The Effect of Aging on Experience-Dependent Plasticity of Hippocampal Place Cells

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Volume 17, Number 17, Issue of September 1, 1997 pp. 6769-6782
Copyright ©1997 Society for Neuroscience

The Effect of Aging on Experience-Dependent Plasticity of Hippocampal Place Cells

Jiemin Shen⁴, Carol A. Barnes¹^,²^,⁴, Bruce L. McNaughton¹^,³^,⁴, William E. Skaggs⁴, and Karen L. Weaver¹^,⁴
¹ Departments of Psychology, ² Neurology, and ³ Physiology, and ⁴ Arizona Research Laboratories, Division of Neural Systems, Memory and Aging, University of Arizona, Tucson, Arizona 85724

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

The firing characteristics of 1437 CA1 pyramidal neurons were studied in relation to both spatial location and the phase ofthe theta rhythm in healthy young and old rats performing a simplespatial task on a rectangular track. The old rats had previouslybeen found to be deficient on the Morris spatial learning task.Age effects on the theta rhythm per se were minimal. Theta amplitudeand frequency during rapid eye movement sleep were virtually identical.During behavior, theta frequency was slightly reduced with age.In both groups, cell firing occurred at progressively earlierphases of the theta rhythm as the rat traversed the place fieldof the cell (i.e., there was "phase precession," as reported byothers). The net phase shift did not differ between age groups.The main finding of the study was a loss of experience-dependentplasticity in the place fields of old rats. During the first laparound the track on each day, the initial sizes of the place fieldswere the same between ages; however, place fields of young rats,but not old, expanded significantly during the first few lapsaround the track in a given recording session. As the place fieldsexpanded, the rate of change of firing with phase slowed accordingly,so that the net phase change remained constant. Thus changes infield size and phase precession are coupled. A deficit in plasticityof place fields in old rats may lead to a less accurate populationcode for spatial location.
Key words: aging; hippocampus; place fields; phase precession; theta rhythm; plasticity

INTRODUCTION

Because effective spatial learning requires an intact hippocampus (e.g., O'Keefe and Nadel, 1978; Morris et al., 1982; Sutherlandet al., 1982; Barnes, 1988; Jarrard, 1993), and because this crucialcognitive function is significantly impaired during normal aging,the study of how neuronal information processing in the hippocampusis altered with age is of considerable interest. In rodents, agedeficits are observed in a variety of spatial learning and memorytasks (Barnes, 1979; Wallace et al., 1980; deToledo-Morrell etal., 1984; Gage et al., 1984; Barnes and McNaughton, 1985; Gallagheret al., 1985; Gallagher and Pelleymonter, 1988). These effectscannot be fully accounted for by sensory or motor deficits (Rappet al., 1987; Gallagher and Pelleymonter, 1988; Gage et al., 1989),suggesting that alterations in hippocampal function with age maycontribute to their etiology. There are three particularly strikingaspects of hippocampal electrophysiology that have attracted interestwith respect to their possible roles in spatial learning, andthe change with age of which could contribute to age-associatedmemory impairment: place-specific firing (O'Keefe and Dostrovsky,1971) of single neurons ("place cells"); the 7-12 Hz theta rhythmin the EEG (Green and Arduini, 1954), which is tightly relatedto "spatial" behaviors (e.g., walking and rearing) (Vanderwolfet al., 1975); and the long-lasting change in synaptic efficacythat can be induced by patterned activation of hippocampal afferents[i.e., long-term potentiation (LTP)] (Bliss and Gardner-Medwin,1973; Bliss and Lømo, 1973).

Unfortunately, the available data on the effects of age on these phenomena are somewhat contradictory, and it remains unclearwhether there are age differences in the theta rhythm (Barnes,1979; Forbes and Macrides, 1984; Markowska et al., 1995) or whetheror how place field characteristics change in old rats (Barneset al., 1983; Mizumori et al., 1996; Markus et al., 1994). Severalfactors may contribute to the variability of the results of previousstudies of age effects on place field characteristics of old rats.A major one is the age of the animals at the time of recording.It is becoming increasingly clear that age effects on the nervoussystem in general are accelerated late in the lifespan and hencemay not show up until the last months of life. Secondly, Mizumoriet al. (1996) have reported an interaction between age and thespatial task used during recording on the quality of place fields.Thus, age effects may not show up in all tasks or may be expresseddifferently in different tasks. Third, different studies haveused different statistical methods. Of particular importance isthe necessity of performing statistics on a per animal ratherthan a per cell basis. Because cells within an animal are notindependent, the latter practice can lead to the detection ofeffects that are attributable to normal between-subject variationand that are not necessarily consistent effects of age per se.Finally, the quality of single-unit isolation and number of cellsrecorded in a given study may influence the power to detect quantitativechanges in place field characteristics with age. In the presentstudy, improved isolation of hippocampal units was accomplishedusing multiple "tetrode" probes (McNaughton et al., 1983b; O'Keefeand Recce, 1993; Wilson and McNaughton, 1993), and statisticalanalysis was conducted by animal rather than by cell. The discrepancyin the literature concerning changes in hippocampal EEG duringaging could be attributed to differences in the extent and velocityof locomotion of animals of different ages. Because the frequencyof the theta rhythm increases with running velocity (McFarlandet al., 1975; Arnolds et al., 1979; Recce, 1994), age differencesin running speed could account for "slowing" in frequency withage. In the present experiment, this parameter was controlledfor.

The effects of age on two recently discovered characteristics of hippocampal dynamics were of particular interest in the presentstudy. First, Mehta et al. (1997) have demonstrated a rapid, experience-dependentexpansion of place fields in young rats during repeated performanceof a route-following task. It was of interest to determine whetherthis process is altered by age. Second, although it has been knownthat single hippocampal neurons are periodically modulated atthe theta frequency (Ranck, 1973; Fox et al., 1986), O'Keefe andRecce (1993) recently found that place cell firing advances graduallyin phase as the rat passes through the place field (Fig. 1). Theycalled this effect "phase precession." Thus, the cell-firing phasecontains spatial information, and may provide a potential neuralmechanism by which temporal sequences can be coded within individualtheta cycles through synaptic modification (e.g., LTP, Skaggset al., 1996). The effect of age on this phenomenon was thus amajor focus of the present study.
Fig. 1. Illustration of the phase precession effect in the spike train of a single CA1 pyramidal cell recorded from a young rat runningfor food reward on a rectangular track. A, Spatial pattern ofspike activity and firing phase. Each spike is represented bya colored dot at the corresponding location (the rat was movingin a clockwise direction around the track). The colors correspondto the theta phases indicated in B and C. The irregular gray linesrepresent the rat's trajectory. Only the corner of the rectangulartrack containing the place field is shown. Note that, as the rattraversed the place field, the phases of the spikes advanced systematically.B, Theta phase of spike discharge versus position on the track.To construct this plot, the rat's position at each moment wasprojected onto a one-dimensional axis corresponding to the trackcenter. Each point represents a single spike. Phase zero is thepreceding peak of the theta cycle during which the spike occurred.C, Plot of the theta rhythm and spike train for a single traversalof the place field. The theta rhythm record was digitally filteredin the range of 6-10 Hz. Each short vertical line below the waveformrepresents a single spike, and the time at which it occurred relativeto the theta rhythm is labeled by a dot on the waveform. Belowthe spike train is a time axis, with ticks indicating the timesat which the peaks of theta rhythm occurred. The period betweentwo neighboring peaks is one theta cycle. As the rat traversedthe place field, the spikes occurred earlier and earlier in thetheta cycle. D, Histogram of activity versus theta cycle numberas the rat passed through the place field over multiple trials.A point was selected on the track, near the center of the placefield of the cell, and, on each pass through the field, the thetapeak that occurred nearest to this point was selected as cyclezero. Near the beginning of the place field (cycle $-$ 3), the spikesare distributed toward the end of the cycle. Thereafter the activitydistributions shift progressively earlier.
[View Larger Version of this Image (38K GIF file)]

