Excitotoxic Septal Lesions Result in Spatial Memory Deficits and Altered Flexibility of Hippocampal Single-Unit Representations

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The Journal of Neuroscience, August 1, 1999, 19(15):6661-6672

Excitotoxic Septal Lesions Result in Spatial Memory Deficits and Altered Flexibility of Hippocampal Single-Unit Representations
Stefan Leutgeb and Sheri J. Y. Mizumori
Program in Neuroscience and Department of Psychology, University of Utah, Salt Lake City, Utah 84112

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The septal nuclei are reciprocally connected with the hippocampal formation and contribute importantly to spatial and memoryprocessing. Using excitotoxic lesions of the septal area, we investigatedwhether neurodegeneration in subcortical projections to hippocampuscan compromise flexible information processing by hippocampalsingle units. In agreement with the mild effects of excitotoxicseptal lesions on hippocampal physiology compared with fimbria-fornixlesions and septal inactivation, we observed limited lesion effectson single-unit activity. The location specificity of hippocampalcomplex spike cells remained unchanged, but a less reliable location-dependentdischarge was observed in experimental animals with a pronouncedpostoperative working memory deficit. Testing in the absence ofambient illumination and in a new environment revealed that thespatial correlates of complex spike cells in lesioned animalsmay rely on a more limited set of sensory cues. Altered sensorycues resulted in a significantly different response pattern betweenthe control and lesion group in the new environment, a situationthat normally results in place field reorganization. Such a groupdifference was not observed during dark testing, a condition inwhich place field reorganization is less prominent. A contributionof hippocampal interneurons to the observed alterations in thespatial properties of the principal cells was suggested by decreasedtheta modulation in the lesioned group. Because excitotoxic lesionsresult in memory deficits that resemble age-related memory problemsin the absence of age-related degenerative processes, we suggestthat septal neurodegeneration could directly contribute to thosebehavioral changes with advanced age that correlate with functionalalterations in the hippocampalformation.

Key words: medial and lateral septum; hippocampus; place cells; spatial working memory; aging; acetylcholine; GABA projection neurons

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The septal nuclei are part of a larger brain system that supports navigational and memory functions. Disconnecting subcorticalareas, including the septum, from hippocampus by fimbria-fornixlesions or temporarily inactivating the medial septal area resultsin an impairment of spatial memory tasks (Sutherland and Rodriguez, 1989; Mizumori et al., 1990; Whishaw and Jarrard, 1995). Thesemanipulations also effectively reduce hippocampal slow wave activityin the 8-12 Hz band (theta activity) and alter the spatial correlatesof hippocampal cells. Control hippocampal complex spike cellsof rodents selectively discharge at restricted locations in theenvironment (O'Keefe and Dostrovsky, 1971; O'Keefe, 1976) andcontinue to identify the same locations when tested repeatedly(Muller et al., 1987; Thompson and Best, 1990). Fimbria-fornixlesions reduce the percentage of hippocampal units with location-dependentdischarge, decrease hippocampal single-unit activity in consistentlocations, and decrease the control of distal landmarks over thelocation of complex spike cell activity (Miller and Best, 1980;Shapiro et al., 1989). Although permanent fornix lesions affectplace fields of all hippocampal subareas to a similar extent,temporary inactivation of the medial septum and its fibers ofpassage results in disintegrated fields in only the hilar/CA3and not the CA1 subarea of hippocampus (Mizumori et al., 1989).

Septal projections to hippocampus have been implicated in contributing to memory problems of aged individuals (Markowska etal., 1995). Excitotoxic lesions of the septum produce behavioralconsequences that resemble age-related learning problems but donot alter hippocampal function as profoundly as fimbria-fornixlesions or septal inactivation (Green and Arduini, 1954; Stewartand Vanderwolf, 1987; Hagan et al., 1988; Mizumori et al., 1989,1990; Gallagher et al., 1993; Leung et al., 1994). Theta activityand acetylcholine neurotransmission are partially preserved afterexcitotoxic lesions, and the same pattern is seen with advancedage (Stewart and Vanderwolf, 1987; Leung et al., 1994; Markowskaet al., 1995). Excitotoxic lesions of the septal area may thereforebe more directly relevant than fimbria-fornix lesions or medialseptal inactivation for understanding the relative contributionof the septal area and hippocampus to age-related memory impairments.Use of the lesion technique in young animals can reveal whetherneurodegeneration in subcortical structures alters hippocampalsingle-unit activity in the absence of additional age-relatedchanges in the hippocampalformation.

We explored the hypothesis that the septal nuclei importantly regulate plasticity of hippocampal place representations, aphenomenon known to change with old age (Barnes et al., 1997;Tanila et al., 1997a,b), by recording the spatial correlates ofhippocampal complex spike cells and interneurons in freely movinganimals after septal lesions by quinolinic acid. Because earlierstudies have shown that fornix lesions decrease the dependenceof hippocampal fields on distal cues (Miller and Best, 1980; Shapiroet al., 1989), we recorded hippocampal units in the absence ofambient illumination to identify whether place fields of animalswith excitotoxic septal lesions are less dependent on well learnedvisual landmarks or whether they fail to integrate multiple sensorymodalities. A subset of the units was also recorded in a secondroom to explore whether relying on limited sensory informationcould result in a decreased likelihood of developing a distinctrepresentation for an environment that shares geometric featureswith the familiarenvironment.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects. Thirteen male Long-Evans rats were obtained from a commercial source (Simonsen Laboratories, Gilroy, CA). The animalswere 7-12 months old at the start of the experimental procedures.They were housed individually with free access to water. Foodwas restricted to maintain the animals at a minimum of 80% oftheir ad libitum body weight. Training and recording sessionswere performed only during the light phase of a 12 hr light/darkcycle.

