Effects of Ibotenate Hippocampal and Extrahippocampal Destruction on Delayed-Match and -Nonmatch-to-Sample Behavior in Rats

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The Journal of Neuroscience, February 15, 1999, 19(4):1492-1507

Effects of Ibotenate Hippocampal and Extrahippocampal Destruction on Delayed-Match and -Nonmatch-to-Sample Behavior in Rats
Robert E. Hampson¹, Leonard E. Jarrard², and Sam A. Deadwyler¹
¹ Department of Physiology and Pharmacology, Wake Forest University School of Medicine, Winston-Salem, North Carolina, 27157-1083 and ² Department of Psychology, Washington and Lee University, Lexington, Virginia 24450

  ABSTRACT

Top
Abstract
Introduction
References

The effects of ibotenate lesions of the hippocampus (HIPP) or hippocampus plus collateral damage to extrahippocampal structures(HCX) were investigated in rats trained to criterion on spatialversions of either a delayed-match (DMS) or delayed-nonmatch-to-sample(DNMS) task. After recovery from surgery, animals were retrainedat "0" sec delays, then assessed at 0-30 sec delays for 15 d,retrained again at 0 sec delays, and retested for another 25 don 0-30 sec delays. Pretrained HIPP-lesioned animals showed markeddelay-dependent deficits in both tasks that never recovered. Detailedexamination of within- and between-trial performance factors,including changes in response preferences, length of previoustrial delay, and sequential dependencies, revealed important factorsoperating in lesioned animals that were either absent or insignificantbefore the lesion. Pretrained HCX-lesioned animals showed deficitssimilar to those of HIPP animals, with the noticeable exceptionof a strong "recency" influence of the previous trial. Anothergroup of HIPP- and HCX-lesioned animals trained on the tasks afterthe lesion showed reduced impairments of the type described above,suggesting that extrahippocampal structures trained after thelesion can assume the role of the hippocampus to some degree.The findings indicate that both the type of lesion and the previoushistory of the animal determine the postlesion DMS and DNMS performanceof animals suffering damage to the hippocampus and/or relatedstructures.

Key words: ibotenate lesion; hippocampus; subiculum; entorhinal cortex; delay tasks; memory; training

  INTRODUCTION

Top
Abstract
Introduction
References

The effects of hippocampal lesions on delayed-match (DMS) and delayed-nonmatch-to-sample (DNMS) performance have historicallyprovided evidence of selective influences on short- versus long-termmemory processes (Correll and Scoville, 1965; Olton and Feustle,1981; Rawlins, 1985; Parkinson et al., 1988; Raffaele and Olton,1988; Zola-Morgan et al., 1993; Shaw and Aggleton, 1995). In recentyears the validity of this assumption has been repeatedly testedwith respect to the species of animal (Aggleton and Mishkin, 1985;Rothblat and Kromer, 1991; Gaffan and Murray, 1992; Rawlins etal., 1993), type of delay task used, (Parkinson et al., 1988;Dunnett, 1989; Rothblat and Kromer, 1991; Rawlins et al., 1993;Steele and Rawlins, 1993; Cassaday and Rawlins, 1995), numberof choices available (Angeli et al., 1993; Gutnikov et al., 1994),type and extent of the lesion (Aggleton and Mishkin, 1985; Aggletonet al., 1989; Jarrard, 1989, 1993; Coffey et al., 1990; Rawlinset al., 1993), nature of stimuli used (Angeli et al., 1993; Yeeand Rawlins, 1994; Cassaday and Rawlins, 1995), and methods ofscoring the data (Ringo, 1991; Steele and Rawlins, 1993).

Several of these issues can be reduced to four important aspects of DMS and DNMS behavior that have yet to be unequivocallydetermined in animals that have damage to the hippocampus andrelated structures. The first is whether the deficit in DMS andDNMS performance reported with lesions of the hippocampus is trulydelay-dependent, i.e., increased impairment (relative to controllevels) as length of delay interval is increased (Ringo, 1991;Alvarez-Royo et al., 1992; Zola-Morgan et al., 1993). The secondissue is whether animals with selective hippocampal lesions actuallyperform the task in the same manner that they did before the lesion.In such instances plotting the data in the same manner for pre-versus postlesion conditions can obscure qualitative differencesin performance and possibly mask more severe deficits in the lesionedanimal (Dunnett, 1989). The third issue regards the nature andextent of the damage and whether the deficits that are reportedare caused by isolated involvement of the hippocampus and/or damageto adjacent structures and fibers of passage (Jarrard, 1993; Murrayand Mishkin, 1998). Finally, are the same deficits observed inanimals that are pretrained on the task before the lesion versusthose trained after the lesion (Irle and Markowitsch, 1990; Ridleyet al., 1996; Maren et al., 1997)?

In the following report we demonstrate that selective lesions of the hippocampus that spare other structures and preservefibers of passage severely disrupt performance on operant-spatialDMS and DNMS tasks. The lesion-produced disruption was specificto (1) hippocampal versus hippocampal plus collateral retrohippocampalinvolvement, (2) the length of delay interval, (3) factors operatingwithin versus between trials, and (4) whether the animal was pretrainedon the task at the time of the lesion. The data support the conclusionthat the hippocampus is critical for successful performance inthis version of the DMS and DNMS task as suggested in previouselectrophysiological investigations (Deadwyler et al., 1996; Hampsonet al., 1998a,b).

  MATERIALS AND METHODS

Subjects. Forty-one male Spraque Dawley rats ranging in age from 150 to 200 d at the initiation of training were used as subjects.The time of surgery and the time of training were interleavedover multiple stages in which different groups of animals (usually6-10 per group) were trained, lesioned, and tested over severalmonths. All animals were trained to the same criteria before surgery,except in the case of the "naive" group that only received trainingon the task after surgery. Several subjects were eliminated inthe early stages of the study as a consequence of adjustmentsto the ibotenate lesion protocol, age of the rat, and variationsin quality of thetoxin.

Apparatus. The apparatus was similar to that used in other studies from this laboratory (Hampson et al., 1993; Deadwyler etal., 1996). Briefly, all studies were conducted in 43 cm × 43cm × 53 cm Plexiglas behavioral-testing chambers with manipulandaand other features described previously (Deadwyler et al., 1996).The entire apparatus was housed inside a commercial sound-attenuatedcubicle (Industrial Acoustics, Bronx, NY). On one wall of thechamber, two retractable levers (Coulborn Instruments, LehighValley, PA) were positioned 3.5 cm above the floor and separatedby 14.0 cm (center to center). A water dispenser trough was positionedmidway between the levers. A nosepoke device, consisting of aninfrared photodetector and light-emitting diode spanning a 2.5cm × 1 cm × 1 cm opening in an aluminum housing, was mounted 4.0cm above the chamber floor on the wall opposite the levers witha cue light (6 V; 10 W) positioned immediately above it. A speakermounted on one wall provided a constant 85 db "white noise" background.Two 12 V, 25 W incandescent lamps (house lights) were mountedon the top of the chamber. Video monitoring of the animal wasprovided by a Sanyo CCD black-and-white video camera mounted abovethe chamber. The apparatus was controlled by a personal computerthat collected all behavioral data, which were subsequently storedon hard drives and then archived to opticaldisks.

Behavioral training procedure. Animals were water-deprived and allowed free access to food for maintenance at 85% of theirweight throughout the duration of DMS and DNMS training (Hampsonet al., 1993). Periodically animals were given water and foodad libitum, and a new weight was calculated to allow for normalbody growth. Before each behavioral session, all animals weretypically water-deprived for 20-22 hr. The DMS and DNMS taskswere similar to those described previously by Hampson et al. (1993)and Deadwyler et al. (1996), respectively. Delay interval respondingwas performed via a nosepoke device on the wall opposite the leversso that animals could not use orienting strategies to code leverposition during the delay intervals (Chudasama and Muir, 1997).