MATERIALS AND METHODS
Animals and behavioral training Six pairs of young (11-12 month) and old (25-31 month) male Fischer 344 rats, obtained from the National Institute on Agingcolony at Harlan Sprague Dawley, were used in this experiment(see Table 1). Rats were housed individually in Plexiglas guineapig tubs and maintained on a 12 hr light/dark cycle. They werehandled for a minimum of 5 min/d for 3 d before entering behavioraltesting. All manipulations were performed in batches of one youngand one old rat. All rats underwent testing of their spatial andvisual discrimination abilities on the Morris swim task (detailsas in Shen and Barnes, 1996). Thereafter, they were food-deprivedand maintained at ~85% of their ad libitum body weights. Subsequentbehavioral training consisted of several steps. For the first2-3 d, the rats were trained to forage for randomly scatteredchocolate cake sprinkles in a 62 × 70 cm box for 60 min/d. Theywere then trained on a linear track (122 × 14 cm). For the first3 d on the track, rats were allowed to forage for scattered chocolatesprinkles for about 90 min. During the subsequent week, chocolatefood reward was only offered alternatively at the two ends ofthe track. Finally, the rats were first placed into a "nest" inthe training room to rest quietly or sleep for 1 hr and then weretransferred onto the track and allowed to obtain food reward atthe two ends for 30 min. This was followed by another sessionin the nest in which they slept for another hour. Implantationof electrodes occurred at the end of this phase of training. Thelinear track described above was used only in this pretrainingphase.

Table 1. Age of rats during recording sessions and total number of sessions conducted and included in the present study

Rat Group Pair Age (months) Sessions

5357 Old 1a 25.5 2

5358 Young 1b 12 2

5344 Old 2a 25 1^a

5397 Young 2b 12 5

5378 Old 3a 29.5 3

5397 Young 3b 12 5

5408 Old 4a 30.5 3

5631 Young 4b 11.5 6

5484 Old 5a 30 4

5554 Young 5b 12 4

5697 Old 6a 26.5 6

5672 Young 6b 11.5 4

^a Two sessions were actually conducted, but the data from one session were corrupted because of a computer malfunction.

Surgery and construction of electrodes The construction of the electrode assembly ("hyperdrive") has been described in detail elsewhere (Gothard et al., 1996). Briefly,the electrode array consisted of 14 independently movable "tetrodes,"12 of which were used for unit recording, one as reference fordifferential recordings, and the other specifically for recordingEEG. Each tetrode consisted of four twisted, enamel-coated nichromewires (13 µm). The tips were gold-plated, resulting in impedancesat 1 kHz in the range of 300-600 k $Omega$ . Each tetrode was insertedinto two nested polyimide cannulas (78 and 110 µm in diameter,respectively), which were themselves inserted into a 30-gaugestainless steel cannula. The stainless steel cannula was bentat a 30° angle near the end, so that the tips of all the tetrodeswere placed within an area <2 mm across, whereas the other endsfanned out into a cone. Each tetrode was attached to a metal screw,one turn of which equaled ~320 µm in depth. Each tetrode wirewas attached to a contact point on a multiple pin connector plug.

National Institutes of Health guidelines were followed for all surgical procedures. Briefly, rats were anesthetized with Nembutal(sodium pentobarbital) and placed in a stereotaxic apparatus.The scalp was retracted, and seven or eight holes were drilledin the skull to accommodate jeweler's screws to anchor the implant.A hole was drilled over the dorsal hippocampus on the right side,at coordinates of 3.8 mm posterior to bregma and 2.0 mm lateralto the midline, into which the tetrode array was positioned andcemented in place with dental acrylic.
Recording techniques and procedures The connector plug on the hyperdrive was attached to a head stage containing two microchips (Multichannel Concepts, Inc.,Gaithersburg, MD), each with 25 unity gain field effect transistoramplifiers, for impedance reduction. The signals from the headstage were carried by a multiwire cable to a set of seven, rack-mounted,eight-channel, software-controlled amplifiers (Neurolynx Corp.,Tucson, AZ) and then to a group of eight, 80486-based microcomputers.Signals were amplified 3000-10,000 times, depending on signalsize, and were filtered with a bandpass of 600-6000 Hz beforebeing sent to analog-to-digital cards (Data Translation, Inc.,Marlboro, MA) on the microcomputers. Data were acquired usingDiscovery software (Data Wave Inc., Broomfield, CO). Wheneverthe amplitude of the spike signal exceeded a predetermined threshold,each tetrode channel acquired a 1 msec sample of data at a rateof 32 KHz. These spike samples were time-stamped and stored ondisk. Additionally, signals from one channel of each tetrode wereamplified by a factor of 2000 and filtered with a bandpass of1-100 Hz. These additional channels were used to record EEG continuouslyat a sampling rate of 200 Hz.

For tracking the movement of the animals on the behavioral apparatus, two small arrays of infrared light-emitting diodes wereattached to the head stage, one extending to the front and theother to the back of the rat. Position data were acquired by atracking device (Tracker SA-2; Dragon, Boulder, CO), which extractedand stored the coordinates of the front and back diode arraysat a resolution of 256 × 256 pixels (2.3 pixels/cm for the currentexperiment). This information was sampled at 20 Hz. The data werelater reprocessed off-line to correct or delete occasional misidentifiedpoints.

