Lesions of the Amygdala Central Nucleus Alter Performance on a Selective Attention Task

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The Journal of Neuroscience, September 1, 2000, 20(17):6701-6706

Lesions of the Amygdala Central Nucleus Alter Performance on a Selective Attention Task
Peter C. Holland¹, Jung-Soo Han², and Michela Gallagher²
¹ Department of Psychology, Duke University, Durham, North Carolina, 27708, and ² Department of Psychology, Johns Hopkins University, Baltimore, Maryland 21218

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previous studies showed a role for the amygdala central nucleus (CN) in attentional processing during the acquisition of Pavlovianassociations. Both the acquisition of conditioned orienting responsesand the surprise-induced enhancement in the ability of conditionedstimuli to enter into new associations depend on the integrityof CN. In this experiment, the role of CN in the performance ofa well-learned selective attention task was examined. Rats withibotenic acid lesions of CN and control rats first learned a discrete-trial,multiple-choice reaction time task. On each trial, after a constant-durationready signal, the rats were required to poke their noses intoone of three ports, guided by the brief illumination of one ofthose ports. Rats with CN lesions were slower to acquire the taskthan control rats but showed equivalent asymptotic sustained performance.Subsequent attentional challenges, which included reducing theduration of the port illumination and varying the duration ofthe ready signal, had greater impact on the performance of lesionedthan control rats. These data resemble those reported from similartasks after damage to the basal forebrain (BF) system. Togetherwith earlier findings, these data support a role for CN in modulatingvisuospatial attention in action as well as in the acquisitionof associations, perhaps by way of its projections to BF cholinergicsystems.

Key words: amygdala; central nucleus; selective attention; basal forebrain cholinergic system; reaction time; rats

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recent data implicate the amygdala central nucleus (CN) in the modulation of attention during the acquisition of Pavlovianconditioning (for review, see Holland and Gallagher, 1999). First,the acquisition of conditioned orienting behavior (OR) to conditionedstimuli (CSs) paired with food depends on the integrity of amygdalonigrostriatalcircuitry. Rats with bilateral lesions of CN (Gallagher et al.,1990) or with asymmetric lesions that disconnect CN from dorsolateralstriatum (Han et al., 1997) fail to acquire these conditionedORs. Second, neural circuitry that includes CN connections withbasal forebrain (BF) structures is important for surprise-inducedenhancements in the ability of CSs to enter into new associations,an attentional property known as "associability" (Pearce and Hall,1980). These enhancements are abolished in rats by bilateral lesionsof CN (Holland and Gallagher, 1993a,b), bilateral lesions of thelarge cholinergic neurons of the substantia innominata/nucleusbasalis magnocellularis (SI/nBM; Chiba et al., 1995), and asymmetriclesions that disconnect CN from those SI/nBM neurons (Han et al.,1999).

Other research demonstrates a role for the BF cholinergic system in the regulation of attentional processes engaged in sustainedor selective attention tasks (Muir et al., 1992; Pang et al.,1993; Voytko et al., 1994; McGaughy et al., 1996; Chiba et al.,1999). In these tasks, animals perform previously learned responsesunder conditions thought to place demands on attentional processingof the stimuli that guide responding. For example, in the multiple-choicereaction time (MCRT) task (Carli et al., 1983), rats must nosepoke into one of several ports when it is briefly illuminated.Performance in this task requires selection of one of many elementsof the stimulus (port) array. Manipulations designed to increaseattentional demands typically depress performance. Notably, ratswith lesions of the BF cholinergic system show impaired performanceon these tasks, especially under conditions of high attentionaldemand (Robbins et al., 1989; Muir et al., 1992, 1994, 1996; Waiteet al., 1999).