Pretraining in both tasks was as described in Hampson et al. (1993). Briefly, the task consisted of three main phases: sample,delay, and match or nonmatch. At the initiation of a trial, eitherthe left or right lever was extended, and the animal was allowedto respond on the extended lever (sample response) while the otherlever remained retracted (Fig. 1, sample). The sample lever wasthen retracted, and the delay phase was initiated (Fig. 1, delayinterval) and varied randomly on any given trial from 0 to 30sec. During the delay the animal was required to nosepoke in thephotocell device, mounted on the opposite wall, in the presenceof the adjacent illuminated cue light; nosepokes shut off thelight on a variable interval schedule the average of once every16 sec in conjunction with the delay contingency. At the terminationof the delay interval, if a nosepoke occurred during the delay,the cue light was turned off, and both levers were extended intothe chamber, signaling onset of the match or nonmatch phase ofthe task (Fig. 1). The animal was then required to press eitherthe same [match (DMS)] or opposite [nonmatch (DNMS)] lever comparedwith the previous sample lever response (Fig. 1, correct lever).If successful, the match or nonmatch response produced a distinct"click" of the solenoid valve that delivered a drop of water tothe trough located between the two levers (Fig. 1, water reward).The levers were then retracted for a 10 sec intertrial interval(ITI). Note that Figure 1 also illustrates that performance ofa DMS-type response pattern would constitute an error for theDNMS task, and performance of a DNMS pattern results in an errorfor the DMS task. On error trials, inappropriate responding wasfollowed by an immediate 5 sec time-out period in which all lightswere turned off and the levers were retracted, leaving the chambercompletely dark for 5 sec. The chamber lights were then turnedback on, and 5 sec (10 sec ITI) later the next trial was initiated.A new trial always commenced with the extension of one of thetwo levers (right or left) in the sample phase after a 10 secITI. Daily training and testing sessions typically consisted of100-150 trials.

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Figure 1. Diagram showing apparatus and contingencies for DMS (top) and DNMS (bottom) tasks. The middle box (Delay Interval) shows that the delay is the same for both types of tasks and consists of requisite nosepokes during the duration of the delay period. Typical behavior is for the animal to nosepoke through the entire delay period of 0-30 sec while the cue light is illuminated. Note that the DMS-type trial constitutes an error if the animal is performing the DNMS task and vice versa. For the Sample phase of the task, the dark lever is the only one presented and to which the animal can respond. For the Match or Nonmatch phase of the task, the dark lever is the correct response to the two levers that are extended simultaneously into the chamber at the end of the delay interval.

Animals were trained to a criterion of >90% correct responses during sessions of 100 trials with "0" sec delays that essentiallyconsisted of performing the required response sequence [i.e.,sample, nosepoke, and match or nonmatch (Fig. 1)] without interruptionby a perceptible delay interval between the sample and match ornonmatch responses. They were then trained on trials with delaysthat varied randomly between 0 and 15 sec (5 d) and then 0 and30 sec until a final criterion of >85% correct responding on trialswith delays of $<=$ 5 sec was met by all animals (i.e., no performancecriterion was set for trials with delays of >5 sec). Before thelesion, equal numbers of animals were trained to the same criteriaon either task, which required approximately the same number ofdaily sessions (DMS = 12.1 ± 0.9 sessions; DNMS = 17.3 ± 1.1 sessions;mean ± SEM). A second group of animals received either DMS (n= 4) or DNMS (n = 4) training after the lesion (naive-lesionedanimals). A third group (n = 4) received training on just leverresponding without the discrimination or delay components beforethelesion.

Lesions. The surgical procedures used to administer ibotenate lesions of the hippocampus were similar to those described elsewhere(Jarrard, 1989). Specifically, the animals were anesthetized witha mixture of chloral hydrate and sodium pentobarbital and placedin a Kopf stereotaxic apparatus; then an incision was made inthe scalp, and the bone overlying the hippocampus was removed.Injections of ibotenic acid (IBO) were made with a 5 µl Hamiltonsyringe mounted on the stereotaxic frame and held with a Kopfmicroinjector (Model 5000). A glass micropipette was glued ontothe end of the needle of the syringe to minimize damage to overlyingneocortex. The IBO was dissolved in PBS, pH 7.4, at a concentrationof 10 mg/ml. Injections of 0.1 µl (0.05 µl at several sites) weremade over ~30 sec at each of 26 sites (for stereotaxic coordinates,see Jarrard, 1989). The pipette was left in place an additional30 sec to prevent spread up the pipettetrack.

Ibotenate lesions were administered to 24 animals that survived surgery and testing. Animals were classified with respectto the extent and completeness of hippocampal damage into twomain classes, (1) complete hippocampal removal (HIPP) or (2) hippocampalremoval plus collateral damage to retrohippocampal structures(HCX). After evaluation of the lesion, the above groups were furthersubdivided by type of lesion and task for finalanalyses.

Postlesion testing. Testing was commenced 1-2 weeks after surgery after the animals had regained their prelesion body weightlevels. For animals pretrained to criterion on the DMS and DNMStasks, initial postlesion testing consisted of 5-7 d of trainingon the task with a 0 sec delay period. All animals reached a 100%criterion performance within 5-7 d on the 0 delay version of thetask. They were then directly exposed to daily sessions consistingof trials with 0-30 sec delays for the same number of successivedays that they were trained before the lesion (see above). Afterthis, another 7-9 d of training with only 0 delay trials was interjectedbefore animals were tested again under the 0-30 sec conditionfor an extended period (24 d) to determine whether they couldregain prelesion performance levels. All daily sessions consistedof 100-120 trials. Animals lesioned before training (naive-lesionedgroup) were trained in the same manner as were the pretrainedanimals (see Behavioral Training Procedure), and the number ofdays to reach criterion performance was noted for eachanimal.

Behavioral data analyses. Assessment of behavioral data consisted of several different analyses designed to elucidate thedeficits produced by removing the hippocampus. The two primarymeasures used to test pre- to postlesion differences were meanpercent correct performance over the entire session for each typeof trial (i.e., left or right) and mean percent correct performanceat each delay interval, assessed in 5.0 sec intervals. Additionalmeasures included time of execution of the trial, influence ofprevious trial delay, and the number of daily sessions to recovercriterion performance. Multifactor ANOVAs were used for most tests,and adjusted pairwise linear comparisons were used for individualcomparisons. The consistency in the data suggests that data fromanimals within the same groups tested at different times did notinfluence theresults.

Histology. After completion of behavioral testing, all animals were administered a lethal dose of pentobarbital and perfusedwith physiological saline followed by formalin. The brains wereremoved from the skull, embedded in egg yoke, and cut into 40µm coronal sections on a microtome. A cresyl violet stain wasused to determine cell loss attributable to the lesion, and selectedsections were stained with the Fink-Heimer silver staining procedure(Fink and Heimer, 1967) to identify degenerating axons and argyrophyliccells. The extent of hippocampal cell loss together with any encroachmentinto adjacent structures was determined by visual inspection (Jarrard,1991). In addition, preservation of fibers of passage and othernoncellular structural changes were evaluated (Jarrard, 1989).

  RESULTS

Histology

The nature and extent of the brain damage resulting from ibotenate lesions of the hippocampus can be seen in Figure 2. Thephotomicrographs are of cell-stained sections taken from threerostrocaudal levels through the hippocampus. Evaluation of theresulting damage indicated that in some animals the damage waslimited to the hippocampus (CA1-CA3 pyramidal cells, dentate granulecells, and interneurons), but there were some that had, in additionto the removal of the hippocampus, bilateral damage that includedadjacent retrohippocampal areas (subiculum, pre- and/or parasubiculum,and/or entorhinal cortex). Thus, for purposes of behavioral analysis,animals were subdivided into two groups: those that had the hippocampusremoved selectively (HIPP group, n = 12) and a group that receivedcollateral damage to retrohippocampal areas in addition to completeremoval of the hippocampus (HCX group, n = 6). Representativelesions from the HIPP and HCX groups and an intact control brainare shown in Figure 2.

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Figure 2. Representative ibotenate lesions for hippocampal (Hippocampus or HIPP, center) and retrohippocampal (HCX, right) groups, compared with the brain from an intact animal (Control, left). The spaces devoid of hippocampal tissue are filled in some cases with the embedding material so that region of the section appears darker than regions where there is no material adhering to the section. Further description is in text.