The principle of the tetrode recording technique was proposed by McNaughton et al. (1983b) as an extension of the stereotroderecording method and has subsequently been described in detail(O'Keefe and Recce, 1993; Wilson and McNaughton, 1993; Gray etal., 1995; Gothard et al., 1996). Briefly, the tips of four microwiresof a tetrode are so closely spaced that most cells recorded byany of the wires will simultaneously be recorded by one or moreof the other wires, typically at a different amplitude. The units,therefore, were isolated by displaying all orthogonal two-dimensionalprojections of the four-channel relative amplitude data and applyingboundaries to each apparent unit cluster by the use of a custominteractive program running on a Sun workstation.

After the rat had recovered from surgery, the reference electrode was lowered into the corpus callosum (~1400-1600 µm underthe dura), and the EEG electrode was lowered into the vicinityof the hippocampal fissure to optimize recording of the thetarhythm. The other 12 tetrodes, however, were gradually lowered,over the course of a number of days, into the CA1 cell body layerof the dorsal hippocampus. During this recording optimizationperiod, the rat was trained to run in a single direction (clockwise)on a rectangular track (94 cm × 40 cm, 6 cm in width) in the recordingroom for at least 20 laps. This apparatus was different from theones used during the pretraining phase. The arrival of each tetrodeinto the hippocampus was recognized by several criteria, includingthe presence of 100-300 Hz "ripples" in the EEG (O'Keefe, 1976;O'Keefe and Nadel, 1978; Buzsàki et al., 1992; Ylinen et al.,1995), the polarity of "sharp waves" in the EEG (Buzsàki et al.,1986; Suzuki and Smith, 1987), and the sudden appearance, at adepth of about 2 mm below the dura, of large numbers of simultaneouslyrecorded cells with complex spike discharges while the rats werein a quiet waking state. Each rat underwent two to six recordingsessions. The fewer cells recorded per session, the more sessionswere conducted, to get approximately equal cell sampling fromeach rat. Each session consisted of three phases. First, the ratwas placed in a nest on top of the rectangular track and was allowedto sleep for about 30-90 min, during which recording was conductedto determine overall cell numbers. Because most cells are activeduring sleep, whereas many cells are silent when the rat is activein a given environment (Thompson and Best, 1989), the proportionof detectable cells with place fields on the maze could be determinedusing this procedure. In the second phase of the session, therat was placed onto the rectangular track and allowed to run inthe clockwise direction for 20-35 laps. Food reward was providedat two corners of the track. In the final phase, the rat was placedback into the nest to sleep again for another 30-90 min, duringwhich time the activity of single units was also recorded.
Data analysis Identification of units. Pyramidal cells in the CA1 region were distinguished from theta cells using standard criteria (Ranck,1973; Fox and Ranck, 1981; Buzsàki et al., 1983; McNaughton etal., 1983a). The classification criteria for inclusion into thepyramidal cell category was that the cell must fire at least asmall number of complex spike bursts during the recording session,be recorded simultaneously with other complex spike cells (inthe stratum pyramidale), have a spike width (peak to valley) ofat least 300 µsec, and have an overall mean rate of <5 Hz duringthe behavioral recording session. To be included into the thetacell category, on the other hand, the cell would be required tofire no complex spike bursts, to have a spike width of less than300 µsec, and to have a mean firing rate of >5 Hz during the behavioralrecording session.

Quantification of theta rhythm. The EEG data were digitally filtered into the 6-10 Hz band. For behavioral episodes, all EEGwas analyzed for periods when the animal's running velocity exceededa predetermined threshold (6 cm/sec), which ensured a reliableseparation of theta and nontheta EEG. For rapid eye movement (REM)sleep, the presence of theta was determined by inspection (seeResults). In practice, there was no difficulty in separating thetafrom nontheta EEG, and there was high interobserver reliability.For the analysis of age effects on theta rhythm, the velocity,theta frequency, and theta amplitude were determined every 0.2sec. The frequency was defined as the inverse of the time betweensuccessive peaks of the filtered EEG. The amplitude for each cyclewas computed as the height of the initial peak of each cycle tothe baseline. Velocity was calculated every 50 msec using a slidingwindow of 200 msec.

Spatial firing measures. For purposes of data analysis, the rectangular maze was "linearized" by projecting each point onthe trajectory of the rat onto the nearest point on a line alongthe center of each arm of the track. This line was divided into64 equal-length bins; the total occupancy time and total numberof spikes were computed for each bin.

A "place field" was defined according to the criteria of Muller et al. (1987): a group of adjoining bins (sharing at leastone side) with the average firing rate of each bin exceeding aspecified threshold. For this study, the minimal number of adjacentbins was set at 10, the analysis was restricted to cells withat least 100 spikes in the recording session, and the thresholdwas set at a constant rate of 1 Hz. The value of 1 Hz was chosenbecause the average mean rate of all the complex spike cells firingon the maze was ~1 Hz. Although the 1 Hz threshold eliminatedabout half of the recorded spikes, these spikes were mostly thosethat occurred while the rat was in nontheta mode (i.e., eating,grooming, and pausing) and hence are not expected to be spatiallyselective. In one analysis, thresholds of 0.5 and 2 Hz were alsoused for comparison. For those cells that had more than one placefield, each field was treated separately in subsequent analyses.The size of a place field was defined unidimensionally; i.e.,firing locations with respect to the principle track axis wereanalyzed. The field rate integral was defined as the sum of therates within the defined place field. In the subsequent analysisof place fields by laps, the field was defined as the locationwhere spikes occurred within the field boundary as defined above,and the lap-specific field size was measured as the unidimensionaldistance between the first and last spikes within the field.

