 |
||||
|
||||
|
||||
|
||||
Correction for Hatfield et al.,J. Neurosci. 16 (16) 5256-5265.
The Journal of Neuroscience, August 20, 2003, 23(20):7702-7709
Previous Article | Next Article
Preserved Sensitivity to Outcome Value after Lesions of the Basolateral Amygdala
Pam Blundell,1 Geoffrey Hall,1 andSimon Killcross2 1Department of Psychology, University of York, Heslington, York YO10 5DD, United Kingdom, and 2School of Psychology, Cardiff University, Cardiff CF10 3YG, United Kingdom
Abstract
Top
Abstract
Introduction
Recent work (Blundell et al., 2001; Balleine et al., 2003
Key words: appetitive conditioning; basolateral amygdala; reward; sensory preconditioning; Pavlovian; instrumental; devaluation
Introduction
Experiments in rats have demonstrated that damage to the basolateral region of the amygdala (BLA) impairs the ability of animals to respond to post-training changes in the value of instrumental or Pavlovian rewards (Hatfield et al., 1996After a recent study (Blundell et al., 2001
Experiment 1 sought to confirm that BLA lesions do not produce deficits in appetitive Pavlovian conditioning but do impair sensitivity to post-training reward devaluation, using a lever approach autoshaping procedure. Experiment 2 examined the sensitivity of BLA-lesioned animals to reward devaluation using a sensory preconditioning procedure.
Materials and Methods
Experiment 1: BLA lesions and devaluation of autoshaped responding
Subjects
We used 16 naive, male, hooded Lister rats. Before surgery, their mean ad libitum weight was 275 gm (range, 250-285). The rats were housed in pairs in a climate-controlled vivarium (lights on 8 A.M. to 8 P.M.). Subjects were tested during the light portion of the cycle. Before the start of training, the rats were reduced to 80% of their ad libitum postsurgical recovery weights. After completion of behavioral testing, the rats were killed, and their brains removed for histological analysis.Surgery
Under anesthesia, eight rats received bilateral lesions of the BLA produced by injection of quinolinic acid (0.09 M); the remainder received a control surgical procedure. Anesthesia was induced by an intraperitoneal injection (10 ml/kg) of Avertin (made up as 1.25 ml of Avertin concentrate added to 5 ml of absolute alcohol and 62.5 ml of physiological saline; Avertin concentrate consists of 100 gm of 2-2-2-tri-bromo-ethanol dissolved in 62 ml of tertiary amyl alcohol). Additional injections (1 ml, i.p.) were given, if necessary. When a rat was fully anesthetized, it was placed in a stereotaxic frame (Stoelting Inc., Kiel, WI). The depth of anesthesia was monitored by assessing the pedal withdrawal reflex and responsivity to a mild tail pinch. An incision was made along the skull, and then skin and fascia were cleared to reveal bregma. A drill mounted on the stereotaxic frame was used to make burr holes above the injection sites. Injections (two on each side) were made with a 30 gauge needle attached by polythene tubing to a 1 µl syringe, which was controlled by an infusion pump (Harvard Apparatus, Holliston, MA). We made 0.25 µl injections at the following coordinates: lateral, ±4.6 mm; anterior-posterior, -2.3 mm, -3 mm; ventral (from dura), -7.3 mm. Each injection was made over 2.5 min, and the injection needle was left in place for an additional 2.5 min to allow the neurotoxin to diffuse. The skin was then closed with suture. Animals were then given an injection of saline if they were dehydrated. Animals were observed during recovery from anesthesia and were returned to the vivarium after starting to eat and drink. Animals were allowed to recover for at least 1 week with ad libitum access to food and water. The control surgical procedure was identical to that which was used to produce lesions, the only difference being that no quinolinic acid was injected.Histology