The question addressed in this study is whether performance on the MCRT task is affected by CN lesions. Although it seemsplausible that attentional processes determining performance inthis task and those affecting acquisition of new learning (knownto be affected by CN lesions) might engage similar brain circuitry,there is reason to think otherwise. For example, considerabledata (Hall and Pearce, 1979; Holland and Gallagher, 1993a) supportthe claim of a popular associative learning theory (Pearce andHall, 1980) that changes in the associability of a cue are independentof its ability to control behavioral performance. Although BFcholinergic neurons may be involved in both surprise-induced associabilityenhancements and response selection in attentional tasks suchas the MCRT, CN might be critical only for theformer.

Rats with ibotenic acid lesions of CN and control rats were first trained on a simplified version of the MCRT task. Afterperformance on the task stabilized, rats were tested under threeconditions of attentional challenge: the reduction of signal duration,the occurrence of auditory distracters, and the introduction ofvariability in the time of signalpresentation.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects, surgery, and histological analysis. The subjects were 16 male Long-Evans rats (Charles River, Raleigh, NC) thatweighed 300-325 gm at the beginning of the experiment. After thesurgical procedure but before the behavioral manipulations ofthis study, they participated in a conditioning experiment inbehavioral test chambers that differed in size, construction,and location from those used in this study. The rats lived inindividual cages with ad libitum access to water and were maintainedat 85% of their ad libitum weights by limiting their access tofood. The colony room was illuminated from 6 A.M. to 8 P.M.

Bilateral CN lesions were made in eight rats by injecting 0.2 µl of ibotenic acid (Sigma, St. Louis, MO), dissolved in PBS(10 µg/µl) at a single site in each hemisphere (anteroposterior, $-$ 2.3; mediolateral, ±4.2; and dorsoventral, $-$ 7.7). Eight controlrats received injections of the same volume of PBS vehicle alone.Injections were made with a Hamilton microsyringe equipped witha 27 gaugeneedle.

Histological procedures. After completing the behavioral experiments, the rats were killed by overdose with pentobarbital(100 mg/kg) and perfused with 4% paraformaldehyde. Brains wereremoved, post-fixed in perfusate for 2 hr, cryoprotected (20%sucrose), and sectioned (coronal plane) on a freezing microtome.Adjacent tissue sections through BF (40 µm) were taken from eachbrain. In each set of four serial sections, every first, second,and third section was processed for choline acetyltransferase(ChAT), parvalbumin immunoreactivity, and acetycholinesterase(AChE) histochemistry, respectively, and every fourth sectionwas mounted on slides for Nissl stain to verify the neurotoxiclesion ofCN.

For ChAT and parvalbumin immunoreactivity, endogenous peroxidase within the tissue was blocked by washing the sections for30 min in a solution of 3% H₂O₂ and 10% MeOH in 0.1 M PBS, followedby two 5 min washes in PBS with 0.3% Triton-X (PBST). To blockbackground (nonspecific) staining, the sections were incubatedfor 1 hr in a solution of PBST with a 10% concentration of theappropriate serum. To visualize ChAT- and parvalbumin-positivecells in BF, sections were then incubated with the appropriateantibody (ChAT, 1:200 dilution; Chemicon, Temecula, CA; parvalbumin,1:1000 dilution; Sigma) overnight at 4°C. The next day, sectionswere rinsed twice in PBST, incubated for 1 hr at room temperaturein the appropriate biotinylated secondary antibody (1:200 dilution),rinsed twice again in PBST, and then incubated for 1 hr at roomtemperature in ExtrAvidin peroxidase conjugate (1:1000 dilution;Sigma). After two PBS rinses for 5 min each, tissue was reactedusing a Vector Laboratories (Burlingame, CA) SG substrate kitfor peroxidase. Tissue sections were then mounted onto Superfrostslides, dehydrated through washes in ascending concentrationsof alcohol, and coverslipped with Permount. The AChE stainingprocedure was adapted from that of Karnovsky and Roots (1964).