Phase precession analysis. After the EEG had been filtered with a bandpass of 6-10 Hz, giving it the appearance of a graduallyvarying sinusoid, theta cycles were defined to begin and end atconsecutive peaks of the resulting wave (Skaggs et al., 1996).Each spike that occurred in the presence of theta rhythm was assigneda nominal phase, according to the fraction of the time betweenthe theta peaks at which it occurred. Precisely, the phase assignedto a spike at time t was (t $-$ t₀)/(t₁ $-$ t₀), where t₀ and t₁ arethe times of the preceding and following peaks of the filteredEEG signal. Note that the phase is always a number between 0 and1, which correspond to 0 and 360°, respectively. The theta phaseof the spike was then plotted against the location of the animalon the track at which the spike occurred (e.g., Fig. 2A). Becausephase is periodic and the entry phase of the place fields wasusually somewhat after the peak of the theta cycle, the distributionof points in this plot was typically discontinuous. To examinethe correlation between the phase and location, the point of discontinuity(i.e., the point at which there was an abrupt change in phase)was estimated by inspection, and 360° was subtracted from thepoints above the discontinuity (O'Keefe and Recce, 1993). Thisresulted in a continuous distribution of points in the phase versuslocation plot (Fig. 2B). Regression analysis was then performedusing a conventional least-squares minimization method (Fig. 2B),to examine the relationship between phase versus location. Theentry phase and exit phase of the place field were the phasespredicated by the regression line for the position of the firstand the last spike of the place field, respectively. The slope,coefficient of determination (r²) of the regression lines, phase change (difference between theentry phase and the exit phase), and field size were averagedfor each rat. The comparison between young and old rats was thenconducted by animal, using one-way ANOVA.
Fig. 2. Illustration of the regression analysis for phase precession from one representative cell. A, Firing phase versus positionas described in Figure 1B. To make the periodicity of this functionclear, two cycles of phase have been plotted. The discontinuitynear 0.75 (arrow) is taken to reflect the boundary between firingrelated to field entry and that related to field exit and servesas the reference point for performing linear regression on a singlecycle of phase data. B, As described in Materials and Methods,the data points above the discontinuity in the plot in A werereplotted at the corresponding phase one cycle earlier, and aregression line was fitted using least squares minimization. Asshown by Skaggs et al. (1996), firing phase typically changesnonlinearly with position, with an accelerated advance near theend of the place field; however, for the present purpose, onlythe linear component is considered.
[View Larger Version of this Image (31K GIF file)]

The mean angles of the entry phase and the exit phase, which are circular (i.e., periodic) variables were calculated for eachrat using:

(1)

(2)

(3)

where n is the number of place fields recorded.

RESULTS

Effect of age on spatial and visual discrimination behaviors
Morris swim task Repeated measures ANOVAs were conducted on the spatial and visual discrimination data. The old rats were significantly poorerat finding the location of the hidden platform in the water pool.Although both age groups showed improvement over trials (F_(1,23)= 2.97; p < 0.0001), the old rats swam longer, less direct routesto it (F_(1,10) = 4.99; p < 0.05). Both young and old rats showedimprovement over trials in the visual discrimination version ofthe task (F_(1,11) = 1.96; p < 0.04), with no effect of age onperformance (F_(1,9) = 0.36; p < 0.56). Thus, consistent with previousreports (e.g., Gage et al., 1984; Gallagher et al., 1985; Barneset al., 1996) the old rats were selectively impaired, comparedwith young rats, on the spatial version of this task.

Effect of age on theta rhythm during REM sleep
The mean frequency and amplitude of theta rhythm during REM sleep were first compared between young and old rats. Becausethe rat is motionless during REM sleep, any effect of movementvelocity on the theta rhythm can be ruled out in this state. Onlythose robust REM sessions lasting >30 sec were included, totaling41 REM episodes from young rats [mean duration, 113 ± 7 (SEM),54 (SD) sec] and 60 REM episodes from old rats [mean duration,129 ± 14 (SEM), 87 (SD) sec]. The mean theta frequency and meantheta amplitude of each episode were then averaged for each animalby taking the frequency of REM theta rhythm calculated in blocksof 0.2 sec. These frequency blocks were averaged over the entiresession to obtain the mean frequency for each session. There wasno significant difference in either the theta frequency (F_(1,10)= 1.09; p < 0.32) (Fig. 3C) or the theta amplitude (F_(1,10) =0.02; p < 0.89) (Fig. 4C) between young and old rats. Note thatthe amplitude of the theta rhythm was quite variable between individualrats of both age groups, presumably because of the fact that theamplitude is sensitive to the exact location of the EEG electrode.
Fig. 3. Effect of age on the frequency of theta rhythm. A, Two representative examples, one from a young rat, the other from an oldrat, for the regression analysis of the relation between runningvelocity and theta frequency in a single recording session. Low-velocity(<6 cm/sec) data were excluded to prevent contamination of resultswith nontheta mode EEG (LIA). The overall age comparison of theintercept and slope are summarized in the bottom panel. Averageregression lines were drawn by taking the mean values of the interceptand slope for each age group. The shaded regions on each sideof these average regression lines indicate ±1 SEM. B, Means ±SEM of the regression slopes and the correlation coefficientsfor theta frequency versus running velocity. Although the correlationcoefficient was significantly lower in old rats, a significantdifference in the slopes was not detected. C, Means ± SEM of theintercept of the regression lines and the theta frequency duringREM sleep. The intercept was slightly but significantly smallerin old rats, whereas there was no difference in the REM thetafrequency between the two age groups. D, Mean ± SEM of the ratiobetween the intercept value of theta frequency and the mean REMtheta frequency for a given rat. The ratio was ~1.0 in young ratsand slightly but significantly smaller in old rats (*p < 0.05;**p < 0.01).
[View Larger Version of this Image (50K GIF file)]

Fig. 4. The effect of age on the amplitude of theta rhythm. A, Two examples, one from a young rat, the other from an old rat, forthe regression analysis of the relation between running velocityand theta amplitude in a single recording session. The bottompanel shows the summarized data in the same way as in Figure 3A,except that the shaded regions representing the SEM were onlydrawn on one side of each line to avoid overlap. B, There wasno significant difference between young and old rats in eitherthe slope or the correlation coefficient. C, Means ± SEM of theintercept of the regression lines and theta amplitude during REMsleep. There was no significant age effect on either measurement;however, as shown in D, the ratio of mean theta amplitude duringREM and the amplitude intercept values during maze behavior, although~1.0 in young rats, was significantly reduced with age (**p <0.01).
[View Larger Version of this Image (49K GIF file)]

Effect of age on theta rhythm during behavior on the rectangular track
There were two food reward locations on the rectangular track, at which the EEG changed from predominantly theta to largeirregular activity (LIA), when the rats stopped to eat (Vanderwolfet al., 1975). Therefore, the EEG at stationary or low velocitieswas excluded from the data analysis, to prevent the contaminationof theta rhythm by LIA. Two methods were used to achieve this:one was to eliminate measurement when the velocity was <6 cm/sec(absolute velocity cutoff); the other was to eliminate the datacollected in the lowest 15% of the velocity range (relative velocitycutoff). Because of the generally low running speed of old rats(see below) and their consequent longer periods on the track,the relative velocity cutoff led to a significantly larger datasample in old rats in comparison with young rats (p < 0.01). Onlythe absolute velocity cutoff data are therefore shown here, althoughsimilar results were obtained from both kinds of analysis.