Histological evaluation of the resulting damage indicated that most of the animals had essentially complete removal of thepyramidal (CA1-CA3) and dentate granule cells at all rostral-caudallevels of the hippocampus (see Fig. 2). Although there were severalanimals in this group that had some sparing of pyramidal cellsand/or dentate granule cells, these cells were few in number andwere confined mostly to the ventral hippocampus. Furthermore,there was an absence of obvious damage to the subiculum and adjacentretrohippocampal areas (HIPP-lesioned animals). As can be seenin Figure 2, there was considerable atrophy of the hippocampus;however, the axons normally found in the fimbria and fornix couldbe seen clearly, forming a tight bundle of fibers coursing alongthe dorsolateral edge of the thalamus. It was shown in previousresearch that these axons could transport horseradish peroxidase,and these axons are thus assumed to be still functional afterthis kind of lesion (Jarrard, 1989). The damage described aboveis essentially similar to that found in other experiments in whichthe same surgical procedure was used (Jarrard and Davidson, 1994;Jarrard, 1995).

In addition to loss of cells that form the hippocampus, animals in the HCX group had damage that was bilateral and extendedin a caudal direction to include neurons in several adjacent retrohippocampalareas (subiculum, pre- and/or parasubiculum, and/or entorhinalcortex). Although the exact nature and extent of this additionaldamage did vary from animal to animal, the common feature wasthat the damage was more extensive than in HIPP rats and includedareas that are afferent and/or efferent to thehippocampus.

Effects of hippocampal removal on DMS or DNMS performance

For behavioral analysis, animals in the HIPP and HCX groups were further divided into subgroups based on pretraining or nopretraining and type of task. Thus, two major groups consistedof animals with HIPP lesions pretrained to criterion on the DNMSor DMS task and retested after recovery from surgery. Two otherHIPP-lesioned animals (n = 2) did not receive pretraining on eitherthe DNMS or DMS tasks. These animals were naive when trainingcommenced after surgery (seebelow).

Two groups of six rats each were trained on the DMS or DNMS tasks before surgery and had lesions limited to the hippocampus(HIPP lesion). Data were analyzed with respect to three main factorsthat characterized the lesion deficits including (1) alterationin the delay dependence of DMS or DNMS performance (Hampson etal., 1998a), (2) qualitative differences in the degree of proactiveinfluence from the previous trial (Deadwyler et al., 1996; Hampsonand Deadwyler, 1996b), and (3) presence of a response bias, orpreference, for a particular trial type (Deadwyler et al., 1996).

Effects on DMS performance
Figure 3A shows overall pre- versus postlesion mean performance for all pretrained HIPP-lesioned animals in the DMS (0-30sec delay) task. Mean overall DMS performance decreased afterthe lesion from 81 to 73% [F_(2,327) = 48.21; p < 0.001]. The decrementwas delay dependent, larger at longer than at shorter delays [F_(1,1263)= 8.12; p < 0.01], and was consistent across animals (see Fig.3A, inset) as well as trials. There were no significant differencesin pre- versus postlesion performance on trials with 0 sec delay(Fig. 3A).

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Figure 3. Comparison of pre- and postlesion performance of HIPP-lesioned animals in the DMS and DNMS tasks. A, DMS trials were sorted by pre- and postlesion performance according to length of delay on individual trials and were grouped according to 5 sec intervals (1-5, 6-10, 11-15, 16-20, 21-25, and 26-30). Trials with 0 sec delays are plotted as a separate point to indicate performance levels with no apparent delay between sample and match or nonmatch phases of the task (see text). Prelesion (n = 11 sessions) and postlesion (n = 11 sessions) performance was averaged across trials, sessions, and animals (n = 6). Each symbol thus represents the mean (± SEM) percent of correct trials performed within each delay across sessions. Prelesion performance was calculated from 0 to 30 sec delay DMS sessions immediately before surgery. Postlesion performance was calculated from the same number of 0-30 sec delay sessions immediately after surgery. Inset, The mean of each individual animal's performance at each delay is shown such that the variability reflects differences between animals in the group. B, DNMS trials were sorted as in A by pre- and postlesion performance according to length of delay on individual trials. Prelesion (n = 15 sessions) and postlesion (n = 15 sessions) performance was averaged across trials, sessions, and animals for six animals that received ibotenate lesions confined to the hippocampus. Each symbol indicates the mean (± SEM) percent of correct DNMS trials performed within each delay across sessions. As in A, prelesion and postlesion DNMS performance was calculated for the same number of 0-30 sec delay sessions immediately before and after the lesion surgery. Inset, The mean performance at each delay averaged across animals is shown.

Because it was known that DMS and DNMS task performance in intact animals was influenced by different trial sequences (Hampsonet al., 1995; Hampson and Deadwyler, 1996b), analyses of individualtrial-type performance were performed on pre- and postlesion data.Figure 4A shows pre- and postlesion performance sorted by "preferred"versus "nonpreferred" trials, a measure that accounted for differentialresponding on each of the two trial types [left (L) or right (R)]in the DMS task. Preference was defined by the position of thesample lever (L or R) at the start of the trial. Hence a preferred(P)-type trial was defined as that with the higher average successrate during the session. The analysis revealed a modest [F_(8,881)= 2.75; p < 0.01] difference (15%) in intact animals with respectto performance on preferred (mean = 88.7%) versus nonpreferred(mean = 73.6%) trials. A major difference in this measure wasthat before the lesion, trial preference was quite inconsistentacross different sessions, as reflected in fluctuating mean differencesfrom day to day (see multiple curve crossings in Fig. 4A, Prelesion).After surgery (Fig. 4, L), the trial preferences of HIPP-lesionedanimals remained consistent from day to day over all postlesiontest sessions (Fig. 4A). If sessions with only 0 sec delay trialswere administered (Fig. 4A, days 1-5 Postlesion), preference wasminimized. On sessions with 0-30 sec trials, the mean separationin performance on preferred versus nonpreferred trials was markedlyincreased relative to pretraining levels [preferred trial mean= 83.9%; nonpreferred trial mean = 59.6%; F_(8,881) = 4.45; p <0.001].

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Figure 4. DMS performance in pretrained HIPP-lesioned animals. A, Mean performance in the DMS task for six animals was sorted by left or right sample lever trials and calculated across daily sessions of 100 trials. Each symbol represents the mean performance of a single DMS session; error bars indicate the largest SEM for each curve. Preferred lever represents either left or right lever sample trials sorted on an individual animal basis, to indicate the trial type with a higher percent correct during the session. Nonpreferred (Non) trials were those performed on the opposite sample lever within the same session. Animals were trained to criterion (>85% correct on trials with $<=$ 5 sec delays) for 11 d (Prelesion) and then received ibotenate lesions (dashed vertical line labeled L). After postoperative recovery (Postlesion), animals were trained for 5 d in the DMS task with 0 sec delays and then for 11 d at 0-30 sec delays. To test postoperative recovery further (2nd Postlesion), a second set of 0 sec trial delay (5 d) and then 0-30 sec trial delay (24 d) sessions were conducted (dotted vertical line at R). Preferred and nonpreferred trial types were determined independently within each daily session. B, DMS performance over the same sessions shown in A was sorted into groups of trials with delays of 1-10, 11-20, or 21-30 sec. Each symbol represents the mean number of trials within each group over each daily session. Trials were not sorted according to preference. For 0 sec trial delay sessions (unfilled squares), all trials are shown. Pre- and postlesion sessions, means, and SEMs are as described in A.

Figure 4B shows mean pre- and postlesion DMS performance of pretrained HIPP-lesioned animals as a function of short (1-10sec), intermediate (11-20 sec), and long (21-30 sec) delay trials.Postlesion mean performance on sessions with 0 sec delays wasclearly not impaired, and the ranking and the relative difficultyof the three delay categories remained the same as that in prelesiontests. There was, however, a significant reduction in pre- versuspostlesion performance in all three delay categories [F_(8,821)= 4.18; p < 0.001] that never recovered, even over the extended(second 24 day) testing period (Fig. 4B).

