearly twice as long to reachthe behavioral criterion of 60% CRs than did the young adult rabbits.

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Figure 1. Aging rabbits are significantly impaired in their ability to learn hippocampally dependent trace eyeblink conditioning. A, A plot of trial to criterion among rabbits that learned illustrates that aging rabbits required significantly more trials than young adult rabbits (p < 0.05). B, A plot of percent CRs shows that, among rabbits that learned, young and aging rabbits were not significantly different from each other on either the first or last day of training. C, Learning curves of rabbits that learned (filled symbols) and rabbits that did not learn (open symbols). The dashed line represents the behavioral criterion of 60% CRs. The aging rabbits that eventually learned (filled circles; n = 7) had an average learning curve that was shifted far to the right of young adult rabbits that learned (filled triangles; n = 6). Notice the relatively poor performance of the slow-learning young adult (open triangles; n = 4) and aging (open circles; n = 5) rabbits.

Aging CA1 neurons exhibit decreased postsynaptic excitability compared with young adult CA1 neurons

Postburst AHPs of CA1 neurons from experimentally naive aged rabbits were significantly larger than those from young adultneurons. Aging CA1 pyramidal neurons had AHPs that were significantlylarger in amplitude (t₂₆ = $-$ 3.199; p < 0.005), integrated area(t₂₆ = $-$ 2.871; p < 0.01), and duration (t₂₆ = 2.068; p < 0.05)than young adult CA1 neurons (Table 1, naive data). The enhancedAHPs observed in aging neurons were similar to previous reportsof age-related changes in the AHP (Landfield and Pitler, 1984;Moyer et al., 1992). The postburst AHP is primarily comprisedof an outward, calcium-activated K⁺ current that modulates postsynaptic excitability of many celltypes, including hippocampal and cortical pyramidal neurons (Hotsonand Prince, 1980; Gustafsson and Wigström, 1981; Lancaster andAdams, 1986; Schwindt et al., 1992; Storm, 1990).


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Table 1. Summary of learning-related changes in CA1 neurons from young and aged rabbits

Spike frequency adaptation or accommodation is another measure of postsynaptic excitability (Madison and Nicoll, 1984; Hedlundand Andersen, 1989; Moyer et al., 1992, 1996; Thompson et al.,1996b). CA1 neurons from experimentally naive aging rabbits firedsignificantly fewer action potentials in response to an 800 msecdepolarizing current injection (t₂₆ = $-$ 2.988; p < 0.01) (Table1, naive data) than did young control neurons. These data areconsistent with previous observations of greater accommodationin aging rabbit CA1 neurons compared with young adult neurons(Moyer et al., 1992; Oh et al., 1999).

No statistically significant differences were observed between young and aging neurons in resting membrane potential, inputresistance, time constant, or action potential characteristics(Table 2, naive data). In addition, the amount of current injectionrequired to elicit a burst of four action potentials (used tostudy the postburst AHP) did not vary as a function of age (aging,0.70 ± 0.05 nA; young, 0.66 ± 0.06 nA; t₂₆ = 0.454; p = 0.65).Analyses of within-burst firing also indicated no statisticallysignificant differences between aging and young adult neurons.Latencies from current onset to each of the four APs elicitedduring the 100 msec current step used to study the postburst AHPwere calculated. No statistically significant differences wereobserved in each of the following: (1) latency to the first AP(mean, ~5.4 msec; t₂₆ = $-$ 0.086; p = 0.93); (2) latency to thesecond AP (mean, ~18 msec; t₂₆ = $-$ 0.483; p = 0.63); (3) latencyto the third AP (mean, ~40 msec; t₂₆ = $-$ 0.901; p = 0.38); or (4)latency to the fourth AP (mean, ~71 msec; t₂₆ = 0.364; p = 0.72).