For each recording session, regression and correlation analyses were used to examine the relationship between the runningvelocity and the frequency of theta rhythm recorded when the ratwas traversing the rectangular track. Consistent with previousresults (Recce, 1994), there was, in general, a weak linear relationshipbetween the velocity and frequency, (i.e., the faster the ratran, the higher the frequency of theta rhythm) (Fig. 3A). All26 sessions recorded from young rats and 17 of 19 sessions recordedfrom old rats exhibited statistically significant correlationsbetween the velocity and theta frequency (p < 0.05). The interceptand slope of the regression line for each session, as well asthe correlation coefficient, were averaged for each rat, followedby one-way ANOVA analysis between young and old rats. As shownin Figure 3C, the intercept of the regression line in old ratswas significantly smaller compared with young rats (F_(1,10) =17.232; p < 0.002). The slope of the regression line in old ratsdid not differ significantly from that of young rats (p < 0.30)(Fig. 3B). The Pearson correlation coefficient, however, was significantlylower in old rats than in young rats (F_(1,10) = 6.96; p < 0.025)(Fig. 3B), possibly because of the reduced range of velocity inthe old rats. These results are also summarized in Figure 3A,bottom panel, which shows that the frequency of theta rhythm inold rats was lower than that of young rats at all velocities measured.It was noted that the intercept value of the theta frequency ofyoung rats is at the same level as the mean theta frequency duringREM sleep (REM, 7.30 ± 0.04 Hz; maze, 7.34 ± 0.06 Hz), suggestingthat this intercept value indeed reflects theta without the influenceof any movement. In old rats, however, the intercept of thetafrequency was slightly lower than the mean REM theta frequency(REM, 7.24 ± 0.04 Hz; maze, 6.959 ± 0.07 Hz). Therefore the ratiobetween the intercept frequency and mean frequency during REMwas calculated for each animal and compared between age groups.As shown in Figure 3D, the ratio was about 1 in young rats andslightly <1 in old rats. This ratio was slightly but significantlydifferent between the two age groups (after log transformation,F_(1,10) = 13.348; p < 0.0044).

The relationship between the amplitude of the theta rhythm and running velocity of the rats was also examined, using the sameEEG data and regression analysis. Twenty-two of 26 sessions recordedfrom young rats and 17 of 19 sessions recorded from old rats exhibitedsignificant correlations between running velocity and theta amplitude(p < 0.05; Fig. 4A). The intercept of regression lines was quitevariable, and there was no significant difference between thetwo groups (F_(1,10) = 0.625; p < 0.45) (Fig. 4C). Furthermore,there was no significant difference in the slope of regressionlines between age groups (F_(1,10) = 0.226; p < 0.64) (Fig. 4B).In addition, there was no difference in the Pearson correlationcoefficient between young and old rats (F_(1,10) = 0.00077; p <0.98) (Fig. 4B). Because the amplitude of the theta rhythm dependson the location of EEG electrodes, the REM theta was used as thereference for each animal. The ratio between the intercept valueof theta amplitude on the maze and the mean amplitude of REM thetawas calculated for each rat. As shown in Figure 4, C and D, theintercept value of the amplitude of movement-related theta rhythmwas close to the theta amplitude during REM sleep in the youngrats (i.e., the ratio is ~1). The ratio, however, was <1.0 inthe old rats. One-way ANOVA revealed a significant differencein the ratio between the two age groups (after log transformation,F_(1,10) = 10.915; p < 0.008).

Selection of complex spike cells
Of the complex spike cells (young, n = 847; old, n = 590) recorded when the animals were sleeping, 57.4% of cells from youngrats and 49.7% of cells from old rats had place fields on themaze (see Materials and Methods), whereas the others became virtuallysilent. One hundred ninety cells from young rats (18.1%) and 84from old rats (12.4%) were identified as theta cells, and allof them fired during both sleep and maze sessions. A $chi$ ² test for differences in proportions revealed a significant differencein the observed proportions of theta cells between the two agegroups ( $chi$ ² = 10.46; p < 0.0014). Twelve cells recorded from young rats andnine cells from old rats could not be placed into either categoryand were not used for data analysis. Because the EEG recordedat reward locations was mostly LIA, for which theta phase is undefined,only those place fields on the part of the rectangular track otherthan reward locations were included for further analysis; however,those cells with multiple place fields that included both rewardand nonreward locations were included in the analysis of the frequenciesof multiple fields. The numbers of pyramidal cells included foranalysis were 354 for young rats and 248 for old rats, as shownin Table 2. The amplitude and width of the spike waveforms ofthose cells with place fields on the track were similar betweenyoung and old rats (Table 3), indicating that there was no differencein the quality of unit isolation between the two age groups.

Table 2. Number of cells recorded from young (n = 6) and old (n = 6) rats while asleep and during behavior on the rectangular track

Age Cell types
No. of complex spike cells

Complex spike cells
Theta cells

No. of cells firing during sleep No. of cells on track (% active) Firing on track (% total active) Firing at food locations (% total active)

Young 847 486 (57.4) 190 354 (72.8) 132 (27.7)

Old 590 293 (49.7) 84 248 (84.6) 45 (15.4)

^a Number of cells with field locations at nonfood locations of the rectangular track versus at food locations on the track.

Table 3. Firing characteristics of complex spike cells recorded from young (n = 6) and old (n = 6) rats

Cell firing property Young (SEM) Old (SEM) F p

Amplitude (µV) 214.8 (14.1) 229.0 (30.3) 0.179 0.68

Width (msec) 0.34 (0.011) 0.34 (0.013) 0.031 0.86

Mean rate in slow-wave sleep (Hz) 0.62 (0.017) 0.62 (0.098) 0.002 0.97

Mean rate in REM sleep (Hz) 0.55 (0.045) 0.71 (0.108) 1.867 0.20

Mean rate on maze (Hz) 1.11 (0.083) 0.81 (0.103) 5.007 0.05^*

Maximum rate (Hz) 11.93 (0.61) 9.05 (1.32) 3.930 0.08

Field size (cm) 30.96 (1.34) 23.84 (2.04) 8.519 0.02^*

Field rate integral (cm × Hz) 179.1 (12.1) 134.7 (14.8) 5.395 0.04^*

No. of fields per cell 2.1 (0.1) 1.9 (0.2) 0.653 0.44

Only cells with place fields on the track are included (young, n = 354; old, n = 248). ^* Statistically significant effects.