Apparatus. An elevated eight-arm radial maze with a 19.5 cm center platform and 58 cm × 5.5 cm arms was used for trainingand recording. The proximal half of each arm was hinged and couldbe lowered by remotely controlled motors to hinder access to thedistal part of the arm, or it could be raised to the level ofthe center platform to provide access. The maze was placed ina quadratic enclosure surrounded by black curtains with a setof four visual cues, each 50 cm high and 80 cm wide, posted insidethe curtains. A second room, which resembled the familiar room,was used to test the animals in a novel environment. The mazein the second room had the same specifications as the one in thefamiliar room and was also placed in a quadratic enclosure. Fivevisual cues that were entirely different from those in the familiarroom were placed inside the curtains; two were positioned in thecorners and three were hung on thewalls.

Behavioral procedures. The animals were pretrained to retrieve chocolate milk from the end of the maze arms. During pretrainingthe animals were allowed to freely explore all eight maze arms,and the arms were rebaited when the animal had consumed the foodrewards. Training began on the day after an animal had enteredeach arm of the maze at least once. During all subsequent trainingsessions, the animals were first placed on the center platform,and a pseudorandom sequence of four arms was then presented. Onearm was initially raised and access to the next arm in the sequencewas provided when the animal had entered the previous arm. Accessto all arms was given after the fourth arm in the sequence, andthe trial was continued until the remaining food rewards had beenretrieved. Re-entries into previously visited arms were countedas working memory errors. The next trial started after the animalwas confined to the center platform for 2 min, and the sessionwas continued for a maximum of 1 hr or eight trials. Preoperativetraining continued until the animals had completed eight trialswithin 1 hr for 7 consecutive days. The animals were retrainedto the same criterion aftersurgery.

Surgery. The animals were deprived of food and water before surgery and deeply anesthetized with pentobarbital (50 mg/kg,i.p.; Nembutal, Abbott Laboratories, Chicago, IL). The level ofanesthesia was monitored continuously and additional doses (10mg/kg, i.p.) were given as needed. The skull was exposed by askin incision, and small drill holes were placed dorsal to themedial septal area and, bilaterally, dorsal to hippocampus. Theglutamate agonist quinolinate (Sigma, St. Louis, MO) was dissolvedin PBS (21 mg/ml) and injected into the medial septum [anteroposterior(AP) +0.7, lateral (L) ±0.0, dorsoventral (DV) 4.5 below dura]with a 33 gauge cannula connected to a Hamilton syringe. A volumeof 0.5 µl of either the drug or vehicle solution was infused,and the needle was left in place for an additional 5 min to limitdiffusion along the needle tract. Recording electrodes were manufacturedas stereotrodes by twisting two 20 µm lacquer-coated tungstenwires (California Fine Wire, Grover City, CA). The stereotrodeswere then coated with epoxylite, inserted into a 30 gauge stainlesssteel cannula, and cut with a pair of sharp scissors protruding~1.5 mm from the distal end of the cannula. Two or three stereotrodeswere mounted on a microdrive and placed stereotaxically at AP $-$ 3.0 to $-$ 5.0, L ±2.0-2.5, and an initial depth of 1.5 mm belowthe dural surface. A 114 µm stainless steel reference electrodewas lowered into the corpus callosum and secured to the skullalong with the microdrives by using dental cement and stainlesssteel screws. One of the skull screws served as an electricalground. Bicillin (300,000 U, i.m.) was given as an antibacterialprophylactic at the end of surgery, and the animals were allowedfree access to food and water for 1 week before again being placedon a food-restrictedschedule.

Recording procedures. The signal from each electrode was preamplified by a headstage holding an array of unity gain FET amplifiers.Incoming signals were then amplified 2,000-10,000 times by a differentialamplifier (Neurolynx, Tucson, AZ), band-pass-filtered between600 and 6000 Hz, and transmitted to an analog-to-digital (A/D)board in a pentium-based computer system. The data acquisitionprogram (Datawave Technologies, Longmont, CO) recorded a 1 msecsequence of each signal that exceeded a preset threshold (samplingfrequency: 26-32 kHz per channel). The headstage also held aninfrared light-emitting diode that was centered on the animal'shead. The infrared signal was recorded by a video camera mountedin the ceiling of the recording room. A tracking system (DragonTracker) identified the position of the animal with a spatialresolution of 256 × 256 (sampling frequency, 20 Hz). The x-y coordinatesof the animal's position on the maze were time-stamped and storedalong with the single-unitdata.

After postsurgical retraining, the animals were screened daily for single units while they were confined to the center platformof the eight-arm radial maze. All recording channels were checkedfor single units by using an audio monitor and an oscilloscope.The microdrives were advanced gradually until single units wereidentified or for a maximum of 90 µm/d. Spike discharges of individualunits were separated by using an on-line spike separation software(Datawave Technologies) that generates scatterplots of spike waveformparameters (e.g., amplitude, width) recorded on each of the twostereotrode wires. Discharges of single units were identifiedwith a window discriminator by first outlining the cluster ofspike discharges on the scatterplot showing the relative peakamplitudes and then refining the boundaries in additional projections.The data were replayed off-line, and clusters were reexaminedby using amplitude, spike width, phase angle, and waveform templatesas parameters to separate singleunits.

Behavioral testing. Daily recording sessions for each set of single units continued until visual inspection revealed thatthe cluster boundaries were different from the previous day orfor a maximum of three phases of behavioral testing. (1) Eachunit was initially recorded for eight baseline trials or, alternatively,in a sequence of 15 trials that included five trials in the standardbaseline condition (light), five trials without ambient illumination(dark), and an additional five trials with the maze lights on(lights restored). (2) Testing on subsequent days included a sessionthat began in darkness for five trials and continued in lightfor five trials. (3) After testing the units in the familiar recordingroom, a sequence of six daily recording sessions commenced thatincluded testing in a novel environment. Testing in the secondrecording room started with two baseline sessions of eight trials,each of which lasted at least 30 min, and continued with recordingsessions in the familiar and novel testing environment on alternatedays to compare complex spike cell activity in each of the testingenvironments. Single-unit activity in the novel environment wastested only once for each animal. Data are reported only for animalswith a complete sequence of recordings. The electrodes were advancedon the day when the spike amplitudes had become unstable or afterthe recording sequence was completed. A new sequence of behavioraltesting commenced when a different set of single units was encountered.When units could not be identified on any of the recording electrodes,the animals were given eight baseline sessions of spatial memorytraining at least every second day. Behavioral testing withoutrecording single units assured that asymptote performance wasmaintained in control and lesionedanimals.