Effects on DNMS performance
Figure 3B shows the performance of the group of pretrained HIPP-lesioned animals (n = 6) on the DNMS task. The overall postlesionreduction in DNMS performance was from 79% (pre) to 71% (post)across all delay intervals. As with the DMS task, performancedecreased significantly [F_(2,327) = 35.97; p < 0.001] in a delay-dependentmanner after the lesion, with longer delays producing more ofa deficit relative to prelesion performance. Also as with theDMS task, the effect across animals was consistent (see Fig. 3B,inset) with the analysis across trials, while postlesion performanceon the 0 delay version of the task was unaffected (Fig. 3B). Theanalysis of performance on preferred (mean = 87.2%) versus nonpreferred(mean = 74.5%) trials (Fig. 5A) also revealed a significant [F_(8,881)= 2.39; p < 0.01] prelesion difference (12%) that increased (23%)after the lesion (preferred mean = 78.8%; nonpreferred mean =55.6%). As with the DMS task, the preferences of HIPP-lesionedanimals were fixated and remained the same across all postlesiontest sessions. The effect of the lesion at different delays wasalso similar to that of the pretrained HIPP-lesioned DMS groupin that performance was significantly reduced (by ~10%) in eachof the short, intermediate, and long delay categories in the first[F_(2,327) = 39.8; p < 0.001] and second [F_(2,327) = 19.4; p <0.001] postlesion test periods (Fig. 5B). A comparison of pre-and postlesion performance between the DMS and DNMS groups revealedno significant differences [F_(8,881) = 0.29, NS]; however, therewas the suggestion of a trend in postlesion improvement on 11-20sec delay trials in the DNMS group that was not present in theDMS group (compare Figs. 4B, 5B). Across all pretrained HIPP-lesionedanimals, irrespective of task, mean performance was considerablyreduced at delays of >5.0 sec [F_(8,1026) = 3.49; p < 0.001] comparedwith prelesion levels. In addition, the difference in performanceon preferred versus nonpreferred trials for both tasks was significantlymagnified relative to prelesion levels [DMS, 24%; DNMS, 24%; F_(8,881)= 4.51; p < 0.001].

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Figure 5. DNMS performance in HIPP-lesioned animals. A, Mean performance in the DNMS task for six animals sorted by left or right sample lever trials and calculated across daily sessions on 100 trials. Plots of differential trial performance were constructed and preferred and nonpreferred trial types determined independently within each set of 0 or 0-30 sec delay sessions from the percent correct of each trial type as described in Figure 4A. Animals were trained to criterion in the DNMS task at 0-30 sec delays before lesions (Prelesion) and then for 5 d at 0 delay after lesions (Postlesion). An initial set of 16 d at 0-30 sec trial delays and then a second set of 0 sec delay (5 d) and 0-30 sec trial delay sessions (24 d) (2nd Postlesion) were conducted (dashed line at R). Each point represents the mean overall performance on a daily DNMS session, with the largest SEM within each curve indicated by the error bars as described in Figure 4A. B, DNMS performance over the same sessions shown in A sorted into groups of trials with delay lengths of 1-10, 11-20, or 21-30 sec. Trials were sorted as described in Figure 4B. Pre- and postlesion sessions, means, and SEMs are as described in A.

Interactions with trial sequence

Prelesion influence
Previous studies of DMS and DNMS performance in intact animals showed proactive influences from different trial sequences(Hampson and Deadwyler, 1996b; Hampson et al., 1998a). The performanceof HIPP-lesioned animals was assessed using similar analyses todetermine whether proactive influences differed after the lesion.Trials were grouped and sorted into categories depending on whetherthey were (1) preferred (P) or nonpreferred (N) and (2) precededby a preferred or nonpreferred trial. This gave rise to four categoriesof trial doublets (P-P, N-N, N-P, and P-N; e.g., P-N, a nonpreferredcurrent trial preceded by a preferred prior trial) for which performancecould be plottedseparately.
Figure 6, top left, shows the prelesion behavioral performance of all HIPP-lesioned animals in both the DMS and DNMS tasks,segregated into the above four combinations of preferred and nonpreferredtrial sequences. As reported previously for intact animals (Deadwyleret al., 1996; Hampson and Deadwyler, 1996b), the major factorinfluencing performance was whether the previous trial was thesame (P-P, N-N) as, or different (P-N, N-P) from, the currenttrial. The proactive influence of same versus different trialswas not present on trials occurring within 25 sec (including ITIof 10 sec) of the previous trial. The divergence in performanceon same versus different trials in intact animals as trials becameseparated by >25 sec (Fig. 6, top right) is not a primacy or recencyeffect (Bolhuis and Van Kampen, 1988; Gaffan and Gaffan, 1992).Rather, the separation results from a shift in response strategythat only occurs after errors on long-delay trials (i.e., a long-delayerror or LDE; Deadwyler et al., 1996). Sequential trial analysesshowed that animals can minimize the likelihood of a "repeat error"after an LDE if they respond as if the opposite trial type (tothe LDE) is going to occur on the next trial. This maximizingstrategy produces the same/different segregation (Fig. 6, topright) and results in a reduced likelihood of a second error,especially if the next trial encountered has a long delay (Hampsonand Deadwyler, 1996b). After implementing the strategy, intactanimals perform the next trial in the task in accordance withthe DMS/DNMS contingency. This maximization strategy is the onlysequential dependency that has been identified in intact animalsin this version of the DMS/DNMS task (Hampson et al., 1998a,b),and it was clearly exhibited in prelesion performance by all animalsthat subsequently received either type of lesion.

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Figure 6. Comparison of preferred and nonpreferred trial influence in pretrained HIPP-lesioned animals. Top left, DMS and DNMS trial performance in 12 trained, nonlesioned animals (11 sessions) sorted according to the delay interval of each trial in 5 sec increments as described in Figure 3. Data were additionally sorted by sample lever position in the current and preceding trial. After trials were sorted according to sample lever position, the set of trials with higher mean performance was termed the preferred lever type (Pref), and the set with lower performance the nonpreferred lever type (Non). Trials were additionally sorted according to whether the preceding trial was the same (i.e., Pref-Pref and Non-Non, filled symbols) or different (Pref-Non and Non-Pref, unfilled symbols). The mean (± SEM) within each delay and trial type is plotted. Note that P-P and N-N trials had were higher in performance than P-N and N-P trial sequences, but there was no difference as a function of P versus N trials. The dashed line indicates the mean performance over all trials. Top right, DMS and DNMS trial performance in the same trained, nonlesioned animals analyzed on the left sorted according to Pref and Non trial type on the current and preceding trial and graphed as a function of time since the preceding trial (ITI of 10 sec). Delays were sorted into 5 sec increments to match the range of delays on the previous trial. The separation in performance for same versus different trials after long delays indicates the influence of proactive interference on the trial after a long-delay error. Middle left, Postlesion DMS and DNMS trial performance in the same 12 animals (11 sessions) with HIPP lesions. Trials were sorted according to Pref versus Non trial types as described above. Note that postlesion trial performance was influenced by lever preference as well as by proactive influences. Middle right, Performance for HIPP-lesioned animals over the same trials shown at left, except sorted by time since the preceding trial. Note the influence of lever preference on P-P and N-N trial sequence with no change in performance across delay, compared with the reversal shown by P-N and N-P trials (see text). Bottom, DNMS trial performance in two animals (16 sessions) with HIPP lesions that were not trained (Naive) before the lesion. Trials were sorted as described above with the current trial delay on the left and the time since the last trial on the right. Note in both panels that the influence of lever preference was greater than its associated proactive effect on the next trial (see text).