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Table 2. Properties of CA1 neurons from young and aged rabbits that do not change after acquisition of trace eyeblink conditioning

Acquisition of trace eyeblink conditioning increased excitability of aging and young adult CA1 neurons

Postburst AHPs were significantly reduced in both young and aging CA1 neurons after acquisition of hippocampally dependenttrace eyeblink conditioning. ANOVA indicated that the effectsof learning were statistically significant for amplitude (young,F_(3,46) = 21.100, p < 0.0001; aging, F_(3,43) = 35.382, p < 0.0001),integrated area (young, F_(3,46) = 11.561, p < 0.0001; aging, F_(3,43)= 10.780, p < 0.0001), and duration (young, F_(3,46) = 3.427, p< 0.05; aging, F_(3,43) = 4.127, p < 0.01) of the AHP (Table 1).An examination of individual neurons indicated that, after learning,6 of 15 (40%) young adult and 17 of 19 (89%) aging neurons hadsignificantly reduced AHP amplitudes relative to data from age-matchednaive controls (Table 1). Previous reports of learning-specificAHP reductions in CA1 neurons involved only the use of young adultrabbits (Disterhoft et al., 1986; Coulter et al., 1989; de Jongeet al., 1990; Moyer et al., 1996). The present study, however,evaluated whether learning-related changes in postsynaptic excitabilityof CA1 neurons are also observed in aging rabbits. Figure 2 showsthe effects of trace eyeblink conditioning on measures of postsynapticexcitability of aging CA1 pyramidal neurons. The voltage tracesshown in Figure 2A clearly illustrate the reduced size and durationof the AHP in CA1 neurons from aging rabbits that reached thecriterion of 60% CRs in a session relative to CA1 neurons fromaging control rabbits (naive and slow-learning).

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Figure 2. Acquisition of hippocampally dependent trace eyeblink conditioning increased excitability of aging rabbit hippocampal CA1 pyramidal neurons. A, Effects of trace conditioning on the size of the postburst AHP. 1, Overlay of voltage recordings of the postburst AHP in CA1 neurons from an aging naive rabbit (Naive), an aging rabbit that showed <15% CRs after 15 sessions (Slow), and an aging trace-conditioned rabbit (Trace). The resting membrane potentials of these cells were approximately $-$ 65 mV, with action potentials truncated for visualization of the AHP. The AHP was measured for 5 sec beginning after a 100 msec depolarizing current injection (solid black line), with minimal current (~0.6 nA) required to reliably evoke a burst of four action potentials. 2, Mean effects of trace eyeblink conditioning on postburst AHP amplitude in aging rabbit CA1 neurons. Notice that, after learning, the AHP was significantly reduced compared with naive and slow-learning aging controls. B, Typical examples of accommodation responses in CA1 pyramidal cells from aging naive (Naive), aging slow-learning (Slow), and aging trace-conditioned (Trace) rabbits. Although the cell from the trace-conditioned rabbit fired more action potentials, accommodation was not abolished, as evidenced by the increase in interspike interval with time during the 800 msec depolarizing stimulus (solid black line), but rather was significantly reduced after learning. The resting potentials of these cells were approximately $-$ 67 mV.

The learning-related changes in size and duration of the AHP did not result from differences in current required to elicitthe burst of four action potentials used to study the postburstAHP. ANOVA indicated that, for both young adult and aging neurons,the current required to elicit four action potentials did notvary as a function of training condition (young, F_(3,46) = 0.633,p = 0.6; aging, F_(3,43) = 0.404, p = 0.75). Also, there were nodifferences in within-burst firing in either age group as a functionof training condition. Latencies to the first (young, F_(3,46)= 0.228, p = 0.88; aging, F_(3,43) = 1.126, p = 0.35), second (young,F_(3,46) = 0.903, p = 0.45; aging, F_(3,43) = 0.752, p = 0.53),third (young, F_(3,46) = 0.854, p = 0.47; aging, F_(3,43) = 0.73,p = 0.54), or fourth (young, F_(3,46) = 1.09, p = 0.36; aging,F_(3,43) = 1.296, p = 0.3) action potential within each burst werenot significantly different after acquisition of trace eyeblinkconditioning.