Data analysis. Hippocampal complex spike cells and interneurons were identified on the basis of discharge rates and waveformcharacteristics (Ranck, 1973; Shen et al., 1997). Examinationof the peak-to-valley (negative to positive) duration of the waveformsrevealed a bimodal frequency distribution with a minimum at 250µsec. Spikes with a duration of >250 µsec and average rates of<5 Hz were classified as complex spike cells, and the validityof the criteria was confirmed by inspecting the autocorrelationhistograms. Conversely, cells with a duration of <250 µsec andmean rates of >5 Hz were identified as interneurons, and interneuronswere further subdivided into rhythmic and nonrhythmic units basedon visual inspection of the autocorrelation histograms. A smallfraction of the total number of hippocampal units did not fiteither criteria and was not furtheranalyzed.

Recording sessions were analyzed by dividing the session into trials and by eliminating data that were recorded during intertrialintervals. Place fields of hippocampal complex spike cells andlocation-dependent discharges of hippocampal interneurons werequantified by dividing the maze into 16 segments based on location(one of eight maze arms) and direction of movement (outbound orinbound). The rate was calculated by counting the number of spikedischarges for each bin, then dividing the count by occupancytime. A specificity score was calculated by dividing the highestrate by the average rate of the 15 remaining bins, and a reliabilityscore was calculated as the proportion of trials (in percent)when the maximum trial rate occurred in the same bin as the overallmaximum rate. Place fields were also quantified by binning thedata into a 64 by 64 grid with each pixel corresponding to a quadratic2.4 × 2.4 cm field on the maze. Rate maps were calculated by countingthe number of spikes at each location and dividing the spike countby occupancy time. The rate maps were used to calculate the informationcontent and covariance indices, which are designed to convey asimilar meaning as specificity and reliability, respectively,but without assuming that the fields best correspond to 16 predefinedbins. The spatial information content score was calculated asdescribed previously (Skaggs et al., 1993, Jung et al., 1994;Markus et al., 1995). The scores of the present study (see below)were consistently higher than reported previously (Markus et al.,1994, 1995). The difference may result from methodological ratherthan actual discrepancies. Preprocessing of the rate maps (Markuset al., 1995) or differences in the total number of bins (Markuset al., 1994) are likely sources for the differing numerical values.The information content score should be interpreted as indicatingfield size in log₂ units rather than reflecting information theoreticalmeasurements. Theoretical accounts of hippocampal functions havesuggested that larger field sizes may be computationally moreefficient (Samsonovich and McNaughton, 1997). The maze area inthe current recording setup corresponded to approximately 1000(or 2¹⁰) pixels, and the theoretical upper limit for the informationcontent score is 10 for a unit that is only active in exactlyone bin of themaze.

The covariance index was calculated by generating rate maps for each trial independently and then entering the rate in identicallocations as repeated observations into the statistical calculationof the covariance (Hays, 1994). If the elements of the vectorX_i correspond to the mean rate in each location and E(X_i)to the arithmetic mean of trial i, the covariance for n trialsis defined as cov(X₁, X₂, ... , X_n) = E(X₁X₂... X_n) $-$ E(X₁)E(X₂) ... E(X_n). By definition,a sequence of maps that is independent results in a zero covariance.Covariance scores greater than zero do not have a statisticallydefined meaning, but may be used descriptively for a unit's tendencyto repeatedly discharge in the same location on the maze duringa series of trials. Examination of the frequency distributionof the covariance scores of complex spike cells showed that asubset of the scores clustered around zero and that the remainingscores were widely distributed in the positive range. An arctantransform was applied to normalize the distribution, and a correspondencebetween the reliability and normalized covariance scores was confirmedby a significant correlation between the variables (r = 0.38,p < 0.001). Correlation analysis also revealed that specificitycorrelated with information content (r = 0.31, p < 0.01) and thatinformation content and the covariance index were related to theaverage rate of complex spike cells (r = $-$ 0.64, p < 0.001 andr = 0.40, p < 0.001, respectively). To ensure that comparisonsof place field properties were not confounded by firing rate,group differences in information content and covariance indexwere subjected to analysis of covariance with the average dischargerate as a covariate. Fields in novel and familiar environmentswere compared by first visually inspecting whether location-dependentactivity was observed in each of the two environments. The fieldswere classified as "unique" if only present in one of the tworooms. If fields were identified in both environments, they werefurther analyzed by rotating the rate maps in 90° steps to examinewhether they overlapped with respect to the quadratic geometryof the recording room. If overlapping in one of the four positions,the fields were categorized as "retained" or, alternatively, ifno overlap could be seen, as "shifted."

Statistical analysis. (1) Correlation coefficients were calculated to compare behavioral performance with lesion size. Theaverage number of working memory errors for all trials duringthe 7 d of postoperative retraining was used as the index forbehavioral performance. Lesion size was determined as describedbelow. (2) Correlation coefficients were also calculated for eachrecording session comparing the number of working memory errorswith the average place field parameters of the session (rate,specificity, information content, reliability, covariance index).(3) Independent t tests were used for comparing continuous variablesbetween the control and lesioned group. (4) Place field parametersof individual units were analyzed using regression analysis. Thebehavioral performance index and lesion size of each animal wereentered as independent variables, and place field parameters wereentered as dependent variables. The variability between unitsof each animal contributed to the error variance. Because regressionanalysis required that individual units of each animal be consideredfor statistical analysis, additional statistical tests of placefield parameters were also performed for individual units ratherthan individual animals. Table 1 shows that four of six controland four of five lesioned animals contributed at least 10 unitsto the total number of observations, assuring that the resultsare not attributable to the contribution of a limited number ofindividuals. (5) The proportion of theta-modulated interneurons,the proportion of units with place fields, and the response patternof the fields in novel and familiar environments were comparedusing $chi$ ² tests. (6) The dark effects on place fields were tested by usingANOVA with lesion group and testing condition as independent variables.