After the completion of behavioral testing, animals were anesthetized with a lethal overdose of sodium pentobarbitol (Sagital; 2 ml per animal, i.p.) and perfused via the ascending aorta with 0.1 M PBS, pH 7.4, followed by 4% paraformaldehyde. The brains were then removed and postfixed in 4% paraformaldehyde solution before being transferred into 20% sucrose solution. After 24 hr, the brains were frozen on a freezing microtome fast-freeze plate before coronal sections (40 µm) were cut on a freezing microtome throughout the full extent of the lesioned area. Every fourth section was taken and mounted on a gelatin-coated glass slide and then stained for analysis using cresyl violet. Slides were cover-slipped, dried, and then examined under microscope to assess the extent and nature of excitotoxin-induced neuronal damage. Areas of neuronal loss were mapped onto standardized sections of the rat brain (Swanson, 1998Apparatus
Behavioral procedures were performed in eight identical operant chambers (25 cm wide x 25 cm deep x 22 cm high; Paul Fray Ltd., Cambridge, UK), housed in light- and sound-attenuating boxes. Each chamber was fitted with two retractable levers, one located on each side of a central, recessed magazine that provided access, via a hinged Plexiglas flap, to a food magazine into which food pellets (45 mg Formula A/I; P.J. Noyes, Lancaster, NH) could be delivered. In addition, each chamber was equipped with a peristaltic pump that, when operated for 0.5 sec, delivered 0.5 ml of a 20% sucrose solution into the same magazine. Opening the magazine flap operated a micro-switch that provided a measure of approach to the site of food delivery. The floor of the chambers consisted of 18 5 mm diameter steel rods spaced 1.5 cm apart, perpendicular to the front wall of the chamber. Each chamber was illuminated by a single, 4.2 W house light located in the center of the ceiling. A BBC Master 128 microcomputer, equipped with a SPIDER extension for on-line control (Paul Fray Ltd.) controlled the equipment and recorded the data.Procedure
Training. After recovery from surgery, each animal was assigned to one of the eight operant chambers and thereafter was always trained in that chamber. At the start of each session, the house light came on and remained on throughout the session. The house light remained on at the end of each session. The reinforcers used were 45 gm Noyes food pellets and 0.5 ml of 20% w/v sucrose solution. Pilot studies indicted that in normal rats these two rewards produce very similar levels of performance of conditioned behaviors such as magazine approach and lever pressing and are well matched for their motivational value. Training consisted of two stages - magazine training and autoshaped lever pressing. There were then several test sessions, for which the rewards were first devalued by specific satiety. One session was run on each day.Magazine training. All of the rats were trained to collect food rewards during two 40 min magazine training sessions. Half the animals (equal numbers of sham- and BLA-lesioned animals) were trained to collect food pellets in the first training session, and half to collect sucrose solution. The following day, rats were trained to collect the alternative reward. The rewards were delivered on a random time 60 sec schedule.
Autoshaped lever press training. In each session, the rats were given 20 10 sec presentations of a lever on a variable time schedule of 90 sec (range, 80-100). During the last second of the lever presentation, a reinforcer, either a food pellet or sucrose solution, was delivered into the food magazine. There was no requirement for the animal to make any response to receive food reward. In each session, only one lever and one reward type was used. The rats were given training on each lever in successive sessions. The first eight sessions were of one type, and the next eight sessions were of the other type. There followed an additional 16 sessions of training with the sucrose reinforcer and 8 sessions of training with the pellet reinforcer. Over the first part of this phase of training, the two types of session were presented in alternation. It became apparent, however, that responding was developing more readily with pellets than with sucrose. In an attempt to achieve comparable levels of performance with the two reinforcers, eight extra sessions of training with sucrose were inserted into the alternating sequence toward the end of training. Whether it was the left or right lever that predicted sucrose solution was counterbalanced across animals, such that for half of the animals in each group, the left lever signaled sucrose, and for the other half, it signaled food pellets.