After learning, CA1 neurons from both young adult and aging rabbits showed less accommodation than their age-matched controlgroups (Table 1). ANOVA revealed that significantly more actionpotentials were elicited after acquisition of trace eyeblink conditioning(young, F_(3,46) = 7.232, p < 0.001; aging, F_(3,43) = 10.606, p< 0.001). Figure 2B clearly shows this effect in aging neurons.Notice that neurons from experimentally naive and slow-learningrabbits exhibited robust accommodation, whereas neurons from trace-conditionedrabbits fired more actionpotentials.

The learning-related changes in postsynaptic excitability (AHP and accommodation) were present in the absence of any statisticallysignificant changes in resting membrane potential, time constant,input resistance, or action potential characteristics (Table 2).This was true for CA1 neurons from both young adult and agingtrace-conditionedrabbits.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aging rabbits were significantly slower than young adult rabbits in acquiring the trace eyeblink conditioning task. CA1 neuronsfrom aging naive rabbits had larger AHPs and exhibited more accommodationrelative to neurons from young naive rabbits. After learning,both the postburst AHP and spike frequency accommodation weresignificantly reduced in a learning-specific manner in CA1 neuronsfrom young adult and aging rabbits. These data represent the firstevaluation of learning-related changes in aging rabbit CA1 neuronsusing intracellular recordings in vitro and implicate changesin postsynaptic excitability of hippocampal neurons in both agingand associativelearning.

Aging rabbits were clearly impaired in their ability to acquire the trace eyeblink conditioning task (Fig. 1), consistentwith previous observations of impaired learning ability in agingrabbits (Graves and Solomon, 1985; Deyo et al., 1989; Solomonand Groccia-Ellison, 1996; Thompson et al., 1996a). The agingrabbits required nearly twice as many training trials than didyoung adult rabbits to reach a behavioral criterion of 60% CRsin a session. Of the 13 aging rabbits that received trace eyeblinkconditioning, only eight were able to reach criterion, whereasthe other five remained below 30%, even after 15 training sessions.Of the eight aging rabbits that were able to learn, only two didso at a rate similar to that seen in young rabbits. These observationsare consistent with previous data indicating substantial heterogeneityof learning ability among populations of aging rabbits receivingtrace eyeblink conditioning (Thompson et al., 1996a). In addition,the inability of the aging rabbits probably did not result froman inability to process CS and US information because animalsswitched to the delay conditioning task learn within several trainingsessions (Thompson et al., 1996a).

Hippocampal CA1 neurons recorded from experimentally naive aging rabbits had significantly larger, longer lasting postburstAHPs (Table 1), consistent with previous reports of decreasedpostsynaptic excitability of aging rabbit and rat CA1 neurons(Landfield and Pitler, 1984; Moyer et al., 1992). After a burstof action potentials, the larger, longer lasting AHPs of agingCA1 neurons could act to dampen the impact of excitatory inputsfor several seconds (the duration of the AHP). Thus, a barrageof excitatory inputs onto an aging CA1 neuron during the AHP wouldbe less likely to drive the cell to threshold than if the cellwas at or near its resting membrane potential. The larger AHPsobserved in aging CA1 neurons could result from an excess influxof calcium during depolarization because bath application of nanomolarconcentrations of the L-type calcium channel antagonist nimodipineeffectively eliminates the aging-related increase (Moyer et al.,1992). Additional evidence implicating calcium or calcium-dependentprocesses in aging comes from work demonstrating that aging CA1neurons have prolonged calcium action potentials (Moyer and Disterhoft,1994) and larger calcium currents (Landfield, 1996) compared withyoung adult neurons. Preliminary data from whole-cell voltage-clampexperiments also suggest that the calcium-activated potassiumcurrent underlying the slow AHP is enhanced in aging rabbit CA1neurons (Power et al., 1999).