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Table 1. Number of complex spike cells recorded from each individual

Histology. At the end of the experiments the animals were given an overdose of pentobarbital and perfused intracardially withsaline followed by a 10% formalin solution. The brains were immersedin a 30% sucrose/formalin solution for at least 24 hr. Sections(40 µm) were taken and stained with cresyl violet. The histologicalsections were used to identify the electrode tracts and to quantifythe septal lesions. Septal lesions were analyzed using NIH Imageby measuring the volume of the septal area from the level of theisland of Calleja to the level of the decussation of the anteriorcommissure (Stewart and Vanderwolf, 1987; Leung et al., 1994).The measured septal area was delimited dorsally by the corpuscallosum, laterally by the ventricles, and ventrally by a horizontalline between the ventralmost extent of the ventricles. The striatalarea laterally adjacent to the septum was measured in identicalsections, and septal volume was expressed as percentage of striatalvolume to correct for variability in individual brain size aswell as tissue shrinkage during histologicalprocessing.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Behavioral performance and histology

Behavioral performance on the radial arm maze was not different preoperatively (Fig. 1A) (df = 11, t = 0.35, NS), but thenumber of working memory errors selectively increased in lesionedcompared with control animals during postsurgical retraining (Fig.1B) (df = 11, t = $-$ 3.87, p < 0.01). Control animals continuedto improve, but working memory errors transiently increased (Fig.1B,C) and then decreased in the lesion group (Fig. 1D) (df = 9,t = $-$ 1.63, NS). The pronounced initial spatial working memoryimpairment is characteristic for hippocampal lesions, fimbria-fornixlesions, electrolytic septal lesions, and septal inactivation(Winson, 1978; Mizumori et al., 1989; M'Harzi and Jarrard, 1992;Whishaw and Jarrard, 1995).

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Figure 1. Behavioral effects of excitotoxic septal lesions. A, Preoperative memory performance was not different among animals that were assigned to the control and lesion group as indicated by the average number of working memory errors per trial (±SEM) during the initial 7 d of training. B, The average number of working memory errors per trial (±SEM) during 7 d of postoperative retraining was higher in lesioned than in control animals. C, The average number of working memory errors per trial (±SEM) for each day of preoperative and postoperative training is shown. Initial preoperative acquisition of the working memory task was similar for control and lesioned animals. Lesioned animals showed a transient increase in working memory errors during postoperative retraining. D, Lesioned and control animals reached similar levels of asymptote performance during the recording sessions. The lesioned animals showed a small but insignificant increase in errors compared with controls. The performance during all recording sessions was averaged for each animal, and an independent t test was used for the statistical comparison. Control (CONTROL) subjects received a vehicle injection; lesioned (MSX) subjects received a quinolinic acid injection in the medial septal nucleus.

The volume of the septal area appeared reduced in lesioned animals (Fig. 2A) compared with control animals (Fig. 2B), andstatistical analysis confirmed the decreased septal volume afterexcitotoxic amino acid injections (Fig. 2C) (df = 11, t = 4.81,p < 0.001). Septal volume correlated with the average number ofpostoperative working memory errors in the experimental group(Fig. 2D) (n = 6, r = 0.821, p < 0.05), but was unrelated to postsurgicalbehavioral performance in control animals (Fig. 2D) (n = 7, r= $-$ 0.432, NS).

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Figure 2. Neurodegeneration in the septal nuclei after excitotoxic lesions. Septal volume was quantified as described in Stewart and Vanderwolf (1987) by measuring the area between the corpus callosum, the lateral ventricles, and a horizontal line between the ventralmost extent of the ventricles. A, B, Coronal sections at the level of the septal area (0.5 mm anterior to bregma) in a lesioned and control animal. Neurodegeneration after excitotoxic lesions resulted in a bottleneck-shaped appearance of the septal nuclei, which was more pronounced for cases with more severe damage. C, The average volume ratio (±SEM) was significantly smaller in lesioned compared with control animals. Septal volume is represented as the ratio of septal compared with striatal volume. D, The volume ratio correlated with the mean working memory errors per trial in the lesioned group but not in the control group. ac, Anterior commissure; cc, corpus callosum; V, lateral ventricle.

Hippocampal physiology: consequences of septal lesions

Hippocampal complex spike cells (n = 147) and interneurons (n = 46) were recorded from six control and five lesioned animals.Recordings were not obtained from one control and one lesionedanimal for which complete behavioral and histological data wereavailable. The apparent overrepresentation of interneurons comparedwith anatomically identified populations presumably resulted fromadvancing the electrodes through hippocampal layers outside ofthe stratum pyramidale and the presence of numerous nonspikingpyramidal cells in the stratum pyramidale (Thompson and Best,1989). Matching the recordings of complex spike cells to histologicallyidentified electrode tracts revealed that 104 units were recordedfrom CA1, and 43 from CA3 (Table 2). In control animals, 7 complexspike cells were recorded in baseline sessions (n = 2), and 64cells were recorded in sessions (n = 18) of 15 trials, which includedtesting in darkness. In lesioned animals, 28 complex spike cellswere recorded in baseline sessions (n = 8), and 48 cells wererecorded in sessions (n = 23) of 15 trials.