Integrity of the basal forebrain cholinergic neurons was examined by comparison of ChAT-immunostained sections from controlrats with anatomically matched sections from rats in the CN lesiongroup. The extent of the neurotoxic lesion of CN was determinedin Nissl-stained sections. For each section through the rostrocaudalextent of the nucleus, the percentage of CN area in which neuronswere absent was estimated for each side separately. Note thatthis criterion provides a conservative estimate of CN damage,because surrounding the region in which no intact neurons arevisible, neurons are typically more sparse as the toxin diffusesfrom the injection site. For the lesion site in each hemisphere,the average of the extent of lesion was calculated across sections.A lesion was determined to be acceptable if lesion size encompassedat least 30% of the nucleus; rats were included in the data analysisonly if this minimum size was achievedbilaterally.

Behavioral apparatus. The test apparatus comprised four 26.5 × 26.5 × 26.5 cm, nine-hole reaction time chambers (Paul Fray,Cambridge, UK) like those used by Muir et al. (1994). The curvedstainless steel front wall of each chamber contained nine 2.5× 2.5 cm ports, all but three of which were blocked with an opaqueinsert. The three ports used were those in the center of the walland 2.5 cm to the right and left of center, 2 cm above the meshfloor. Each port included an infrared phototransistor to detectnose pokes and could be illuminated by a 3 W bulb at the backof the port. A recessed food cup, covered by a hinged acrylicplastic door, was located in the center of the rear wall of thechamber, 2 cm from the floor. A 3 W house light and a speakerwere mounted in the center of the topwall.

Behavioral procedures. The rats were first familiarized with the apparatus in four sessions. In the first two 15 min sessions,the response ports were covered, food pellets (45 mg; Noyes, Lancaster,NH) were present in the food cup, and the acrylic door to thefood cup was propped open. In the next two 30 min sessions, theresponse ports were open, and food pellets were placed in eachresponse port as well as in the foodcup.

In the baseline task used here, the beginning of a trial was signaled at random intervals by the illumination of the houselight. After a constant 5 sec ready period, one of the three targetports was illuminated for 0.5 sec. Each port was equally likelyto be illuminated on any trial. The first response to the correctport within 5 sec of port illumination was reinforced with thedelivery of a food pellet to the food cup (accompanied by a 0.3sec illumination of the food cup) and the darkening of both theport (if still illuminated) and the house light. If no correctresponse was made before the end of the 5 sec response window,the house light was darkened, and the trial ended. Responses tothe ports that were not illuminated on a trial were recorded aserrors and had no scheduled consequences. Trials were presentedin random order at predetermined intervals within the 30 min sessions;trial delivery was not affected by the rats' behavior. Each ratreceived two sessions daily, the first at ~7 A.M. and the secondat ~3 P.M.

Rats were shaped to this procedure gradually, but all rats received the same treatment (the shaping was not individualized).The duration of port illumination was reduced between sessions,from 30 sec in the first two training sessions to 0.5 sec in thelast two sessions, with the values 30, 25, 20, 15, 10, 5, 3, 2,1, and 0.5 sec. Each duration was used in two consecutive sessions.In the first two sessions there were 10 of each trial type; insessions 3-6 there were 12 of each type; in sessions 7 and 8 therewere 15 of each type; and in all subsequent training sessionsthere were 20 of each type. When the target duration was $>=$ 5 sec,responses were effective throughout the illumination of the targetstimuli.

Three additional acquisition sessions with 0.5 sec target cues provided an initial behavioral baseline for assessing the effectsof attentional challenges. In the first two attentional challengesessions, the target duration was reduced to 0.25 sec; otherwisethese sessions were identical to the training sessions. In thenext two sessions, distracter stimuli were added during the 5sec ready period. The distracters were the 1 sec presentationof an 80 dB white noise during the first, third, and fifth secondsof the 5 sec ready period and during the 0.25 sec target cue presentations.In the fifth test session the rats were returned to the original0.5 sec target condition, with a session that was identical tothe final training session. This session served as a baselineto assess the effects of the last two challenge sessions, in whichthe ready period was made variable. These two sessions were identicalto the baseline session, except that the ready periods for eachtrial type were equally likely to be 1, 5, or 9 sec in duration.A final session in this series served as a return to the constantready-time baseline and was identical to the fifth testsession.