Satiation procedure. Before test sessions, the rats were put in a distinctive consumption cage made of white plastic, measuring 21 cm wide x 31 cm long x 19 cm high. The ceiling was a metal grid, through which a drinking spout could be inserted for presentation of sucrose solution. Cat litter was placed on the floor of the cage. When rats were to be sated on sucrose solution, 50 ml was presented in a centrifuge tube fixed with a metal drinking spout and black rubber bung. When rats were to be sated on food pellets,
100 gm of pellets was placed in a clear glass ramekin dish, and placed in the cage. The rat was given 90 min access to the reinforcer. The test session followed immediately. After each test session, the effect of the satiation procedure was assessed in a consumption test. The procedure used was identical to that used for pretest consumption but lasted only 30 min.
Test procedure. There were two types of test session: single-lever and choice tests. In the single-lever test, there were 10 presentations of one of the levers, scheduled as in training, but no reinforcers were delivered. In the choice test, rats received 10 trials in which both levers were presented simultaneously. Again, no reinforcers were delivered. Retraining on the autoshaping procedure was given between each test. This consisted of two sessions, one with each reinforcer type. All rats received, in turn, pairs of single-lever tests after satiety with first one, and then the other reinforcer. These pairs of single-lever tests were conducted first with one lever, and then the other (i.e., a total of four tests). The arrangement of tests was fully counterbalanced with respect to order of reinforcer satiety and order of lever presentation. After this, all rats received choice tests after satiety with first one, and then the other reinforcer, again counterbalanced.
Experiment 2: BLA lesions and devaluation in sensory preconditioning
Subjects
The subjects were 15 male, hooded Lister rats with a mean free-feeding weight of 523 gm (range, 425-600) at the beginning of the experiment. They had previously been used in a study of appetitive conditioning(experiment 1) (Blundell et al., 2001
Surgery and histology
Eight of the rats received surgery to lesion the BLA, whereas seven had undergone the sham-surgery procedure. The surgical procedure was the same as that in experiment 1, except for the anesthetic that was used. Anesthesia was induced with 4% halothane, delivered in O2 and N2O gas (Apparatus
Inverted 50 ml centrifuge tubes equipped with stainless steel, ball-bearing-tipped spouts were used to present measured amounts of flavor solution to the rats. The flavor stimuli that were used were 10% sucrose solution, 0.16 M saline solution, 0.01 M hydrochloric acid, and 60.0 µM quinine (A, B, X, Y, respectively; solutions were counterbalanced in pairs A and B, and X and Y). When the solutions were presented in compound, they were formulated to retain these concentrations. All of the sessions were conducted in the rats' home cages.Procedure
Preexposure. The rats were allowed 2 d to adjust to the water deprivation schedule before the start of phase one, which comprised 8 preexposure days. Rats received 30 min exposure to 10 ml of the flavor compounds AX or BY, on alternate days, at 11 A.M. Half of the rats were exposed to AX on the first day, and half to BY. Thereafter, the solution the rats received was alternated. All rats were given free access to water for 30 min each day at 5 P.M.Conditioning. At 11A.M. on day 1 of phase two, all of the rats were given 10 ml of solution X for 30 min, immediately followed by an injection of 0.15 M LiCl at 20 ml/kg (X+). The rats were given 30 min free access to water at 5 P.M. and were allowed to recover on the following day, receiving 30 min access to water at 11 A.M. and 5 P.M. At 11 A.M. on day 3 of phase two, the rats were given 10 ml of solution Y for 30 min, with no consequence (Y-). They were given free access to water at 5 P.M., and the following day was a recovery day, identical to day 2 of phase two. This 4 d cycle was then repeated, so that each rat received two X+ and two Y-training trials.
Test. Finally, all rats were tested for consumption of solutions A and B. They were given a two-bottle choice test, with 10 ml of each solution available to the animals, for 30 min, at 11 A.M. The side of presentation of each solution was counterbalanced. Consumption was measured by weighing the drinking bottles before and after the test.