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Table 2. Hippocampal single units were classified according to their location along the electrode tract and physiological criteria

Complex spike cells
For analyzing the entire population of complex spike cells recorded in control and lesioned animals, data from the initialfive trials in light were combined with data from sessions withbaseline trials only. Two-way analysis of covariance with rateas a covariate did not reveal significant interactions betweenrecording site and lesion group for any of the field parameters.Therefore data from CA1 and CA3 were combined for statisticalcomparisons. Spike amplitudes of complex spike cells recordedfrom control and lesioned animals were not different (control155.3 ± 5.9 µV, lesioned 150.6 ± 6.5 µV; df = 144, t = 0.53, NS),and quantitative comparisons of scores for field parameters didnot reveal significant differences for specificity (log transform)(Fig. 3A) (df = 142, t = $-$ 0.44, NS), information content (Fig.3B) (df = 144, t = $-$ 1.39, NS), and reliability (Fig. 3C) (df =144, t = 0.67, NS). The covariance index was significantly decreasedin lesioned compared with control animals (Fig. 3D) (df = 141,t = 2.73, p < 0.01), suggesting that spatial correlates of hippocampalcomplex spike cells were not consistently maintained when septalfunction was compromised. The effect was controlled for rate byconfirming that the average firing rates for cells of controlanimals were not different from those of lesioned animals (0.72± 0.09 Hz vs 0.61 ± 0.11 Hz; df = 146, t = 0.77, NS) and by testingthe effect of the septal lesion by using analysis of covariancewith rate as a covariate. Analysis of covariance revealed a significantgroup effect (F_(1,141) = 4.87, p < 0.05) in addition to confirmingthe correlation between covariance index and rate (F_(1,141) =22.73, p < 0.001). The significant difference in the covarianceindex in the absence of a difference in reliability may reflectthe lower sensitivity of the latter measurement. The reliabilityscore only indicates changes to a different arm, whereas the covarianceindex is also sensitive to variations within maze arms. In addition,the reliability score only measures consistent location-dependentactivity when the units have a well defined place field, whichis not the case for a subset of the complex spike cells (see below).

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Figure 3. Location-dependent discharge of complex spike cells. Location specificity was unaffected in the lesioned group as indicated by the specificity score (A) and information content (B). The reliability score of complex spike cells (C) was not different between control and lesioned animals, but the covariance index (D), which is a more sensitive measurement for reliable location-dependent discharge (see Materials and Methods), revealed an increase in the between-trial variability for complex spike cells recorded from lesioned compared with control animals.

Proportion of units with place fields
When selecting for place fields by using similar criteria as in a previous study (Mizumori et al., 1992b), i.e., by usinga specificity score of $>=$ 2.0 and a reliability score of $>=$ 37.5%,70.4% of the units of control animals were found to have spatialcorrelates in control animals, whereas only 52.6% of the complexspike cells fulfilled the criteria for spatial correlates in lesionedanimals (df = 1, $chi$ ² = 4.89, p < 0.05). The same trend was independently observedfor control/lesion units in CA1 (69.4%/57.1%) and CA3 (77.8%/47.1%)but did not reach significance in either area separately, probablybecause of the smaller number of observations for eachcase.

Correlation analysis
When induced by neurotoxic agents, neuronal cell death in the septal area continues for several days (Stewart and Vanderwolf,1987), and the initial loss of cell populations may result inadditional structural changes attributable to compensatory processes(Cotman and Nieto-Sampredo, 1982). It has been shown, however,that the decrease in theta power after excitotoxic lesions isstable as early as 3 d after the lesion (Leung et al., 1994),and postsurgical retraining in the present study did not beginuntil >10 d after the neurotoxin injection. There were no correlationsbetween the working memory errors during a recording session andany of the measurements of location-dependent properties of thecomplex spike cells (df = 51; all p values > 0.4). Attempts weremade to correlate the behavioral performance during the acquisitionphase of the spatial memory task with the data on place fields.Although the fields were not recorded along with the impairedbehavioral performance, the initial performance during acquisitionmay measure the functional status of the septohippocampal system.In addition, lesion size was correlated with the memory performanceduring postsurgical acquisition of the memory task (seeabove).
Regression analysis revealed that both behavioral performance and septal volume were related to the covariance index (Fig.4) (F_(1,142) = 17.97, p < 0.001; F_(1,142) = 6.78, p < 0.05, respectively),but no relation to either reliability (F_(1,145) = 0.17, NS; F_(1,145)= 0.004, NS) or average rate (F_(1,146) = 2.39, NS; F_(1,146) =0.76, NS) was found. The correlation between behavioral performance,septal volume, and covariance index suggests that the septal neurons,which degenerate after the lesion, contribute to consistent location-dependentdischarge of complex spike cells in normal animals as well asthe acquisition of the spatial working memory task.

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Figure 4. Less reliable location-dependent activity of hippocampal complex spike cells correlated with the working memory deficit during postoperative retraining. A, The average covariance index (±SEM) for complex spike cells that were recorded from individual subjects is shown. B, Stereotrode waveforms and rate maps for a complex spike cell recorded from a lesioned animal. The traces in the top and bottom box represent the waveforms of individual action potentials on each of the two stereotrode wires. Rate maps for two of five individual trials are shown. The size of the circle corresponds to the rate in each location of a 64 by 64 grid, and vectors represent the direction of movement during single-unit activity. Lower covariance indices resulted from inconsistent location-dependent activity during a sequence of trials. C, Waveforms and rate maps for a complex spike cell recorded from a control animal. Consistent location-dependent activity during individual trials resulted in higher covariance scores. Calibration bars: B, 50 µV, 250 µsec; C, 100 µV, 250 µsec.

Dark effects
The contribution of visual cues to the activity of hippocampal units was tested by including dark trials in the recordingsessions. The number of fields observed in only one of the conditions(light or dark) was similar for control and lesioned animals (42.2and 41.7%, respectively). In addition, changes of the fields betweenconditions were analyzed. In control animals, 43.8% of the complexspike cells had fields in both conditions, and one-third of these(10/28) had fields in identical locations. In lesioned animals,29.2% of the cells had fields in both conditions, and 3 of 11fields were in identical locations. When the pattern of organization(identical, different, or unique to one condition) was comparedbetween conditions, significant differences in response to alteredlighting conditions were not seen (Table 3).