At the end of the challenge sessions, the rats were given ad libitum access to food in their home cages for 1 week. The ratswere then placed in the experimental chambers for another test,identical to the baseline sessions of the previous phase. Thistest was intended to assess the effect of a manipulation thatwould depress the level of responding, without necessarily affectingselective attention. Previous data suggest that CN lesions donot influence the effects of satiation on several aspects of Pavlovianappetitively conditioned responding (Gallagher and Holland, 1992;Hatfield et al., 1996).

This MCRT procedure differed from most previous versions of the task. First, only three stimulus and response ports were usedin this experiment, rather than the five or more used in previousstudies. Second, in this experiment, trial delivery was completelyunder the experimenter's control, rather than the subject's. Followingthe suggestion of Bushnell (1998, p 247), trials were initiatedby a scheduled ready signal. In the usual MCRT protocol, eachsubject's behavior influences the initiation, postponement, andtermination of trials. These additional operant contingenciesincrease the complexity of the task and might generate substantialbetween-subject variability in the sequencing and spacing of trials.Furthermore, this variability could potentially be confoundedwith lesion treatment if lesions affected the subjects' abilityto master these contingencies. Minimizing the subjects' controlover event scheduling, as in this study, makes such confoundsless likely. Third, simplification of the task made it possiblefor each rat to learn without individualized shaping. In mostprevious studies with the MCRT procedure, the training parameterswere adjusted as necessary for each rat during acquisition (Robbinset al., 1989; Muir et al., 1992, 1994; Waite et al., 1999); asa result, the rats may have been exposed to very different initiallearning contingencies. Thus, our simplified MCRT procedure mayprovide an assessment of visuospatial attention less confoundedby other factors. On the other hand, it could also be argued thatour simplifications may also have substantially reduced the attentionaldemands of the task. Nonetheless, the conditions used were sufficientlysensitive to detect the effects of CN lesions when attentionaldemands wereincreased.

Behavioral data analysis. Behavioral performance was assessed with several measures. The primary measure was the latency tothe first correct response, defined as the time between the onsetof the target stimulus and the breaking of the photobeam in thatport. If no correct response occurred on a trial, a maximum latencyvalue was assigned. When the target duration was <5 sec, thatmaximum latency was 5 sec, the response window duration; whenthe target duration was >5 sec, the maximum latency was definedas equal to the target duration. Thus, this measure might be viewedas a composite measure of performance, influenced somewhat bythe accuracy of responding as well as the speed of responding.When the accuracy of responding was substantially <100%, thismeasure was supplemented by two additional latency measures: thelatency to the first correct response, limited to trials on whichcorrect responding occurred, and the latency to the first correctresponse on trials on which the first response to occur was thecorrectresponse.

Two measures of accuracy were computed: the percentage of trials on which at least one correct response occurred and the percentageof trials on which the first response was the correct response.In addition, the latency to the first error and the percentageof trials on which errors occurred were recorded. Finally, twoaspects of anticipatory responding were recorded: the number ofresponses to all ports (combined) during the ready signal butbefore the illumination of a target stimulus and the latency betweenthe onset of the ready signal and the first anticipatoryresponse.