The effect of age on general firing characteristics
There was no difference between groups in the mean firing rate during either slow-wave sleep or REM sleep before the behavioron the rectangular track (Table 3). The mean rate during behavioron the track, however, was significantly lower in old rats thanin young rats (Table 3). Old rats exhibited smaller place fieldsthan young rats (F_(1,10) = 8.519; p < 0.015) (Fig. 5A,B) and asmaller field rate integral (F_(1,10) = 5.395; p < 0.04) (Table3). This age difference cannot be attributed to the thresholdvalue (1.0 Hz) for determining the field size, because using eithera lower (0.5 Hz) or higher (2.0 Hz) threshold, the field sizesof old rats were also significantly smaller than those of youngrats (0.5 Hz, F_(1,10) = 9.809; p < 0.011; 2.0 Hz, F_(1,10) = 8.494;p < 0.015) (Fig. 5B). The differences between the means of eachgroup were similar for a given threshold cutoff value. Furthermore,in both age groups, the field size increased as the thresholdvalue decreased. This is consistent with the previous findingof Muller et al. (1987), in which a linear relationship betweenfield size and the logarithm of the threshold cutoff value wasfound. Interestingly, the ratio of field rate integral to fieldsize was almost identical, suggesting a general broadening, ratherthan a mere rate increase. The maximum firing rates were not differentbetween age groups (p > 0.05) (Table 3).
Fig. 5. Effects of age on place field characteristics. A, Representative examples from young and old rats of data from cells withsingle, double, and triple place fields on the rectangular track.The individual spikes are color-coded according to firing phaseas in Figure 1. B, Age comparison of place field sizes (computedfor separate fields over the entire recording session) using differentcutoff thresholds (0.5, 1.0, and 2.0 Hz). At all three thresholds,the field size of old rats was significantly smaller than thatof young rats (*p < 0.05). C, Frequency distribution (in percent)for the number of discrete place fields exhibited per cell ineach age group. A place field was defined as a contiguous regionof at least 10 bins with firing rates of >1 Hz. The distributionswere approximately exponential, with no significant differencebetween ages. Note that the percentages are for cells with atleast one field. Cells with no field are not included.
[View Larger Version of this Image (47K GIF file)]

It is clear that some cells have more than one place field in a given environment. Therefore, the effect of age on the numberof fields on the track was examined. Only 48.6% of old cells and40.7% of young cells had single place fields. The remaining cellshad two or more "place fields" as defined here. There was, however,no difference in the relative proportions of cells with a givennumber of fields between young and old rats (nonparametric Kolmogorov-Smirnovtest, $chi$ ² = 5.716; p < 0.11) (Fig. 5C). The average number of place fieldsper cell was 1.9 ± 0.2 in old rats and 2.1 ± 0.09 in young rats(F_(1,10) = 0.653; p < 0.44).

Effect of age on phase precession
The relationship between the firing phase and position within the field was examined as described in Materials and Methods.The phase precession of the majority of cells had a total phasechange of <360° within a given place field, although many cellshad more than one field (see Fig. 5C). A few cells (six youngand six old), however, exhibited apparent double (i.e., bimodal)fields, which overlapped spatially and in which phase precessionextended across two theta cycles. These cells will be describedin more detail elsewhere. In these cases, the precession slopewas taken as the average of the slopes within the two cycles.The mean total phase change within place fields was first averagedwithin rats and then within age groups.

The slopes of the regressions of phase versus location were significantly greater in old rats than in young rats (F_(1,10)= 6.654; p < 0.027) (Fig. 6B). There was no difference in thetotal phase change over the place field between young and oldrats (F_(1,10) = 0.092; p < 0.76) (Fig. 6C). It should be notedthat both the field entry phase and exit phase are values derivedfrom the regression lines. Because of scatter about the regressionline, the total phase change calculated from the difference betweenexit phase and entry phase is substantially <360°, although therange of actual spike phase values typically approached 360°.There was no significant effect of age on either the entry phase(young, 230 ± 8.7°; old, 227.0 ± 4.7°; U² = 0.116; p > 0.20) or the exit phase (young, 12.7 ± 20.4°; old,5.27 ± 16.1°; U² = 0.06; p > 0.05).
Fig. 6. Effect of age on phase precession and place field size. A, Phase precession plots for two representative CA1 complex spikecells, one from a young rat (blue dots) and the other from anold rat (red dots). The regression lines calculated for the youngcell and old cell are shown superimposed on the scatter plots.For illustration, the two fields have been aligned at the positionwhere the first spike occurred. The x-axis, therefore, representsthe normalized position of spike occurrence relative to that ofthe first spike within the field. Both fields start and end atapproximately the same phase. The phase advance of the spikesrecorded from the old rat, however, progresses more quickly, andthe field size is correspondingly smaller (see Fig. 5B). B, Theslope for phase versus location was significantly larger in oldrats, indicating a more rapid phase precession with distance (*p< 0.05). C, There was no difference in the total phase changeof place fields between young and old. Total phase change wastaken as the difference between entry and exit phases estimatedfrom the regression analysis. There were no differences in thecoefficients of determination for the regression lines (r²) of young and old rats.
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Expansion of place fields
It has been shown previously that place fields enlarge within a few traverses of a route even in a familiar environment (Mehtaet al., 1997). The effect of age on this field expansion was alsoexamined. The field sizes, as measured by the distance betweenthe first and last spikes in the place field of the cell, on laps1, 5, 10, and 15, were averaged for each animal [these pointswere selected on the basis of the finding of Mehta et al. (1996)that the changes in place fields saturate within a few laps].One old animal ran <15 laps, thus data on lap 15 were lacking.Two-way, repeated measures ANOVA revealed a significant effectof lap (F_(3,27) = 9.247; p < 0.0002), a significant age effect(F_(1,9) = 6.065; p < 0.036), and a significant interaction betweenage and lap (F_(3,27) = 7.591; p < 0.0008). As shown in Figure7A, for the young group, the field size increased on laps 5, 10,and 15 in comparison with lap 1. In the old group, however, thefield size remained approximately the same across laps. For lap1, there was no significant difference in the field size betweenthe two age groups (F_(1,10) = 0.296; p < 0.60). On the other hand,there were significant or marginally significant differences inthe field size on the other laps between young and old rats (lap5, F_(1,10) = 4.861; p < 0.052; lap 10, F_(1,10) = 4.792; p < 0.053;lap 15, F_(1,9) = 9.79; p < 0.012). Furthermore, the integral offiring rate within the place field of each lap was also analyzed.The field rate integral of old rats was significantly reducedcompared with young rats on laps 5, 10, and 15 (lap 5, F_(1,10)= 6.558; p < 0.028; lap 10, F_(1,10) = 19.159; p < 0.0014; lap15, F_(1,10) = 6.662; p < 0.03) (Fig. 7C), but not on lap 1 (F_(1,10)= 3.799; p < 0.08). There was a significant effect of lap on thefield rate integral in both age groups (F_(3,37) = 9.318; p < 0.0002).The percent increase of the field rate integral on laps 5, 10,and 15 relative to lap 1, however, was significantly lower inold rats than in young rats (unpaired t test, one-tailed, t =1.924; p < 0.03) (Fig. 7D).
Fig. 7. The effect of age on experience-dependent place field expansion as the animal traversed the rectangular track. A, Mean ± SEMplace field sizes for laps 1, 5, 10, and 15 of young (n = 6) andold (n = 6) rats. Although the place fields of young rats expandedsignificantly from lap 1 to lap 5 and remained at the higher levelon laps 10 and 15, those of old rats did not undergo any lap-relatedchange. B, Mean ± SEM of the slope of the phase precession asa function of lap for the two age groups. The slope was calculatedby taking the mean difference of entry and exit phases for laps1, 5, 10, and 15 for each animal, divided by the correspondingmean field sizes. There was a significant effect of age on theslope for laps 5-15 (*p < 0.05) but no effect for lap 1. C, Mean± SEM integral of firing rates within the place field for laps1, 5, 10, and 15 of the two age groups. The field rate integralof old rats was significantly lower than that of young rats onlaps 5, 10, and 15 but not on lap 1. D, Mean ± SEM of the percentincrease of the field rate integral on laps 5, 10, and 15 relativeto lap 1 in young and old rats. The percent increase of the fieldrate integral was significantly lower in old rats than in youngrats (*p < 0.05). E, The mean ± SEM of the velocity through theplace field for each lap for the two age groups. There was noeffect of lap on the mean velocity. The velocity of old rats,however, was significantly smaller than that of young rats (p< 0.0001). F, Velocity-tuning curves of firing rate for youngand old rats. This was quantified by dividing the total numberof spikes at each velocity (in 5 cm/sec bins) by the total timespent at that velocity. The overall velocity range of old ratswas smaller than that of young rats. Although, for both age groups,there was a tendency for firing rate to increase with runningvelocity, the firing rate for old rats reached a lower plateaulevel more quickly than for young rats. The arrows indicate themean velocities for the two age groups.
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The mean value of the phases of the first and last spikes of the place field for each lap was calculated for each rat usingcircular statistical methods (see Eqs. 1-3 in Materials and Methods).The difference between the mean entry and mean exit phase foreach lap was then calculated for each rat. A two-way ANOVA analysisrevealed no effect of age (F_(1,39) = 0.587; p < 0.45), no effectof lap (F_(3,39) = 0.378; p < 0.77), and no significant interactionbetween age and lap (F_(3,39) = 0.672; p < 0.57) on the phase changewithin the place field. In young rats, the lack of a significanteffect of lap on the total phase change, combined with a significanteffect of lap on place field size, indicates that the rate ofchange of phase with distance decreased across laps in young animals.Because of the small number of spikes per trial, however, it wasnot possible to obtain reliable slope functions for single cellson a trial by trial basis. Therefore, the slope was estimatedby taking the mean difference of entry and exit phases for trials1, 5, 10, and 15 for each animal, divided by the correspondingmean field sizes. The results were compared between age groups(Fig. 7B). There was a significant effect of age on the slopefor laps 5-15 (F_(1,33) = 5.513; p < 0.025) but no effect for lap1 (F_(1,10) = 0.063; p < 0.81).