Results
Experiment 1: BLA lesions and devaluation of autoshaped responding
The Pavlovian training procedure used in the present experiment was a version of autoshaping (or sign tracking) (Jenkins and Moore, 1973Histology
Three rats died during or immediately after surgery, two from the lesioned group and one sham-operated control. Histological analysis revealed that all rats in the lesioned group had bilateral lesions of the lateral and basolateral nuclei of the amygdala. Figure 1 shows the extent of the smallest and largest lesions that were included in the analysis. For some of the rats that were included in the experimental group, damage extended unilaterally into the basomedial nucleus. One rat also had damage to the central nucleus and was excluded from further analysis. There were five BLA-lesioned rats and seven sham-lesioned rats in the final analysis.
View larger version (42K):
[in this window]
[in a new window]
Figure 1. Schematic representation of excitotoxic lesions to the basolateral amygdala from experiment 1. The shaded areas represent the smallest (black) and largest (gray) extent of neuronal damage. Coronal sections are -1.8 to -3.8 mm relative to bregma (Swanson,1998
Acquisition of autoshaped responding. Figure 2 shows the group mean responses per trial for two-session blocks of initial acquisition of the autoshaped lever presses. Both BLA- and sham-lesioned animals increased lever pressing over trials, and there was no obvious difference between the groups. Both BLA- and sham-lesioned animals made fewer responses when the reinforcer was sucrose than when the reinforcer was a food pellet. The data for the acquisition phase were separately analyzed for pellet reinforcer and sucrose reinforcer, because there were different numbers of training sessions. An
level of 0.05 was adopted for this and all subsequent statistical analyses.
View larger version (12K):
[in this window]
[in a new window]
Figure 2. Group mean number of lever presses in each 10 sec trial, during acquisition of autoshaping, with sucrose solution reward (left) and food pellet reward (right).
An ANOVA was conducted on the data, summarized in the left panel of Figure 2 (acquisition with a sucrose solution US), with the between-groups variable of lesion (sham, BLA) and the within-subject variable of session (1-16). This revealed a significant effect of session (F(15,204) = 3.67) but no significant effect of lesion (F < 1) and no interaction between these variables (F < 1).
A parallel ANOVA on the data, summarized in the right panel of Figure 2 (acquisition with food pellet US), yielded equivalent results. There was a significant main effect of session (F(11,132) = 16.42) but no other significant effects (F < 1).
Satiation
During consumption tests assessing the efficacy of the satiety treatment, both BLA-lesioned and sham-lesioned rats consumed more of each type of reward when it was not the food on which they had been sated than when it was the food on which they had been sated. BLA-lesioned rats consumed (±SEM) 7.9 (1.1) gm of the reward on which they had been sated, but 13.3 (1.3) gm of the reward on which they had not been sated. Similarly, sham-lesioned rats consumed (±SEM) 3.9 (1.0) gm of the reward on which they had been sated, but 12.2 (1.1) gm of the reward on which they had not been sated. A two-way ANOVA conducted on the data from the sucrose consumption tests, with the variables of satiation (sated, nonsated) and lesion (BLA, sham), revealed a significant main effect of satiation (F(1,10) = 41.98) but no effect of lesion (F < 1) and no lesion x satiation interaction (F < 1). An identical two-way ANOVA conducted on the data from the pellet consumption test revealed a significant main effect of satiation (F(1,10) = 6.49), no main effect of lesion (F(1,10) = 1.84), and no lesion x satiation interaction (F < 1).Single-lever tests