Separate multivariate ANOVAs for each of the response measures, which used lesion condition, session, target cue (left, center,or right), and port response (left, center, or right), showedthat there were no biases to respond to any of the cues or toperform any of the port responses in either lesion condition.Consequently, each measure was collapsed across target cue andport response and analyzed with univariateANOVAs.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Histological results

Nissl staining showed acceptable bilateral lesions in six of the eight lesioned rats; behavioral data from the remaining twolesioned rats were discarded. These rats were excluded becausesufficient bilateral damage was not evident. One control rat showeduniltateral damage to CN and along the injector track; behavioraldata from this rat were also discarded. In the six rats with acceptablelesions, the CN lesions ranged in size from 30 to 70% of the nucleus,with the average lesion encompassing ~40% of the nucleus. MedialCN was damaged in all cases (Fig. 1, top right panel). Althoughthese lesions were relatively small, they were found to have significanteffects on task performance. Cholinergic neurons with ChAT immunostainingand GABAergic neurons with parvalbumin immunostaining were evidentthroughout BF in both control and lesioned brains. Importantly,no difference in the pattern and relative density of acetycholinestrasestaining was detected in comparing CN lesioned brains with controlbrains. In addition, as shown in Figure 1, cholinergic neuronslabeled with ChAT antibody and GABAergic neurons labeled withparvalbumin antibody were clearly visible in close proximity tothe area of gliosis because of removal of CN neurons.

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Figure 1. Schematic of the amygdala complex (top left) with the arrow indicating the position of the CN lesion at the level of the sections shown in the photomicrographs. The photomicrograph of a Nissl-stained section (bottom left) reveals heavy gliosis at the lesion site in the dorsal region of CN. Photomicrographs (center panels) show intact ChAT-immunopositive cholinergic neurons surrounding CN at two magnifications. Similarly, photomicrographs (right panels) show intact parvalbumin-immunopositive GABAergic neurons surrounding CN. ABL, Basolateral nucleus; st, striatum.

Behavioral results

By both speed and accuracy measures of correct responding, rats with CN lesions were somewhat slower to learn the three-choicetask than control rats (F_(1,11) $>=$ 7.22; p < 0.02). In contrast,measures of error responses and anticipatory responses showedno effects of the lesion at any point in training (F < 1). Therewere very few errors of omission; at least one response (corrector error) occurred during target presentation or the subsequentresponse window on 97.3% of the training trials in lesioned ratsand on 98.1% of the trials in controlrats.

By the last three sessions of training with 0.5 sec target cues, there were no differences between lesioned and control ratsin any response measure (F < 1; Table 1).


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Table 1. Performance in final three training sessions

Attentional challenges

Figure 2 shows the effects of the three intended attentional challenges on the latency to the first correct response, andTable 2 shows those effects on the percentage of trials on whichthe first response was correct. Figure 2a and Table 2, top portion,show performance during the final training session with 0.5 sectargets and the first session with 0.25 sec targets. Reducingthe target duration compromised performance in the lesioned butnot the control rats. ANOVAs showed a reliable lesion × durationinteraction (F_(1,11) $>=$ 7.58; p $<=$ 0.019) but no reliable main effectof either lesion (F_(1,11) $<=$ 3.06; p $>=$ 0.108) or duration (F_(1,11) $<=$ 2.37; p $>=$ 0.152). Separate contrasts of the effect of lesionwere reliable for the 0.25 sec target cues (F_(1,11) $>=$ 6.59; p $<=$ 0.026) but not for the baseline, 0.5 sec target cues (F < 1).Reduction in target duration had no reliable effects on errors,anticipatory responding, or the percentage of trials on whichat least one correct response occurred (data not shown; F < 1.2).

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Figure 2. Latencies to the first correct response in the behavioral tests. The filled bars show performance of CN-lesioned rats, and the open bars show performance of control (CTL) rats. a, Responding when the target duration was reduced to 0.25 sec and during the immediately preceding baseline session with 0.50 sec targets. b, Responding when distracter stimuli were presented during the trials and during the immediately preceding baseline session. c, Responding in a test session in which the ready signals were of variable duration (V-1, 1 sec; V-5, 5 sec; V-9, 9 sec) and responding in the immediately preceding baseline session in which the ready signal was always 5 sec (C-5).