The mean running velocity for each lap was also determined. A two-way ANOVA revealed a significant effect of age on mean velocity(F_(1,39) = 35.776; p < 0.0001) but no effect of laps (F_(3,39)= 0.320; p < 0.81) or significant interaction between age andlap (F_(3,39) = 0.245; p < 0.86) (Fig. 7E). Thus, the change infield size with lap number in the young rats was not attributableto any change in their running speed. There was, however, an overalleffect of running speed on firing rate, as has been shown previously(McNaughton et al., 1983a). This was quantified by dividing thetotal number of spikes at each velocity (in 5 cm/sec bins) bythe total time spent at that velocity (Fig. 7F). For both agegroups, there was a significant tendency for firing rate to increasewith running speed (F_(4,40) = 72.86; p < 0.0001); however, therelative increase was significantly less in the old animals (F_(4,40)= 20.34; p < 0.0001). Thus, the difference in mean firing ratebetween young and old rats cannot be accounted for by a differencein mean running velocity. The main effect of aging on place fieldsseems to be a failure of place field expansion during the firstfew passes through the field on a given day, leading to a smallermean place field size and firing rate in old rats.

DISCUSSION

Effect of age on experience-dependent place field plasticity
The main effect that emerges from the present study is a loss of experience-dependent plasticity in the spatial firing propertiesof aged hippocampal pyramidal cells. Old rats failed to exhibitthe expansion of place fields that normally occurs in young ratsduring the first few traversals of a route (even a "familiar"one) on a given day (Mehta et al., 1997). There was no differencebetween ages, however, in the initial size of the place fieldsand no significant difference in firing rate during either REMor slow-wave sleep. The failure of this experience-dependent expansionprovides an explanation for the earlier reports that place fields,averaged over numerous trials, tend to be smaller in old rats(Markus et al., 1994; Mizumori et al., 1996). The mechanism ofthe place field expansion in young animals is currently unknown.On track mazes it is asymmetric, in the sense that the expansionis predominantly in the direction opposite to the direction ofmotion of the rat. The firing rate near the entry point of theplace field is thus increased, whereas there is little changein rate near the exit point (Mehta et al., 1997). This characteristicwas predicted by Blum and Abbott (1996) on the basis of the temporalasymmetry of LTP induction mechanisms (Levy and Steward, 1983;Gustafsson et al., 1987; Levy, 1989). Temporal asymmetry impliesthat, as the rat passes through two adjacent points, A and B,synapses from place cells at A onto place cells at B would bepreferentially enhanced. In the model of Blum and Abbott (1996),when the animal traverses a sequence of locations, asymmetricLTP causes cells at a given location to activate subsequent cellsin the sequence, before the rat actually reaches their originalfiring locations. This causes the fields to enlarge in the directionopposite to the animal's motion. Temporally asymmetric LTP wasalso invoked by Tsodyks et al. (1996) and subsequently by Jensenand Lisman (1996) to explain the theta phase precession effect.In these models, the asymmetric modification of intrinsic connectionsis the source of the phase precession effect itself. These modelspredict that, with increased asymmetric strengthening of connections,the size of the place fields should increase asymmetrically inspace, but the net change in phase over the theta cycle shouldremain the same. This is what was observed in the young rats.As the place field expanded, there was a corresponding reductionin the rate of change of phase with position, thus keeping thenet phase change constant. Thus, place field size and phase precessionare strongly coupled.