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Table 3. Spatial correlates during baseline conditions and in the absence of ambient illumination

Due to the smaller number of dark fields relative to light fields in the control group (Table 3), the proportion of fieldsthat were observed in the absence of visual cues was not differentfrom lesioned animals (58.5 and 47.9%, respectively, NS). Moreplace fields were seen in controls compared with lesioned animalsduring the baseline light condition (see above) and when the lightingwas restored (80.3 and 53.1%, respectively; df = 1, $chi$ ² = 9.70, p < 0.01). Changes in the place fields in darkness werealso partially reflected in the quantitative measurements of thefields properties (Fig. 5). Specificity, reliability, and covarianceindex changed with the illumination (F_(2,106) = 18.47, p < 0.001;F_(2,109) = 7.48, p < 0.01; F_(2,108) = 3.80, p < 0.05, respectively),but rate and information content remained unaffected (F_(1,111)= 0.16, NS, F_(1,109) = 0.00, NS, respectively). In addition, asignificant effect of the septal lesion on both reliability andcovariance index was revealed (F_(1,109) = 4.23, p < 0.05; F_(1,108)= 5.10, p < 0.05, respectively). Interactions were not observedfor any of the measurements (all p values > 0.1). Beginning therecording session in darkness resulted in effects (data not shown)that resembled those that were seen when dark trials were introducedafter the light trials, indicating that the initial absence ofvisual cues does not further disrupt the fields of control andlesioned subjects in the familiar environment.

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Figure 5. Location-dependent activity of complex spike cells during sessions that included baseline trials (LIGHT), trials in darkness (DARK), and trials with the lights restored (RESTORED). An effect of the septal lesion was not seen for specificity (A) and information content (B), but the overall reliability (C) and covariance index (D) were significantly higher for the control compared with the lesion group. A dark effect was observed for specificity, reliability, and covariance, but not for the information content. Interactions were not observed for any of the place field parameters.

Novel environment effects
Experience with novel environments results in a reorganization of the hippocampal representations for space (O'Keefe and Conway,1978; Kubie and Ranck, 1983; Muller and Kubie, 1987; Thompsonand Best, 1989; Wilson and McNaughton, 1993). A subpopulationof complex spike cells changes immediately in response to novelvisual cues and a different subset of cells develops fields overa time course of at least several minute. Stable recordings throughoutthe test period were obtained from two control and three lesionedanimals. Testing of place fields in the control animals (n = 8cells) indicated that the majority of fields in the control groupwas different across environments (n = 7/8); that is, cells continuedto show fields in the novel environment, but the spatial distributionof the fields differed (Fig. 6A). In contrast, the pattern ofresponses by place cells from lesioned animals (n = 9 cells) wascomparatively limited. The fields of only two of the nine complexspike cells were redistributed, whereas the remaining place fieldstended to either be identical across environments (n = 3/9) (Fig.6B) or present in one or the other environment (n = 4/9). Identicalplace fields in the two environments were seen in lesioned animalsdespite the overall inconsistency in location-dependent activityin the familiar environment (see above). A $chi$ ² test indicated that the reorganization between environments isdifferent for the control and lesion group (Table 4) (df = 2, $chi$ ² = 7.75, p < 0.05).

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Figure 6. Reorganization of spatial representations in a novel environment. A, Waveforms and rate maps for a complex spike cell recorded from a control animal are shown for the familiar and novel environment. Rate maps are oriented with the north arm toward the top of the figure. The subfield on the northeast arm was highly directional and, although in the same relative location in each of the recording environments, showed activity during inbound movement in the familiar room and activity during outbound movement in the novel room. Testing in a different environment resulted in place fields with a different spatial distribution in the majority of complex spike cells (n = 7/8) of control animals. B, Waveforms and rate maps for a complex spike cell recorded from a lesioned animal in the familiar and novel environment. The example illustrates the response of a subset of complex spike cells (n = 3/9) that showed similar fields in both environments. Others (n = 4/9) were present in either one or the other environment, and only two of nine units of lesioned animals showed the redistribution that was the typical response for the units of control animals. Calibration bars: B, 80 µV, 250 µsec; C, 100 µV, 250 µsec.


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Table 4. Comparison of place fields in the familiar and novel environment

Interneurons

Average spike amplitudes and rates of interneurons in the control and lesioned group were not different (spike amplitudes:control 99.3 ± 7.2 µV, lesioned 134.6 ± 13.8 µV, df = 43, t = $-$ 1.97, NS; rates: df = 43, t = 0.68, NS) (Fig. 7A). Autocorrelationhistograms revealed that 94.7% (18/19) of the interneurons inthe control group showed peaks in the theta range, and only 51.9%(14/27) of the units in the lesioned group showed evidence ofrhythmicity (Fig. 7B, inset, C,D) (df = 1, $chi$ ² = 9.69, p < 0.01). Comparing the peaks of the autocorrelationhistograms of theta-modulated units did not reveal a differencein the preferred discharge frequency (Fig. 7B) (df = 30, t = 1.53,NS). The decreased probability of rhythmic activity without changesin theta frequency are consistent with EEG data, which have shownthat theta amplitude, not frequency, is predominantly affectedafter excitotoxic septal lesions (Bland and Bland, 1986; Leunget al., 1994).

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Figure 7. Lesion effects on hippocampal interneurons. A, The mean discharge rate in Hz (±SEM) for interneurons of lesioned animals was not different from that of controls. B, The theta frequency of individual interneurons was estimated by measuring the mode of the peak in the 50-200 msec range in the autocorrelation histogram. The inverse of the mode was considered the predominant theta frequency of the interneuron. The mode was calculated from the subpopulation of interneurons that showed theta modulation, which was different for the control and lesioned group (as shown in the inset). C, Autocorrelation histogram (in arbitrary units) of a theta-modulated interneuron that was recorded in a control animal. D, Autocorrelation histogram of an interneuron recorded in a lesioned animal. Theta modulation was absent in 48.1% of the interneurons that were recorded along electrode tracts that also yielded recordings from complex spike cells.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Behavioral deficiency during the acquisition phase of a spatial memory task correlated with reduced septal volume after excitotoxiclesions. The increased number of working memory errors as wellas the decreased septal volume were related to less reliable location-dependentactivity of hippocampal complex spike cells, although locationspecificity was unchanged. A smaller proportion of complex spikecells with place fields was observed in lesioned compared withcontrol animals, and testing of the spatial correlates of placecells in the absence of ambient illumination showed that the numberof fields decreased in control but not lesioned animals. Conversely,a trend for a lesser degree of visual context dependence for thecomplex spike cells of lesioned animals was seen during testingin a new environment. A contribution of the interneuron populationto the functional changes in hippocampal physiology is suggestedby a significantly lower proportion of theta-modulated interneuronsin lesioned compared with controlanimals.