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Table 2. Performance in attentional challenge tests: percentage of trials with first response correct

The deleterious effect of the reduction in target duration on the performance of lesioned rats was short-lived, as indicatedby the performance during the second session with 0.25 sec targetcues. Figure 2b and Table 2, middle portion, show performanceduring that session as well as during the first session with 0.25sec target cues with distracters added in the ready period. Lesionby distracter (no distracter baseline vs distracter session) ANOVAsshowed no reliable effect of lesion (F_(1,11) $<=$ 1.61; p $>=$ 0.230),distracter (F < 1), or their interaction (F < 1) on any of thelatency or accuracy measures of either correct or error respondingor on anticipatory responding (F < 1.3).

Figure 2c and Table 2, bottom portion, show performance during the first test session with variable (1, 5, or 9 sec) readysignals as well as during the immediately preceding baseline sessionwith constant 5 sec ready signals. Performance was disrupted bythe introduction of variable ready times in both lesioned andcontrol rats, but the disruption was substantially greater inlesioned rats. ANOVAs with lesion condition and test trial typeas variables showed reliable main effects of lesion (F_(1,11) $>=$ 6.69; p $<=$ 0.025) and trial type (F_(3,33) $>=$ 14.98; p $<=$ 0.001) andreliable interactions of those two variables (F_(3,33) $>=$ 4.27;p $<=$ 0.012). In control rats, performance was poorer on trialswith the short (1 sec) ready signal than on any of the other trialtypes (F_(1,11) $>=$ 5.08; p $<=$ 0.046) but did not vary across theother trial types (F < 1). In lesioned rats, performance duringthe baseline session with constant 5 sec ready times (C-5 trials)was reliably better than performance on 1 sec ready-time trialsin the variable session (F $>=$ 44.64; p $<=$ 0.001) and 9 sec variabletrials (F_(1,11) $>=$ 8.30; p $<=$ 0.015) and marginally better thanon 5 sec ready time trials in the variable session (0.05 < p <0.10). Lesioned rats showed poorer performance than control ratson both 1 sec (F_(1,11) $>=$ 17.22; p $<=$ 0.002) and 9 sec (F_(1,11) $>=$ 7.20; p $<=$ 0.022) trials in the variable session but not on 5sec trials in either the variable or baseline session (F < 1).As described later, the percentage of trials on which correctresponses occurred was reduced on 1 sec trials in both lesionedand control rats. Consequently, we were concerned that differencesin latency to the first correct response may have reflected thisfailure to respond correctly more than changes in the speed ofcorrect responses actually made. However, analyses of the latencyof correct responses confined to trials on which a correct responsedid occur and those confined to trials on which the correct responsewas the first response to occur showed patterns of significanceessentially identical to those justreported.

Unlike the duration effect shown in Figure 2a, the effects of introducing variation in the ready times were persistent. Performancein the second variable test session (data not shown) was essentiallyidentical to that in the first test. Nevertheless, performancerecovered immediately in the final test session, in which therats were returned to the 5 sec constant ready-time baseline.The mean latency to the first correct response in that sessionwas 1.65 ± 0.15 sec in the lesioned rats and 1.63 ± 0.11 sec inthe control rats, and the percentage of trials with the firstresponse a correct one was 80.1 ± 3.5% in the lesioned rats and81.2 ± 4.0% in the control rats (F <1).

The introduction of variable ready times also affected several of the other response measures. Not surprisingly, there weremore anticipatory responses per trial when the ready times wereextended to 9 sec and fewer when they were shortened to 1 sec(F_(1,11) $>=$ 7.37; p < 0.02). However, unlike with target responding,anticipatory performance of lesioned and control rats was identical(F < 1). Control rats emitted an average of 0.3 ± 0.2 responsesin the 1 sec ready periods and 2.9 ± 0.2 responses in the 9 secready periods, and lesioned rats emitted 0.2 ± 0.2 and 2.8 ± 0.4responses, respectively. This pattern of responding would be expectedfrom the evidence for timing shown in the final training sessions(Table 1). In those sessions, the first anticipatory responseon average occurred just before the scheduled time of target presentationin both lesioned and control rats. When the target was delayedin the variable test session, responding began at approximatelythe same time and continued at approximately the same rate forthe next few seconds, as is typically observed in tests of animaltiming performed using the "peak procedure" (Roberts, 1981). Inaddition, both control and lesioned rats emitted marginally moreanticipatory responses during the 5 sec ready time trials in thevariable session (2.4 ± 0.3 and 1.9 ± 0.3, respectively) thanin the constant session (1.5 ± 0.6 and 1.3 ± 0.5; F_(1,11) = 3.37;p = 0.09).