Postlesion influences
After ibotenate lesions that successfully removed only the hippocampus in pretrained (HIPP-lesioned) animals, proactive influenceswere assessed based on the above trial preferences and sequentialinfluences. A major effect of the lesion in both the DMS and DNMStasks related to a shift in the dominance of preferred (P) versusnonpreferred (N) previous trial influence (instead of same ordifferent) on the next trial (Fig. 6, middle). Performance inpretrained HIPP-lesioned animals was not homogenous with respectto similarity of trial type. For instance, when a preferred trialfollowed a preferred trial, performance was maximized at all delayintervals (Fig. 6, middle left, Pref-Pref). Inspection of thedata revealed that this occurred most often when short-delay Ptrials followed correct P trials of any delay length. In contrast,performance on N-N trial sequences was never above chance if trialshad >5.0 sec delays (Fig. 6, middle left, Non-Non), irrespectiveof how far in time the two trials were separated (Fig. 6, middleright, Non-Non). Thus, performance was segregated along a completelydifferent behavioral dimension than before thelesion.
An overall probability of 73% correct on any given trial was the result of a differential distribution of 78% correct on preferredtrials and 68% correct on nonpreferred trials. In circumstancesin which the current trial differed from the previous trial (i.e.,P-N or N-P sequences), performance in pretrained HIPP-lesionedanimals was strictly a decreasing function of length of the delayon the current trial (Fig. 6, middle left, Pref-Non). This resultedfrom a tendency to shift responding to the P type (see below)if the delay exceeded 15 sec. The most influential trial sequencein pretrained HIPP-lesioned animals was the P-N-P sequence. Inparticular, when a correct preferred trial with delay of <15 secpreceded a nonpreferred trial (P-N sequence) with delay of <5sec, the nonpreferred trial was correct >80% of the time. Surprisingly,however, when a preferred trial with delay of >5 sec followeda correct nonpreferred trial (N-P sequence), the P trial was likelyto be incorrect (80-85% errors) as shown in Figure 6, middle right.The latter anomaly is not easily explained (see Discussion); howeverit does illustrate a profound change in sequential trial influencein pretrained HIPP-lesioned animals after thesurgery.

Lack of previous training on DMS/DNMS and HIPP lesions

Previous training also proved to be a powerful factor that interacted with the effect of HIPP lesions. Two animals trainedafter the lesion on the DNMS task had reliable HIPP lesions. Thesetwo naive HIPP-lesioned animals exhibited an overall performancelevel of 79% (Fig. 6, bottom), significantly above [F_(10,1263)= 2.63; p < 0.001] pretrained HIPP lesioned animals but significantlylower [F_(10,1263) = 2.80; p < 0.001] than the prelesion performanceof that same group (Fig. 6, top). However, like pretrained HIPPanimals, naive HIPP animals exhibited performance that was differentiallyinfluenced [F_(10,1263) = 2.51; p < 0.01] by preferred versus nonpreferredtrials (Fig. 6, bottom left). Performance in naive HIPP-lesionedanimals, however, was superior on nonpreferred trials to thatof pretrained HIPP-lesioned animals, especially at longer (>6.0sec) delay intervals (Fig. 6, bottom left). The parallel setsof flat curves in Figure 6, bottom right, indicate another differencewith respect to training status; the proactive effect of timebetween trials did not interact statistically [F_(10,1263) = 4.39;p < 0.001] with P and N trials in naive HIPP-lesioned animals(Fig. 6, bottom).

Effects of hippocampal removal with collateral retrohippocampal damage

Animals with HCX lesions sustained destruction of tissue in surrounding retrohippocampal areas (subiculum, pre- and parasubiculum,and entorhinal cortex) in addition to complete removal of thehippocampus (see Fig. 2, HCX). Three groups of animals sustainingsuch damage were examined: (1) pretrained HCX-lesioned animals(n = 4), (2) partially trained (see Materials and Methods) HCX-lesionedanimals (n = 4), and (3) naive HCX-lesioned animals (n = 4) thatreceived no training before the lesion. Animals in all HCX lesiongroups were trained on the DMS or DNMS version of the task. HCX-lesionedanimals were given the same number of training days that pretrainedHIPP- and HCX-lesioned animals received before surgery. Afterthe lesion, naive and partially trained HCX-lesioned animals weretrained to 90% correct performance on 0 sec delay trials. Therewere no differences in performance between any of the HCX-lesionedanimals [F_(8,451) = 0.47, NS] before initiation of testing with0-30 secdelays.

Pretrained HCX-lesioned animals
The number of days to achieve criterion performance of the HCX-lesioned animals before surgery was not significantly different[F_(10,1263) = 0.49, NS] from the prelesion performance of HIPPanimals with respect to either task (DMS vs DNMS). Although overallpostlesion performance in pretrained HCX-lesioned animals washighly impaired (69% correct) relative to prelesion performancelevels [F_(10,1263) = 4.32; p < 0.001; Fig. 7 top, dotted line],overall performance was not significantly different compared withthe postlesion performance of pretrained HIPP-lesioned animals[71%; F_(10,1263) = 0.83, NS]. However, three major differencesbetween pretrained HIPP- and HCX-lesioned animals were detected;(1) performance was more dichotomized with respect to preferred(mean = 81% correct) versus nonpreferred (mean = 48%) trials [F_(10,1263)= 8.17; p < 0.001; Fig. 7, top left], (2) performance on P-N trialsequences was not differential with respect to delay (Fig. 7,top left), and (3) proactive influences were strongly dictatedby temporal proximity to the previous trial [F_(10,1263) = 5.21;p < 0.001]. The HCX lesion uncovered a strong "recency effect"that rapidly dissipated after 15 sec in lieu of the overridingP/N trial bias (HIPP-lesioned animals; Fig. 7, top right).

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Figure 7. Comparison of preferred and nonpreferred trial influence in pretrained HCX-lesioned animals. Performance sorted by preferred (Pref) versus nonpreferred (Non) trial type for pairs of trials (preceding and current) as shown in Figure 6. Data are shown for three groups: animals that were fully pretrained before the lesion (Top; Trained, HCX; n = 4 animals, 10 sessions), animals that were partially trained before the lesion (Middle; Partial, HCX; n = 4 animals, 11 sessions), and animals that were not trained before the lesion (Bottom; Naive, HCX; n = 4 animals, 16 sessions). Mean (± SEM) DMS and DNMS performance sorted according to current trial delay is shown on the left; performance sorted according to time since the preceding trial is shown on the right. Dashed lines (left) indicate mean performance across all trials for a given training group. Symbols are described in Figure 6.

Partially trained HCX-lesioned animals
Figure 7, middle left and middle right, shows performance by HCX-lesioned animals trained to lever press before the lesion(partially trained). As with pretrained HCX-lesioned animals,performance on preferred trials was significantly [F_(10,1263)= 4.91; p < 0.001] elevated relative to that on nonpreferred trialsacross all delays; however, the degree of separation between preferredversus nonpreferred trials was significantly reduced in comparison[F_(10,1263) = 5.73; p < 0.001]. Partially trained HCX-lesionedanimals showed significantly lower overall performance [F_(10,1263)= 3.84; p < 0.001] than did naive HCX-lesioned animals, especiallyon nonpreferred trials at all delays (Fig. 7, middle, bottom).Most importantly, the same recency effect [F_(4,1263) = 4.19; p< 0.001] seen in pretrained HCX-lesioned animals was also evidentin partially trained HCX-lesioned animals (Fig. 7, middle right).

Naive HCX-lesioned animals
Naive HCX-lesioned animals (n = 4) showed the least impairment of DMS and DNMS performance of all HCX-lesioned animals (Fig.7, bottom). This group exhibited superior overall performance,compared with both pretrained (69%) and partially trained HCX-lesionedanimals [73%; F_(10,1263) > 2.63; p < 0.001]. Naive HCX-lesionedanimals took fewer days to reach the criterion performance of85% correct for trials with $<=$ 5 sec delays (mean = 16.4 d) thandid pretrained (mean = 21.6 d) or partially trained (mean = 22.3d) HCX-lesioned animals. However, consistent with all lesion effects,trials with delays of >6 sec showed performance segregated intopreferred versus nonpreferred categories [F_(10,1263) = 3.19; p< 0.001], but to a much lesser degree than in other HCX-lesionedanimals (Fig. 7, bottom left). Naive HCX-lesioned animals alsoshowed the same recency effect related to temporal proximity ofthe previous trial [F_(10,1263) = 1.91; p < 0.05] that pretrainedHCX animals showed, although, again, this was significantlyreduced.