It seems plausible, therefore, that the age deficit in place field expansion may be a consequence of a failure of an asymmetric,LTP-like process, although other explanations remain possible.The LTP deficit explanation is made more plausible by recent invitro findings on age-related deficits of LTP induction (Deupreeet al., 1991, 1993; Moore et al., 1993) and new evidence suggestingthat such an LTP induction failure in old rats may result froma reduction in the net synaptic input in old pyramidal cells (Barneset al., 1996). The latter effect may partly be a consequence ofa reduced number of functional synaptic contacts made by a givenCA3 pyramidal cell axon (Barnes et al., 1992; Barnes, 1994) orreduced temporal summation in old hippocampal cells (Rosenzweiget al., 1997). Another possibility may be the reduction in frequencypotentiation that occurs in old rats during LTP-inducing formsof stimulation (Landfield, 1988), which would also lead to a reductionin net dopolarization. Either of these changes might lead to areduced cooperativity (McNaughton et al., 1978) at a given stimuluslevel and hence less LTP. Additionally, an age-related deficitin LTP maintenance has also been found, which is significantlycorrelated with a loss of spatial memory capacity (Barnes andMcNaughton, 1980, 1985; deToledo-Morrell and Morrell, 1985; deToledo-Morrellet al., 1988). Nevertheless, until the expansion effect is demonstratedto be LTP-mediated, other explanations should be considered. Atleast one of these, however, can be excluded. It is known thatthe transition from quiesence to activity is accompanied by changesin brain temperature, and that this change is associated withalterations in hippocampal evoked potential waveforms (Moser etal., 1993). Three observations rule this temperature effect outas a possible source of the place field plasticity. First, Mehtaet al. (1997) showed that the expansion effect occurs robustlyin rats that have been running continuously for 20 min or morewhen the rats are placed on a novel track, even in cells thathad expanded fields on the familiar track. Second, the expansionis directionally asymmetric, which cannot be easily explainedby a mere excitability change. Finally, Erickson et al. (1991)studied carefully the effects of age on the behavior-induced,temperature-dependent change in evoked potentials. There was nodifference between young and old rats.

What would be the expected functional consequence of the loss of place field expansion during experience? Paradoxically, theinformation transmitted by an ensemble of neurons can be substantiallyimproved if each neuron is broadly rather than narrowly tuned(e.g., Lehky and Sejnowski, 1990; Treves et al., 1996). The lackof field broadening might thus be expected to lead to a loss ofprecision of the spatial code in old rats and can be interpretedas a failure of the hippocampal ensemble to increase the amountof spatial information it transmits as a consequence experience.The reason for this paradoxical effect can be understood in simpleinformation theoretic terms. Up to a limit, the expansion of placefields increases the number of neurons with place fields thatoverlap at any given location. Hence, the population code forlocation conveys more bits of information per second as placefields expand. Consider the two extremes of infinitely compactplace fields on one hand and of completely spatially uniform firingon the other. In both cases, there is no information about spacetransmitted by the population code. Somewhere in between thesetwo extremes, there is an optimal size of place fields, whichmaximizes the information transmitted. Roughly speaking, the theoreticaloptimum size is reached when exactly half of the population ofneurons is active at any given location. This corresponds to thecase of fully distributed coding. Fully distributed coding israrely encountered, because it is extremely inefficient from thepoint of view of information storage (as opposed to informationtransmission). Thus, systems such as the hippocampus, which arethought to be involved in Hebbian associative learning, use rathersparse coding in which only a small fraction of the cells is activeat any given time (Marr, 1971; McNaughton and Morris, 1987; Rollsand Treves, 1990). In the sparse coding regime, expansion of placefields with increased overall number of spikes, as observed inyoung rats, would increase the information transmission.

Age-related changes in hippocampal theta rhythm
Theta rhythm frequency was slightly reduced in old rats for any given running speed. There was no age effect, however, oneither the frequency or the amplitude of the theta rhythm in REMsleep. In young rats, the zero velocity intercept for both frequencyand amplitude matched the corresponding values during REM sleep.In contrast, in old rats, the zero velocity intercepts for movement-relatedtheta differed from REM theta in both frequency (5%) and amplitude(20%). Interestingly, although the correlation between the thetafrequency and running velocity was significantly decreased inthe old rats, there was no age difference in the correlation betweenthe theta amplitude and velocity. Thus, although theta frequencyand amplitude undergo reliable age-related changes, these alterationsare subtle and state-dependent.

What could account for the differential effects of age on theta frequency and amplitude during REM sleep and movement? Activationof serotonergic projections to the medial septum or hippocampusdesynchronizes and reduces the amplitude of hippocampal EEG (Macadaret al., 1974; Assaf and Miller, 1978; Maru et al., 1979; Yamamotoet al., 1979; Vertes, 1981; VanderMaelen et al., 1986; Kinneyet al., 1994; Vertes et al., 1994), and lesions of cholinergicseptal neurons also decrease theta amplitude (Lee et al., 1994).Thus, age-related dysfunction of serotonergic or cholinergic hippocampalprojections (Potier et al., 1992; Van Luijtelaar et al., 1992;Taylor and Griffith, 1993; Venero et al., 1993; Shen and Barnes,1996) may contribute to the effects of aging on the theta rhythmduring behavior.

Effect of age on the number of hippocampal CA1 interneurons
There was a significant (~35%) reduction in the proportion of theta cells recorded in the old rats. This is consistent witha recent report that the number of interneurons containing calbindinis significantly decreased in hippocampal CA1 of old rats (Potieret al., 1994), whereas the number of interneurons containing parvalbuminis preserved (Miettinen et al., 1993; Potier et al., 1994). Unfortunately,at present it is not possible to assign hippocampal interneuronsrecorded extracellularly during behavior to corresponding anatomicaland neurochemical categories, nor is there yet a sufficientlyclear picture of the role of the different types of interneuronsin either place field dynamics or the regulation of LTP to warrantserious speculation on the functional significance of a possibleloss of interneurons during aging.

Summary and Conclusions
Place field size at the beginning of a repeated, stereotyped behavioral task was not different between age groups, but theexpansion of place field size that occurred in young rats aftera few traversals was severely attenuated in old animals. Thisdifference is unlikely to be related either to changes in thetheta rhythm between age groups (which were very modest or nonexistent)or to alterations in the phase of theta at which single cellsfired during entry to and exit from their place fields. Regardlessof the exact mechanism of the attenuated place field expansionin old rats, the results suggest that the aged hippocampus failsto exhibit an experience-dependent increase in the amount of spatialinformation it transmits. The present results contribute to agrowing body of evidence suggesting that a deficit of functionalplasticity of information transmission within the hippocampuscould be a major factor in age-related memory impairment.

FOOTNOTES

Received March 19, 1997; revised May 21, 1997; accepted June 13, 1997.

This work was supported by National Institutes of Health and National Institute of Mental Health Grants AG12609 and MH01227.We thank M. Suster, R. D'Monte, and J. L. Gerrard for help withconstructing the hyperdrive, animal training, and recording, M.R. Mehta for helpful insights into data analysis strategies, andA. Treves for useful discussion.

Correspondence should be addressed to Dr. Carol A. Barnes, Life Sciences North Building, Room 384, University of Arizona,Tucson, AZ 85724

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