The percentage of trials with at least one correct response dropped to 61.9 ± 4.6 in control rats and 57.8 ± 9.1 in lesionedrats on 1 sec ready-time trials compared with 84.5 ± 4.6 and 78.6± 6.4 on the remaining trial types. ANOVA and subsequent contrastsshowed no effect of lesion (F_(1,11) = 1.02) but significantlylower responding on the 1 sec trials (F_(1,11) = 21.38; p < 0.001).Finally, although the percentage of trials on which an error occurreddid not differ across lesion condition or trial type (F < 1),the latency to the first error was longer on 1 sec trials thanon the remaining trial types in both lesioned rats (4.24 ± 0.14and 3.65 ± 0.09 sec, respectively) and control rats (4.33 ± 0.07and 3.69 ± 0.04 sec; F_(1,11) = 25.33; p < 0.001). Thus, reductionof the ready time slowed all responding to thetargets.

Satiation

Performance of rats in the postsatiation test showed across-the-board reductions in performance compared with performancein the presatiation baseline session (p < 0.01). None of thesereductions involved lesion effects (F < 1). For example, aftersatiation, control rats failed to respond (with either a correctresponse or an error) on 20.5 ± 2.3% of the trials, and lesionedrats failed to respond on 21.7 ± 2.8% of the trials, comparedwith <1% before satiation. Likewise, the latency to the firstcorrect response was 3.40 ± 0.24 sec in the control rats and 3.31± 0.34 sec in the lesionedrats.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Rats with CN lesions performed as well as control rats at the end of training and in a number of return-to-baseline sessionsduring the study but were especially susceptible to two attentionalchallenges. The reduction of target duration and the introductionof variability in the duration of the ready signal both reducedthe accuracy and speed of target responding. These lesion effectsare interpretable as deficits in the rats' ability to direct respondingselectively to the appropriate elements in the stimulus arrayunder conditions of increased attentional load superimposed onperformance of the well-learned MCRT task. The observations thatCN damage did not affect the depressive effects of satiation,the timing of anticipatory responses, or any aspect of performancein the baseline test sessions make it unlikely that the lesioneffects were mediated by deficits in motivational or responseproduction mechanisms. Previous studies from our laboratoriesshowed CN to be critically involved in conditioned orienting (Gallagheret al., 1990) and in the surprise-induced enhancement of CS associability(Holland and Gallagher, 1993a,b; Han et al., 1999). Taken togetherwith those earlier findings, the present results indicate thatamygdala CN may be important in a wide range of attentional processes,including both those involved in the acquisition of new learningand those involved in directingaction.

Because our MCRT training procedures were somewhat different from those typically used (see Materials and Methods), and ourlesions were made before (rather than after) training on thattask, it is difficult to compare our results directly with thoseof other lesion studies of MCRT performance. Nevertheless, ourresults can be viewed as analogous to those reported after damageto the BF system. BF lesions, made after training MCRT performance,produce an initial deficit in baseline performance followed byrecovery to control levels after retraining (Robbins et al., 1989;Muir et al., 1994, 1996; Waite et al., 1999). This pattern parallelsour observation of CN lesion deficits in the initial acquisition,but not final performance, of the MCRT task. Likewise, Muir etal. (1994, 1996), Robbins et al. (1989), and Waite et al. (1999)found that rats with damage to BF were especially sensitive todisruption by variation in the intertrial interval (correspondingto our ready-time interval). Also, as in our study, these investigatorsfound no effect of BF damage on anticipatory responding in mostcases. Similarly, Muir et al. (1994, 1996) found that rats withBF damage showed greater deficits than controls when the durationof the target cue was reduced, although Waite et al. (1999) showedno lesion effects with this manipulation. Unlike these other investigators,we did not find reliable lesion effects on performance when distracterstimuli were introduced. However, also unlike Muir et al. (1994,1996) (but like Waite et al., 1999), our distracter manipulationhad no effect on the performance of controlrats.