Lesion versus training effects in DMS and DNMS performance

It is clear from the above results that two major variables, (1) type of lesion and (2) presence of previous training, affectedthe performance of all lesioned animals. Figure 8 summarizes theeffects of these two variables for each of the four major lesiongroups plotted as a function of delay interval. The curves withsolid versus unfilled symbols (Fig. 8) reflect differences inpretrained versus naive lesioned animals in each lesion condition(HIPP vs HCX). The bold (dashed vs solid) lines depict differencesin performance between HCX- and HIPP-lesioned animals.

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Figure 8. DMS and DNMS performance curves for all combinations of task training and type of lesion. Combined mean (± SEM) DMS and DNMS performance across all trials. Performance is shown for animals trained before HIPP (Pretrained, HIPP) or HCX (Pretrained, HCX) lesion as well as for animals that were not trained (i.e., Naive) before receiving HIPP or HCX lesion. Performance in the combined intact group before lesion (Pretrained, Intact) is shown for comparison. Filled versus unfilled symbols indicate the trained versus untrained groups, respectively. Solid versus dashed lines indicate HIPP versus HCX lesions, respectively.

With respect to performance, there was a marked delay-dependent two-way interaction [F_(9,1261) = 13.67; p < 0.001] betweenboth the type of lesion and whether the animals were pretrainedon the task. At delays of >10 sec, performance of both naive lesiongroups (HIPP and HCX) was superior to that of pretrained lesionedanimals with the same type of lesion. Also, HCX-lesioned animalsirrespective of pretraining showed significantly worse performanceat delays of $<=$ 10 sec than did HIPP-lesioned animals [F_(1,1261)= 6.43; p < 0.01]. Thus pretraining on the task had no influenceon performance at short ( $<=$ 10 sec) delay intervals, but HCX-lesionedanimals showed significantly more impairment than did HIPP-lesionedanimals at thesedelays.

At longer delays (>15 sec), pretraining interacted significantly with the severity of the lesion deficit [F_(9,1261) = 4.22;p < 0.001]. The most striking example was the performance of naiveHCX-lesioned animals (Fig. 8, dashed line with unfilled invertedtriangles) that was impaired on trials with short delays (0-10sec) but not significantly different from the performance of intactanimals on trials at the longest delays (26-30 sec). In contrast,the performance of pretrained HIPP-lesioned animals (Fig. 8, solidline with filled squares) exhibited no effect on performance at0 sec delays but a classic delay-dependent decrease (relativeto prelesion levels) for all other delays. Finally, pretrainedHCX-lesioned animals exhibited even greater performance deficitsat intermediate delays (6-17 sec) than did both naive HCX-lesionedand pretrained HIPP-lesioned animals (Fig. 8). This dissociationbetween extent of lesion and previous training as a function ofdelay interval provides very strong evidence of differential processingof information by hippocampal versus retrohippocampal structuresas a function of previous experience with the task (Hampson etal., 1995).

Changes in proactive influences in lesioned animals

Several factors led to differences in the performance of lesioned versus intact animals. A concise description of these differenceswith respect to one of the most influential variables, previoustrial sequence, is presented in this section. In most cases thesedifferences were severely exaggerated in animals trained beforethe lesion (Figs. 6-8). To assess changes in such proactive influences,a measure of the degree of influence of previous trial sequenceson a given trial was derived by sorting trials by all possiblecombinations of three trials (the relevant or current trial beingthe last trial in the three trial sequence). Each third trialin the sequence was analyzed on the basis of whether there wasa significant deviation from mean overall performance as a functionof the preceding of two trials. The proportion of third trialsin which no significant change from overall performance occurredwas determined and considered to be controlled primarily by "within"-trialinfluences, whereas those in which the previous sequence affectedperformance were considered to be controlled by "between"-trialinfluences. Both between- and within-trial influences were furtheridentified in terms of the length of delay. Only trials in whichthe two above influences could be clearly isolated (i.e., >15%difference in performance of the third trial as a function ofthe previous sequence) were included in the analysis (~50% oftotal trials), because the other trial sequences consisted ofruns of like trials and single alternating sequences, both ofwhich contained strong preference effects (Figs. 4-7). The sametypes of trial sequences were compared in all four groups of animals,generating between- and within-trial performance curves for (1)intact animals, (2) pretrained HIPP-lesioned animals, (3) pretrainedHCX-lesioned animals, and (4) naive HIPP- and HCX-lesioned animals(combined).

Figure 9, A-C, shows performance curves for within- and between-trial influences as a function of the delay for all four groups.For intact animals, on trials in which there was minimal previoustrial influence, increasing the trial delay produced only a slightdecrease in mean performance (Fig. 9A, Control Within). The samemeasure plotted after both types of lesions revealed a strikingdeficit in performance [F_(10,388) $>=$ 3.58; p < 0.001] on trialswith >5 sec delays (Fig. 9B,C, HIPP, HCX). The dotted line inFigure 9A indicates that both the within- and between-trial influenceson performance in the combined naive HIPP- and HCX-lesioned animalswere markedly reduced [F_(10,388) = 2.55; p < 0.01] relative topretrained lesioned animals. The difference between the intactgroup performance (Fig. 9B,C, replotted as dotted line) and thelesion group curves across increasing delays is a measure of theinability to sustain use of within-trial information to solvethe task.

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Figure 9. Separation of within- versus between-trial influences for intact and pretrained HIPP- and HCX-lesioned animals. Trials were sorted as a function of three trial sequences and categorized with respect to significant influences of the previous two trials on the performance of the third trial in the sequence. The trials were then averaged and plotted as a function of delay interval of that third trial. This provided an estimate of the degree to which animals could perform the trial based only on DMS and DNMS contingencies operating within the trial independent of between-trial (i.e., proactive) influences. Between- and within-trial performance curves were calculated only from sequences in which the previous trial was of a different type (~50% of total trials). A, Intact animals. Within-trial performance curve (filled circles) for intact (Control Within) animals is plotted as mean percent correct (± SEM) across all delays for trials in which there was no between-trial influence. Between-trial performance curve for intact animals (unfilled circles) shows a sharp decline for >10 sec delay trials, indicating increased proactive influence as the delay on the current trial is increased. The dotted curve indicates the performance of the combined naive (HIPP and HCX) lesioned animals. Significance levels for all points [pairwise comparisons, within vs between, F_(1,388) > 10.9] are indicated at p < 0.001 (asterisks). B, Pretrained HIPP-lesioned animals. Within- and between-trial performance curves for pretrained HIPP-lesioned animals are shown. The dotted curve represents the within-trial curve for intact animals (Control) in A replotted for comparison. C, Pretrained HCX-lesioned animals. Within- and between-trial performance curves for pretrained HCX-lesioned animals are shown. The dotted curve is a replot of the intact animal (Control) within-trial curve as in B. D, Small graph (Recency) showing the effects of recency removed from all other between-trial sequential influences for each of the four groups of animals (Control, circles; HIPP, squares; HCX, triangles; and combined Naive, dashed line). The only trial sequences plotted were those that produced recency effects in pretrained (triangles) or naive (dashed line) HCX-lesioned animals.

The complementary plot for trials in which the previous sequence significantly affected DMS and DNMS performance is shownas unfilled symbols in Figure 9, A-C. Figure 9A shows that inintact animals, between-trial influences are minimal on trialsof <10 sec delay and increase linearly to maximum on trials withthe longest delays (30 sec) where within- and between-trial performancecurves are maximally separated. This indicates that a major detrimentalinfluence on performance in intact animals is previous trial sequencewhen delays exceed 10-15 sec. This appeared to be the case inpretrained HIPP-lesioned animals as well, even though overallperformance was significantly decreased [F_(10,388) = 2.39; p <0.01] at all delays (Fig. 9B). Performance was significantly decreasedat all delays >5 sec relative to overall mean levels [F_(10,388)= 5.31; p < 0.001] and with respect to the performance of intactanimals [F_(10,388) = 6.47; p < 0.001] under the same sequentialinfluences. It is clear that proactive influences increased asdelay increased for intact and pretrained HIPP-lesioned animals(Fig. 9A,B) but leveled off quickly at delays of >15 sec for pretrainedHCX-lesioned animals (Fig. 9C). Thus, pretrained HCX-lesionedanimals showed a more severe impairment from previous trial influences(with little delay dependence) than did pretrained HIPP-lesionedanimals [F_(10,388) = 4.22; p < 0.001]. The inset in Figure 9Cshows that one reason for the severe deficit in pretrained HCX-lesionedanimals (triangles) was the previously described strong recencyeffects (Fig. 7) resulting from this lesion, illustrated hereas a significant difference [F_(10,388) = 5.16; p < 0.001] in thepercent change in performance on trials in which recency effectswere most likely to occur (i.e., preceding trials that were closerintime).