In addition to the enhanced AHPs, CA1 neurons from aging control rabbits also exhibited more robust accommodation during along depolarizing current injection than young adult neurons (Table1) (Moyer et al., 1992). This latter observation suggests that,even when aging CA1 neurons reach threshold, they are less likelyto exhibit a sustained firing pattern in response to a continuousstream of inputs. That CA1 neurons from experimentally naive agingrabbits exhibited both larger AHPs and more robust accommodationthan neurons from young adult rabbits is not surprising becausemodulation of the AHP by intracellular calcium or neurotransmitterstypically alters accommodation (Schwartzkroin and Stafstrom, 1980;Cole and Nicoll, 1983; Haas and Greene, 1984; Hedlund and Andersen,1989; Oh et al., 1999; Weiss et al., 2000).

After learning, CA1 neurons from aging rabbits had postburst AHPs that were 52.5% smaller in amplitude than those from agingcontrol rabbits (Table 1). Inspection of individual neurons indicatedthat, after acquisition, 89% of the aging CA1 neurons exhibitedreduced AHPs. These effects were observed on the amplitude, theintegrated area, and the duration of the AHP. In response to longdepolarizing current steps, CA1 neurons from aging rabbits fired76.9% more action potentials after learning than did neurons fromaging control rabbits (Table 1). These data indicate that acquisitionof trace eyeblink conditioning in aging rabbits was accompaniedby increased postsynaptic excitability of CA1 pyramidal cells.In addition, CA1 pyramidal neurons from young adult rabbits hadAHP amplitudes that were 39.6% smaller after acquisition of traceeyeblink conditioning than control neurons with 40% of the neuronsexhibiting reduced AHPs (Table 1). When given a long depolarizingcurrent injection, young adult CA1 neurons fired 41.7% more actionpotentials after learning than did control neurons. Such changeswere not observed in CA1 neurons from aging or young rabbits thatshowed fewer than 30% CRs after 15 training sessions (Table 1,Slow learners), suggesting that the effects were learning-specific,as previously observed in CA1 and CA3 neurons from young adultrabbits (Moyer et al., 1996; Thompson et al., 1996b).

Previous in vitro studies only evaluated the electrophysiological properties of aging rabbit CA1 neurons in experimentallynaive animals (Moyer et al., 1992; Moyer and Disterhoft, 1994;Oh et al., 1999). The present data show that, although CA1 neuronsfrom aging control rabbits had larger AHPs and stronger accommodationthan neurons from young adult controls, aging rabbits that learnedthe trace eyeblink conditioning task had AHPs that were significantlyreduced relative to aging controls. In fact, after acquisitionof trace conditioning, AHPs from aging rabbit CA1 neurons werereduced to a size that was similar to that observed in the youngadult rabbits after learning (Table 1). This latter point isquite interesting because it suggests that a similar level ofpostsynaptic excitability must be attained for successful acquisitionof trace conditioning, independent of the age of the animal. Theactual differences between aging control and aging conditionedneurons were much greater than those between young control andyoung conditioned neurons (Table 1). That is, the aging neuronshad to change more than the young adult neurons to achieve thesame level of postsynaptic excitability (e.g., similarly sizedAHPs). The greater change required for an aging neuron to reachthe conditioned state may partly underlie the need for aging rabbitsto receive significantly more training trials to successfullylearn the trace eyeblink conditioning task. These data providestrong support for a correlation between changes in postsynapticexcitability, learning, and aging-related learningdeficits.