Septal lesion effects on behavioral performance and hippocampal physiology

Spatial working memory deficits are consistently seen after nonspecific septal lesions (Winson, 1978; Hepler et al., 1985;Hagan et al., 1988) and to a lesser extent after selective cholinergiclesions of medial septal projection neurons (Shen et al., 1996;Walsh et al., 1996; McMahan et al., 1997). Consistent with thistrend, in the present study lesion size correlated with the memorydeficit during reacquisition of the spatial memory task. Thesedata suggest that increased septal neurodegeneration results inthe expression of more severe working memory impairments. In addition,less proficient behavioral performance during the reacquisitionphase of a spatial task correlated with a decreased consistencyin location-dependent single-unit activity. The single units wererecorded, however, after the spatial working memory impairmentwas measured, at the time when the behavioral performance of lesionedanimals was similar to controls. Comparable performance duringthe recording sessions assured that our results were not confoundedby different behavioral patterns. Because the memory impairmentsthat were initially observed were sufficiently compensated for,the pattern of hippocampal single-unit activity may be a consequenceof reacquiring the task by using different strategies than thoseused by control animals, which could then result in altered hippocampalinformation processing. The prominent direct anatomical connectionsbetween septum and hippocampus would suggest, however, that hippocampalfunction is impaired as a direct result of the septal lesion andthat brain structures that are less affected by the septal lesioncan accommodate the apparent behavioralcompensation.

The lesion effects on hippocampal single-unit activity in the present study were relatively moderate compared with those thatwere described after fimbria-fornix transsections and septal inactivation.In contrast to fimbria-fornix lesions and septal inactivation,theta activity is present after excitotoxic lesions of the septalnuclei (Stewart and Vanderwolf, 1987; Leung et al., 1994), andcholinergic neurotransmission is partially preserved (Hepler etal., 1985; Hagan et al., 1988; Brandner and Schenk, 1998). Projectionsfrom hypothalamic nuclei contribute to synchronized populationactivity in the hippocampal formation (Vertes and Kocsis, 1997)and, along with the remaining cholinergic projections from themedial septum, may result in partially preserved population activity.The average discharge rate of complex spike cells was not alteredin animals with excitotoxic lesions but either increased or decreasedafter fimbria-fornix lesions (Miller and Best, 1980; Shapiro etal., 1989). Miller and Best (1980) also reported a decreased signal-to-noiseratio of place field activity. The specificity and informationcontent measurements used here would be sensitive to these changes,but lower scores were not observed after the excitotoxic lesion.Consistent findings for both types of lesion studies include decreasedreliability scores for place fields of animals with fimbria-fornix(Shapiro et al., 1989) and excitotoxic lesions. In addition, whencriteria about reliability and specificity of place fields arecombined, a decreased proportion of complex spike cells with placefields was reported for the fornix-transsected animals (Millerand Best, 1980), a result that is also seen with the excitotoxiclesion in the present study. An entirely different pattern ofresponses than with permanent lesions is observed when place fieldsare tested while the medial septal nucleus is transiently inactivated.Temporary inactivation of the medial septal area results in adecreased discharge rate of complex spike cells in the CA3/hilararea and the absence of place fields in this subregions of hippocampus.CA1 fields are unaffected by the same manipulation, indicatingthat their pattern of activity can be reestablished when the contributionfrom CA3 neurons is diminished (Mizumori et al., 1989). The differencesin hippocampal physiology after permanent and temporary deficitsin septal functions could be a consequence of compensatory changesin the relative strength of intrahippocampal inhibitory and excitatoryconnections.

Relative contribution of the septal area and hippocampus to spatial learning

The combined behavioral and physiological data suggest that functional deficits in hippocampus result in memory deficits or,alternatively, that hippocampal physiology is inconsequentialfor behavioral performance and a mere indicator of septal dysfunction.The behavioral deficit may result, for example, from a directseptal contribution to working memory using projections from thelateral nuclei to subcortical areas. In the absence of substantialevidence for a role of descending septal projections in spatialmemory performance, we argue that the effects of lesions on behaviorare likely mediated by direct septal contributions to hippocampalfunction or medial septal projections to cortical areas (e.g.,entorhinal cortex) that are connected to hippocampus. The lateralseptal nuclei could indirectly modulate hippocampal function byeither sparse direct or more prominent indirect projections tothe medial septum (Jakab and Leranth, 1995; Risold and Swanson,1997).

The medial septal nuclei have been implicated in working memory processes rather than in contributing directly to the spatialrepresentation of the environment (Givens and Olton, 1990; Givens,1996). Recent studies have also found location and directionalcorrelates in the lateral and medial septal nuclei (Ono et al.,1997; King et al., 1998). Single units in the septum could thusprovide information to hippocampus that may regulate when andwhere increased flexibility is required. We hypothesize that septallesions result in a suppression of transient increases in theflexibility of hippocampal representations, which may be necessaryto establish context dependency as well as to support workingmemory.

Reorganization in response to altered sensory cues

Changing the lighting condition does not result in new and independent hippocampal place representations in normal rats, i.e.,the representations for the light and dark conditions partiallyoverlap. Differences between the control and lesion group thereforeshould not be readily observed with such relatively minor changesin environmental conditions. Testing without ambient illuminationrevealed a similar response pattern of control and lesioned animals.Conversely, testing place fields in new environments normallyresults in a complete reorganization of the hippocampal representationin controls, and the fields of lesioned animals did not reorganizeas readily to the altered context. The latter result was recentlyconfirmed in a preliminary report showing that place fields areless likely to be reorganized in novel contexts after selectiveseptal cholinergic lesions (Ikonen et al., 1998).