Deficits in MCRT performance after BF lesions have been attributed to removing cholinergic neurons that innervate cortex.The histological examination of the brains of the rats in thecurrent study showed that BF magnocellular cholinergic neuronswere spared in the presence of CN neuron loss. The BF cholinergicsystem, however, receives innervation from CN (Groves, 1988),and it seems reasonable to suggest, by analogy, that the roleof CN in MCRT performance is mediated by its connections withSI/nBM. Using a disconnection lesion procedure, Han et al. (1999)showed that CS associability enhancements depend on the integrityof the connections of CN with SI/nBM. It is possible that therole of CN in both aspects of attentional processing is mediatedby these connections. If so, then CN-SI/nBM disconnection lesionswould also be expected to disrupt MCRTperformance.

BF cholinergic systems, including SI/nBM, are frequently assigned a role in the modulation of cortical attentional function(Voytko, 1996; Everitt and Robbins, 1997; Sarter and Bruno, 1997).Indeed, performance in MCRT tasks is disrupted by lesions of anumber of cortical regions as well as by lesions of SI/nBM. Forexample, Muir et al. (1996) found lesions of the medial frontalcortex (which receives heavy projections from SI/nBM) to haveessentially the same effects on performance in the MCRT task asSI/nBM lesions. It is tempting to speculate that CN might ultimatelyinfluence cortical attention circuitry involved in sustained andselective attention tasks via its connections with SI/nBM. Thispossibility is consistent with evidence from studies of associabilityenhancements. These attentional changes are dependent not onlyon the connectivity of CN and SI/nBM (Han et al., 1999) but alsoon projections from SI/nBM to posterior parietal cortex (Bucciet al., 1998). In this context, it would be especially interestingto examine the role of medial frontal cortex in associabilitychanges and that of posterior parietal cortex in performance onselective attention tasks. Although Muir et al. (1996) found noeffects of lesions of the parietal cortex on MCRT task performance,their lesions explicitly excluded the posterior subregion identifiedin the research of Bucci et al. (1998, 1999).

Considerable research, for the most part conducted in nonhuman primates, has revealed that the regulation of attention isan integral dynamic property of neural networks in cortex (forreview of recent research, see Behrmann and Haimson, 1999). Atthe same time, increasing evidence points to a role for subcorticalsystems in the regulation of cortical processing in attention.The examination of such circuitry is likely to be important forunderstanding the normal operation of attention, as well as disordersin which attention is impaired. For example, certain evidencepoints to a loss of integrity in the basal forebrain cholinergicsystem as a basis for deficits in attention in aging and Alzheimer'sdisease (Parasuraman and Haxby, 1993). Study of the role of theamygdala central nucleus, which may regulate basal forebrain cholinergicneurons in a broad range of attentional functions, may providean additional basis for understanding these and other disorders,as well as a possible entry into the development of new therapeuticinterventions.

  FOOTNOTES

Received March 3, 2000; revised June 12, 2000; accepted June 13, 2000.

This research was supported by Grant MH-53667 and Research Scientist Award K08 MH01149 (M.G.) from the National Instituteof Mental Health. We thank Helena Winfield for technicalassistance.
Correspondence should be addressed to Peter Holland, Department of Psychology: Experimental, Duke University, Box 90086, Durham,NC 27708. E-mail: pch{at}duke.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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