In the present study, rabbits were trained to a behavioral criterion of 60% CRs in an 80 trial session. When rabbits weretrained to the more difficult criterion of 80% CRs, there werelittle additional increases in CA1 postsynaptic excitability (Table1). Although only one aging rabbit was able to reach 80% CRs,three of the four cells recorded from this aging rabbit had reducedAHPs, and the mean amplitude was basically the same as those trainedto a criteria of 60% CRs ( $-$ 3.06 ± 0.5 vs $-$ 3.01 ± 0.2 mV, respectively).The data from young adult rabbits indicated that, when trainedto a criterion of 80% CRs, their CA1 neurons had a mean AHP amplitudethat was only slightly smaller than those trained to a criteriaof 60% CRs ( $-$ 2.5 ± 0.3 compared with $-$ 3.02 ± 0.2 mV, respectively).Similarly, there was a slight change in accommodation as a resultof using a behavioral criterion of 80% CRs. On average, in bothage groups, training to a criterion of 80% CRs resulted in anincrease of approximately one action potential during accommodationversus that seen when rabbits were trained to a 60% criterion(Table 1). Interestingly, there were no statistically significantdifferences in AHP amplitude, AHP area, AHP duration, or accommodationbetween young or aging CA1 neurons from either trace-conditionedgroup. When compared with data from a previous study in whichyoung adult rabbits were trained to a criterion of 80% CRs, theAHP and accommodation data observed 24 hr after acquisition (Moyeret al., 1996) were similar to the data obtained in young adultCA1 neurons after conditioning to 80% CRs in the present study.These data suggest that the AHP reductions were nearly maximalwhen aged rabbits were trained to a behavioral criterion of 60%CRs. However, in young adult rabbits, further reductions of theAHP occurred with additional training to 80% CRs (Table 1).

Additional support for involvement of changes in postsynaptic excitability of hippocampal CA1 neurons with learning and agingcomes from studies in which compounds that reduce both the AHPand accommodation were given to young adult or aging animals.For example, administration of the L-type calcium channel antagonistnimodipine facilitates acquisition of trace eyeblink conditioningin aging rabbits (Deyo et al., 1989; Straube et al., 1990; Kowalskaand Disterhoft, 1994), and nanomolar concentrations of nimodipinereduce both the AHP and accommodation in aging rabbit CA1 neuronsin vitro (Moyer et al., 1992). Similar effects have also beenobserved in aging rabbits treated with cholinesterase inhibitorsand muscarinic agonists (Kronforst-Collins et al., 1997; Oh etal., 1999; Weiss et al., 2000). Compounds that directly enhancethe postburst AHP have not been tested in eyeblink conditioning,but the aforementioned data suggest that such drugs would likelyimpairlearning.

Increased postsynaptic excitability appears to be one mechanism used by hippocampal neurons in both young and aging animalsfor acquisition of trace eyeblink conditioning. Previous datafrom young rabbits demonstrated that changes in hippocampal excitabilitywere transient, lasting 5-7 d after acquisition to a criterionof 80% CRs in a session (Moyer et al., 1996; Thompson et al.,1996b). Although in the present study postsynaptic excitabilityof aging rabbit CA1 neurons was similar to young neurons afterlearning, it is unknown whether the increased excitability seenin aging neurons would last as long as those seen in young adultneurons. The current study was not designed to address this issue,but data from aging rats suggest that memory consolidation (Olerand Markus, 1998) and information processing (Barnes et al., 1997;Tanila et al., 1997) are significantly impaired in agingrats.

In conclusion, the present study is the first to report learning-related excitability changes in aging CA1 neurons. Thesedata provide additional support for the hypothesis that alterationsin postsynaptic excitability are involved in both aging and associativelearning.

  FOOTNOTES

Received March 6, 2000; revised April 18, 2000; accepted April 25, 2000.

This work was supported by National Institutes of Health Grants RO1 MH47340, RO1 AG08796, and RO1 DA07633 to J.F.D. We thankF. Cutting and J. Hauser for technicalassistance.
Correspondence should be addressed to Dr. James R. Moyer, Jr., Department of Psychology, Yale University, P.O. Box 208205,New Haven, CT 06520-8205. E-mail: james.moyer{at}yale.edu.

Dr. Power's present address: Department of Neuroscience, Australian National University, John Curtin School of Medical Research,Canberra, Australia2601.

Dr. Thompson's present address: School of Human Development, GR 4.1, University of Texas at Dallas, Richardson, TX75083.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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