  DISCUSSION

The findings described here indicate that the hippocampus plays a key role in the performance of tasks in which retentionof item-specific information across variable delay intervals isrequired. In each instance in which animals were tested beforeand after the lesion, performance in both tasks (i.e., DMS andDNMS) was equally impaired relative to prelesion levels (Fig.3). A major finding in the present study was that animals withcomplete and selective removal of the hippocampus (HIPP lesion)were severely compromised in terms of retention of item-specificinformation within a trial and also highly susceptible to trialbiases (preferences) as well as sequential dependencies betweentrials (Figs. 6, 9). Hippocampal removal that also caused collateraldamage to adjacent structures (HCX-lesioned animals) producedadded deficits in the form of strong recency effects (Figs. 7,9). Performance in all pretrained (HIPP or HCX) lesioned animalsnever recovered to prelesion levels over ~40 successive days ofpostoperative training (Figs. 4, 5). Quite unexpected was thefinding that animals trained after either type of lesion (naive-lesionedanimals) showed less impairment on the tasks than did pretrainedlesioned animals, suggesting that pretraining with the hippocampusintact rendered remaining anatomic structures (retrohippocampal)less capable of adapting to perform the task (seebelow).

The most distinct consequence of isolated and complete hippocampal removal was the fixation of a permanent preference fora particular trial type (Figs. 4, 6). This tendency interactedwith other proactive factors that affected performance at alldelays (Figs. 4, 6, 9). Before the lesion, such preferences werenot consistent over sessions and did not influence performance(Fig. 6, top). After surgery in pretrained HIPP- and HCX-lesionedanimals, this bias maximized performance (>90%) on preferred trialsand reduced responding to chance levels on all but the shortest-delaynonpreferred trials (Figs. 6, 7). Numerous other studies of hippocampallesions on spatial and nonspatial tasks in rats have identifiedfactors affected by the lesion, including stimulus complexity(Rawlins et al., 1993; Yee and Rawlins, 1994; Cassaday and Rawlins,1995), context (Davidson and Jarrard, 1993; Honey and Good, 1993;Deacon and Rawlins, 1995), response strategies (Rawlins et al.,1988; Gutnikov et al., 1994; Gutnikov and Rawlins, 1996), andamount of information per trial (Steele and Rawlins, 1993), aswell as the effects of reinforcement per se (Jarrard et al., 1986;Yee et al., 1997). However, few have mentioned the type of trial-basedpreference identified in the pretrained HIPP- and HCX-lesionedrats described here. Dunnett (1989) described a deficit in fornix-lesionedanimals that exacerbated the same/different differentiation seenin normal animals (Fig. 6, top), but this was not analyzed interms of preferred versus nonpreferred trialdifferences.

One possible explanation is that animals with hippocampal ibotenate lesions respond faster than intact animals (Jarrard, 1993)such that on operant-type tasks like the one used here, failureto inhibit responding at the appropriate time may influence performance.Although such disinhibition could contribute to the deficit, acomplete analysis must take into account the fact that performancewas decreased in both the DMS and DNMS types of tasks, which eliminatesexplanations in terms of a simple response bias for one or theother levers. At long-delay intervals, lesioned animals essentiallyperformed only one trial type; therefore, it seems that they wereimpaired when required to perform in the opposite manner (i.e.,nonpreferred trials) with respect to sample and to match or nonmatchtask requirements using the samestimuli.

The above results are somewhat inconsistent with reports of the lack of severity of either electrolytic or excitotoxic lesionsof the hippocampus on DMS and/or DNMS performance in rodents (Lyfordet al., 1993; Rawlins et al., 1993; Steele and Rawlins, 1993;Jarrard and Davidson, 1994; Yee and Rawlins, 1994). Those studiesindicated that unless areas other than the hippocampus were affectedthe performance deficit was relatively small. It is not knownwhether the marked deficit demonstrated in HIPP-lesioned animalsin this version of the DNMS and DMS task was caused by the differentialspatial requirements of task-relevant responses (Jarrard, 1995)or other factors such as exaggerated proactive interference fromthe previous trial (Deacon and Rawlins, 1995). It has been suggestedthat motor mediation may account for successful DMS and DNMS performancein rats tested in other types of rodent DMS and DNMS tasks (Gutnikovet al., 1994; Chudasama and Muir, 1997). Although this possibilitywas to a large extent eliminated by the apparatus design and versionof the current tasks (Fig. 1), such a behaviorally dependent explanationcould still not account for the sequence- and time-dependent natureof the effects of prior trials in lesioned animals (Fig. 9) orfor the marked differentiation of performance on preferred versusnonpreferred trials (Figs. 4-7) in the presentstudy.

A second important finding derived from post hoc analyses of the data was that the pretrained (HIPP and HCX) lesioned animalswere not performing the delay tasks in the same manner as beforethe lesion, or with the same success as animals trained afterthe lesion (Figs. 6-8). Pretrained HIPP-lesioned animals seemedto revert to alternation strategies in which runs of the sametype of trials could be performed at maximum levels (93% correct)if the trials were of the preferred (P) type (Fig. 6, middle).Nonpreferred (N) trials were performed at random unless they closelyfollowed a short successful preferred trial. It is possible thatall animals have an innate response bias in the task that is normallymasked and of little influence on performance because of effectivememory for the sample information across most delays. The inabilityto suppress response bias in lesioned animals may therefore bean indirect outcome of the memory impairment in the task, eventhough it seems to reflect a maximization strategy. PretrainedHCX-lesioned animals showed a pronounced recency effect in additionto these same P and N biases (Fig. 7, top). Animals trained afterthe lesion exhibited delay-dependent performance levels significantlyabove those of pretrained HIPP- and HCX-lesioned animals, suggestingthat they were less susceptible to P and N trialdifferences.

Another difference between the two types of lesions in pretrained animals seemed to be the ability to perform the tasks atlong-delay intervals. When delay curves exhibit parallel shiftsat all delays, Ringo (1991) has maintained that memory disruptionis not delay dependent. Demonstration of selective hippocampalinvolvement in the task requires under this assumption that performanceat the very shortest delay intervals (1.0 sec) be maintained,whereas performance at longer delays is systematically more impaired(Figs. 3, 8, 9). The corresponding difference in slope of thepre- versus post-HIPP and -HCX lesion within-trial curves (Fig.9A) indicates that the deficit can in part be attributed to aninability to perform at delays of >6 sec when other between-trialfactors are accounted for. A similar delay specificity was shownto be responsible for performance deficits in studies with nonhumanprimates (Alvarez-Royo et al., 1992).

The results of the present study also suggest that the long-held notion of well learned tasks being less affected by hippocampallesions (cf. Squire, 1992) might have to be modified for tasksthat use highly redundant trial-specific information. In the reportedstudies with hippocampal ibotenate lesions, very few animals aretested on the same task before and after the lesion to comparedifferences in performance as a function of when the lesion wasadministered (Irle and Markowitsch, 1990; Ridley et al., 1996).The present results indicate that certain retrohippocampal areasmay have been permanently "altered" during prelesion trainingon the task, such that after hippocampal removal, the remainingpostlesion plasticity was insufficient to allow these areas tobe modified to perform the task to the same level as animals thatwere not pretrained (Figs. 8, 9). Thus, performance that requiredthe use of within-trial information was severely disrupted inpretrained lesioned animals but spared to a large extent in naivelesioned animals trained after surgery (Fig. 9A, dotted curve).It is also clear from Figures 4 and 5 that postlesion performancedid not improve significantly in pretrained HIPP-lesioned animalseven though extensive retraining sessions wereprovided.