Fimbria-fornix lesions also modify place field responses to changes in the sensory environment. Disrupting the constellationof visual and intramaze cues resulted in disintegrated fieldsor fields that were controlled only by intramaze cues (Millerand Best, 1980; Shapiro et al., 1989). Although the earlier resultscan be interpreted as an increased dependence of the place fieldsof lesioned animals on local cues, the present transfer teststo a novel environment would not be consistent with this interpretation.Assuming similar contributions to hippocampal dysfunction withdifferent lesion techniques, the combined findings could be interpretedas a deficit in appropriately integrating information from differentsensory modalities during periods of new learning. A specificcontribution of medial septal cholinergic neurons to the flexibleuse of hippocampal spatial representations is suggested by thefinding that acetylcholine projections are more important forworking than reference memory (Torres et al., 1994; Baxter andGallagher, 1996; Walsh et al., 1996; Shen et al., 1996) and thatacetylcholine release prevents already learned information frominterfering with new learning (Hasselmo and Bower, 1993).

Relation of the excitotoxic lesion model to aging studies

Functional changes in the aged hippocampus could primarily be a result of either degenerative processes within the hippocampalformation or compromised basal forebrain projections to hippocampus.Age-related degenerative processes in the septum involve cholinergicand noncholinergic cell populations (de Bilbao et al., 1991; Miettinenet al., 1993; Krzywkowski et al., 1995), which may contributeto, or be more consequential in the presence of, structural andphysiological changes in principal neuron and interneuron populationsof the aged hippocampus (Barnes, 1979; de Toledo-Morrell and Morrell,1985; Mizumori et al., 1992a; Shen and Barnes, 1996; Shetty andTurner, 1998). A hippocampal contribution to the spatial learningcompromise with advanced age does not result from the loss ofpyramidal cells (Rapp and Gallagher, 1996). Rather age-relatedchanges in neural plasticity of existing connections may resultin hippocampal-dependent memory disturbances. Age-related changesin the hippocampal formation include dendritic reorganization(Flood et al., 1985), loss of inhibitory interneurons (Shettyand Turner, 1998), decreased efficiency of second messenger systems(Colombo et al., 1997), changes in slow wave activity (Markowskaet al., 1995), and physiological changes in principal and interneuronpopulations (Barnes, 1979; de Toledo-Morrell and Morrell, 1985;Mizumori et al., 1992a; Shen and Barnes, 1996; Shetty and Turner,1998).

Recordings of hippocampal single units in aged freely moving animals have shown that their place fields are less flexiblethan those of young animals in situations that result in the reorganizationof hippocampal fields in younger animals, i.e., during the acquisitionof spatial memory tasks, extended exposure to familiar environments,or learning of novel visual cues (Mizumori et al., 1996; Shenet al., 1997; Tanila et al., 1997b). A decreased flexibility ofhippocampal representations in testing environments where remappingis expected was also seen in the present study after excitotoxicseptal lesions. In contrast, less consistent (i.e., more flexible)location-dependent discharge of hippocampal complex spike cellshas been observed when aged animals were repeatedly tested inan identical environment (Barnes et al., 1997). Similarly, weobserved less consistent location-dependent activity in individualswith septal lesions during continued exposure to a familiar recordingroom. Our findings in animals with compromised septal functionparallel the seemingly contradictory results in aged individualsacross test conditions. The apparent contradiction in memory-impairedaged individuals, however, could be accounted for if their hippocampalrepresentation corresponds to subsets rather than the full extentof sensory information (Rapp, 1998). We suggest that a similarexplanation could apply to the septal-lesionedanimals.

The consequences of excitotoxic lesions of the septum on hippocampal function provide evidence for a subcortical contributionto cortical information processing in the absence of additionalage-related degenerative processes in hippocampus. Behavioraleffects after nonselective excitotoxic septal lesions includespatial reference and working memory deficits (Hepler et al.,1985; Hagan et al., 1988), and these deficits are also seen inaged animal populations (Gallagher et al., 1993). In contrast,selective degeneration of cholinergic projection neurons is notsufficient for producing the same range of memory deficits (Berger-Sweeneyet al., 1994; Torres et al., 1994; McMahan et al., 1995; Baxterand Gallagher, 1996). The anatomical organization of the septalnuclei differs from other cholinergic cell groups by the additionalpresence of GABA projection neurons, which selectively projectto interneuron populations in the hippocampus (Freund and Antal,1988). Excitotoxic lesions reduce not only cholinergic neurotransmissionbut also the number of GABA neurons, in particular in the lateralseptal nuclei (Stewart and Vanderwolf, 1987; Leung et al., 1994).The combined loss of different neuron populations in septum mayresult in memory impairments that are not seen when the cholinergiccell population is selectively targeted. GABA release from subcorticaland intrahippocampal sources may serve to disambiguate the inputpatterns that are received from cortical connections (Wallensteinet al., 1998). Functionally this may serve to select referenceframes for interpreting incoming spatial information. The smallerproportion of theta-modulated interneurons in lesioned animalsindicates a direct effect of septal projections on interneuronactivity and supports the hypothesis that interneuron populationscontribute to physiological and behavioral deficits in aged animals(Mizumori et al., 1992a; Shetty and Turner, 1998).

Conclusion

Although the relation between the changes in hippocampal physiology and the working memory impairment remains to be furtherclarified, we have shown that neurodegeneration in a subcorticalstructure can importantly influence spatial information processingby an intact hippocampus. These findings indicate that compromisedseptal function may, in addition to intrinsic hippocampal degenerativeprocesses, contribute to less flexible information processingin hippocampus with advancedage.

  FOOTNOTES

Received Dec. 2, 1998; revised May 14, 1999; accepted May 14, 1999.

This work was supported by the National Science Foundation (IBN 9514880), the Human Frontiers Science Program (HFSP RG0110),National Institutes of Health (MH 58755), and a University ofUtah research fellowship. We thank Dr. Kristen Keefe for assistingwith the histological analysis and Jill Howard, Dr. Robert Marc,and Dr. Scott Rogers for their support with imageprocessing.
Correspondence should be addressed to Dr. Sheri J. Y. Mizumori, Department of Psychology, University of Utah, 390 S. 1530E. Room 502, Salt Lake City, UT84112.

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RESULTS
DISCUSSION
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