Scores recorded on single-lever tests were pooled for each animal to produce a score for responding when the lever used on test was that associated with the reward on which the animal was sated (sated lever) and responding when the lever used on test was that associated with the reward on which the animal had not been sated (nonsated lever). Sham-lesioned rats made more responses on the nonsated lever than on the sated lever. Responses (±SEM) made in extinction were: sated, 19.1 (6.9) lever presses (lp)/session; nonsated, 37.7 (13.1) lp/session. In contrast, BLA-lesioned rats showed a very much smaller difference in responding on the two levers during extinction. Responses (±SEM) were: sated, 41.4 (10.1) lp/session; nonsated, 46.6 (13.1) lp/session. Hence, regardless of their state of specific satiety, BLA-lesioned rats responded during test at the same level as sham-lesioned rats on the nonsated lever. This was confirmed by a mixed ANOVA with factors of lesion (sham, BLA) and devaluation (sated, nonsated). Before analysis, scores were expressed as a percentage of baseline responding to reduced variability (baseline rates did not themselves differ: sham, 31.0 lp/session; BLA, 32.9 lp/session; t(10) <1.0) and were subject to square-root transformation to reduce systematic changes in variance in relation to the mean (Howell, 1997Magazine entries during the CS presentation were also recorded. The mean responses (±SEM) were: sham: sated, 12.1 (4.8) entries/session; nonsated, 12.5 (3.7) entries/session; BLA: sated, 12.1 (2.8) entries/session; nonsated, 10.8 (2.6) entries/session. Hence, there was little effect of satiety on the number of magazine entries during the CS, and there was no difference between BLA- and sham-lesioned rats. This pattern of results was confirmed by a two-way ANOVA on the magazine-entry scores, which revealed no significant effects (all F < 1).
Choice test
Once again, the responses on the sated lever and the on the non-sated lever were summed across tests. As might be expected, actual rates of responding (±SEM) during the choice tests were lower than in single-lever tests [sham: sated, 3.0 (1.0) lp/session; nonsated, 12.6 (5.8) lp/session; BLA: sated, 6.5 (2.6) lp/session; nonsated, 6.1 (3.9) lp/session]. This is likely to reflect not only the effect of repeated extinction testing, but also a degree of generalization decrement in performance because of transfer from training with single levers to a test with both levers. Sham-lesioned rats made substantially more responses on the nonsated lever than on the sated lever. In contrast, BLA-lesioned rats showed no such effect of satiety on responding and, in fact, made slightly fewer responses on the nonsated lever than on the sated lever. Data were subject to square-root transformation before analysis by mixed ANOVA with factors of lesion and devaluation. This revealed an interaction of lesion and devaluation that approached the level of rejection of the null hypothesis (F(1,10) = 4.6; p < 0.06). Simple effects analysis, again, demonstrated a significant effect of devaluation in sham-lesioned animals (F(1,10) = 9.8) but not BLA-lesioned animals(F < 1). Because the levels of responding of the BLA-lesioned animals on the two levers lay between those of the sham-lesioned animals, simple effects analysis found no significant overall effect of lesion on either the sated or the nonsated lever (minimum, F(1,10) = 2.3). This also confirmed that lesions of the BLA did not alter absolute rates of lever pressing per se, but that levels of responding in single-lever and choice tests reflected a common absence of specific satiety devaluation that varied in nature depending on the availability of alternative responses.Experiment 2: Sensory preconditioning
Experiment 1 demonstrated that both BLA- and sham-lesioned rats could acquire autoshaped CRs, confirming the finding that lesions of the BLA do not impair acquisition of appetitive Pavlovian conditioning. When a specific US was devalued by prefeeding, sham-lesioned rats selectively reduced their extinction responding on the lever that had paired with that US during training. In contrast, BLA-lesioned rats demonstrated little of no influence of this manipulation. This pattern of results parallels that reported by Malkova et al. (1997Because satiety is reinforcer specific in normal animals, it must affect the representations of the unique sensory properties of the reinforcer (Balleine, 2001
Histology
Figure 3 shows the extent of the smallest and largest lesions. Figure 4 shows photomicrographs with representative sham and BLA lesions. Histological analysis revealed that all eight BLA-lesioned rats had bilateral damage to both the basolateral and lateral nuclei of the amygdala. No rats were excluded.