In the emerging conceptualization of the role of medial temporal lobe structures in memory (Eichenbaum, 1997), the hippocampushas been relegated the specific function of supporting semantic(Squire and Zola, 1997; Reed and Squire, 1998) versus episodic(Tulving and Markowitsch, 1997; Vargha-Khadem et al., 1997) memoryprocesses. Substantial evidence now shows the importance of othertemporal lobe structures, in particular perirhinal and postrhinalcortex as well as retrohippocampal regions (subiculum, parasubiculum,and entorhinal cortex), in traditional "hippocampal-type" memorydeficits (Suzuki et al., 1993; Zola-Morgan et al., 1993; Squireand Zola, 1997). This has been supported by recent studies showingindependent anatomic connectivity between the above retrohippocampaland cortical areas and their associated input structures (Burwellet al., 1995; Tamamaki and Nojyo, 1995; McIntyre et al., 1996;Naber et al., 1997; Burwell and Amaral, 1998; Naber and Witter,1998).

In the present study, differentiation between the involvement of the hippocampus in DMS and DNMS performance and retrohippocampalareas in rodents confirms the distinction in roles played by thesedifferent areas. The emergence of a strong recency effect notpresent in HIPP-lesioned animals (Figs. 8, 9B) was a shared characteristicof all HCX-lesioned animals, irrespective of when the animalswere trained relative to surgery. It is interesting that in thepresent study, variable combinations of collateral damage to retrohippocampalstructures (subiculum, pre- and/or parasubiculum, and entorhinalcortex) across different animals led to similar deficits in allHCX-lesioned animals (Fig. 7). This raises the interesting possibilitythat damage to any of these retrohippocampal areas interrupteda "functional circuit" (Eichenbaum et al., 1994; Eichenbaum, 1997;Murray and Mishkin, 1998) through which information could be processedeither in conjunction with (pretrained HCX-lesioned animals) orparallel to (naive HCX-lesioned animals) the hippocampus. Lesionsof the entorhinal and perirhinal cortex that spare hippocampusin the rat also produce major deficits in delay-type tasks (Rothblatet al., 1993; Holscher and Schmidt, 1994; Glasier et al., 1995;Wiig and Burwell, 1998). Therefore it is possible that if theanimal is pretrained with all structures (i.e., circuits) intact,areas that remain after the removal of the hippocampus lose theability to adjust the processing of task-relevant informationto compensate for hippocampalremoval.

Vargha-Khadem et al. (1997) showed the surprising dissociation of amnesia from other types of intellectual abilities in childrensuffering damage to the hippocampus as infants, suggesting thatthe semantic memory system may be able to overcome hippocampalinsult but that episodic memory remains impaired. The findinghas provoked serious re-evaluation of whether hippocampal damageaffects only episodic or also semantic memory in humans (Squireand Zola, 1997; Tulving and Markowitsch, 1997). Eichenbaum (1997)suggests that similar data are available from animal studies inthat hippocampal-lesioned rats: (1) "lack flexibility in adaptingappropriate strategies based on nonexplicitly paired stimuluselements and (2) are highly susceptible to interference from similartypes of stimulus elements." The above findings in this studyin which hippocampal removal impaired permanently the use of within-trialinformation in pretrained HIPP- and HCX-lesioned animals providesevidence of a distinction in the two processes. These deficitswere either not present or severely reduced in naive lesionedanimals, demonstrating the flexibility of intact retrohippocampalareas to overcome the loss of hippocampal structures as long ascritical processes within those regions have not been altered,as in "hippocampal-dependent learning" before thelesion.

A recent report by Murray and Mishkin (1998) showed that selective ibotenate removal of hippocampus and amygdala did not producedeficits in DNMS tasks in nonhuman primates. Using tasks in whichsuch deficits had been demonstrated in the past, the authors suggestthat other lesion methods used in monkeys interrupted fibers projectingfrom subiculum to and from perirhinal and entorhinal cortex andother structures (Stefanacci et al., 1996). Although this contradictssome earlier reports of the necessity of hippocampal involvementin DNMS performance (Zola-Morgan et al., 1982, 1989a; Murray andMishkin, 1984; Zola-Morgan and Squire, 1990; Alvarez-Royo et al.,1995), it is consistent with a series of recent studies showingmore pronounced effects of perirhinal, postrhinal, and parahippocampallesions on delay tasks in nonhuman primates (Zola-Morgan et al.,1989b,c; Gaffan and Murray, 1992; Meunier et al., 1993; Suzukiet al., 1993; Leonard et al., 1995).

There are some caveats to the Murray and Mishkin (1998) study however. The first has to do with the lack of an effect of delayon memory in the task that was not disrupted by their lesions.Control animals in their study did not exhibit memory deficitsat any delay (except when list length and delay were combined),rendering the absence of a lesion effect somewhat questionable.Secondly, there were acknowledged differences in the type of pretrainingreceived by the animals that were compared in that study (Zola-Morganet al., 1989b,c; Meunier et al., 1993). In view of the findingsreported here with rodents, it is possible that the lack of adeficit may have interacted with the extent of training beforethe lesion. Third, with respect to the stated necessity to interruptthe projection from retrohippocampal areas to entorhinal or postrhinalcortex (Stefanacci et al., 1996), the present findings revealmarked deficits in delay-dependent performance without such encroachment,when fibers of passage remained intact (Fig. 2) (Jarrard, 1989,1991). In addition, when such collateral damage did occur, somedeficits were qualitatively different than removal of hippocampusalone (i.e., HIPP vs HCX). Finally, in none of the animals inthe HIPP-lesioned group was damage to the amygdala or surroundingstructures noted. Thus it is unlikely that the deficit attributedto HIPP-lesioned animals in the current study was the result ofthe interruption of the pathway claimed by Murray and Mishkin(1998) to be relevant for short-term memory inmonkeys.

One reason isolated hippocampal removal was so devastating in this study may have been the heavy "spatial loading" inherentin the operant task used. It is evident from the rodent literaturethat the hallmark indicator of hippocampal damage is performancedeficits in tasks requiring use of spatial information (Morriset al., 1982; Morris, 1991). Because the performance of HIPP-and HCX-lesioned animal at delays of <6.0 sec was unaffected (Figs.6-9), it could be hypothesized that (1) spatial information is inherentlymore difficult to encode than nonspatial information (Hampsonand Deadwyler, 1996a; Deadwyler and Hampson, 1997), (2) spatialinformation is more susceptible to the types of proactive interferenceinherent on each trial as the delay increases (Fig. 9B), or (3)after spatial information is encoded, it "decays" at a higherrate across the delay than nonspatial information (Fig. 9A). Whateverthe reason, it is clear that animals with complete and isolatedhippocampal removal did not perform the task in the same manneras before the lesion. The deficit was a direct function of thesame variable that makes the task difficult to perform in intactanimals, i.e., the increasing temporal interval between the encodingof the sample information and the subsequent retrieval of thatinformation to make a specific discriminative response. In thatcontext, the results support and confirm extensive electrophysiologicalstudies showing a close correspondence between the "strength"or "distinctiveness" of the neural code for the sample stimulusindicated by the intensity of cell firing within ensembles ofhippocampal neurons and the ability to perform the task at extendeddelay intervals (Deadwyler et al., 1996; Deadwyler and Hampson,1997; Hampson et al., 1998b). Therefore, unless the hippocampusis present to provide or regulate such encoding, the accuracyof performance in delay tasks will depend on when the hippocampusis removed during training as well as on the extent to which remainingretrohippocampal areas can subsume that encoding function (Fig.8).

  FOOTNOTES

Received Sept. 25, 1998; revised Nov. 30, 1998; accepted Dec. 2, 1998.

This research was supported by National Institute on Drug Abuse Grants DA03502 and DA00119 to S.A.D. and DA08549 to R.E.H.We thank Doug Byrd, Joanne Konstantopoulos, and Terry Bunn fortechnicalassistance.
Correspondence should be addressed to Dr. Robert Hampson, Department of Physiology and Pharmacology, Wake Forest UniversitySchool of Medicine, Medical Center Boulevard, Winston-Salem, NC27157-1083.

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Abstract
Introduction
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