View larger version (40K):
[in this window]
[in a new window]
Figure 3. Schematic representation of excitotoxic lesions to the basolateral amygdala from experiment 2. Shaded areas represent the smallest (black) and largest (gray) extent of neuronal damage. Coronal sections are -1.8 to -3.8 mm relative to bregma (Swanson, 1998
View larger version (68K):
[in this window]
[in a new window]
Figure 4. Photomicrographs from sections of two representative brains showing sham (a) and excitotoxic (b) lesions basolateral nucleus of the amgydala. Each photomicrograph shows a high magnification of the area indicated in the associated outline, representing a section at 1.88 mm posterior to bregma. Subregions of the amygdala are marked (BLA, Basolateral nucleus; LA, lateral nucleus; CeA, central nucleus. In a, the BLA is marked by arrows; in b, the lesioned area is marked by arrows.
Consumption during preexposure. All of the rats consumed similar amounts of fluid on all preexposure days. Mean consumptions (±SEM) were: BLA AX, 9.2 (0.3) ml; BLA BY, 9.2 (0.1) ml; sham AX, 9.2 (0.3) ml; sham BY, 9.4 (0.1) ml. There were no obvious differences in the consumption of BLA-lesioned and sham-lesioned animals. A two-way ANOVA was conducted on these data with the variables of lesion (BLA, sham) and flavor (AX, BY). This found no significant effects (all F < 1) or interactions, confirming that during the preexposure phase, there were no differences between volumes consumed by BLA-lesioned rats and sham-lesioned rats.
Conditioning
There were no obvious differences between sham-operated and BLA-lesioned animals in the acquisition of conditioned taste aversion to flavor X. The mean volumes consumed (±SEM) during the first conditioning session were: sham X, 9.3 (0.2) ml; sham Y, 8.7 (0.5) ml; BLA X, 9.1 (0.2) ml; BLA Y, 8.4 (0.5) ml. The mean volumes consumed (±SEM) during the second conditioning sessions were: sham X, 3.4 (1.1) ml; sham Y, 9.1 (0.2) ml; BLA X, 3.6 (1.0) ml; BLA Y, 8.8 (0.2) ml. The reduction in consumption of X in the second conditioning session in the sham-lesioned animals reflects the acquisition of the conditioned taste aversion to X, but not to Y. BLA-lesioned rats also reduced their consumption of X, appearing to be the same as the sham animals in their acquisition of the conditioned taste aversion. Both BLA- and sham-lesioned animals discriminated between flavors X and Y, drinking more of flavor Y than flavor X in the second session. A three-way mixed ANOVA was conducted on these data, with variables of lesion (BLA, sham), flavor (X, Y), and session (1, 2). This revealed no significant main effect of lesion (F < 1), a significant main effect of flavor (F(1,13) = 30.59), and a significant main effect of session (F(1,13) = 47.39). The lesion x flavor interaction was not significant (F < 1), nor was that of lesion x session (F < 1). The flavor x session interaction was significant (F(1,13) = 49.52), and the lesion x flavor x session interaction was not significant (F < 1). A simple main effects analysis of the flavor x session interaction revealed a significant effect of flavor at session 2 (F(1,13) = 44.88) but not at session 1 (F(1,13) = 4.62). There was also a significant effect of session on consumption of X (F(1,13) = 61.07) but not of Y (F(1,13) = 1.05). This reflects the acquisition of an aversion to flavor X, but not flavor Y, in session 2. The absence of significant effects involving lesion confirms that the BLA lesion did not affect conditioned taste aversion learning in these animals.Test
The mean volumes (±SEM) of A and B consumed by BLA and sham-lesioned rats during the test session were: sham A, 6.5 (1.5) ml; sham B, 8.8 (0.6) ml; BLA A, 5.4 (1.6) ml; BLA B, 9.3 (0.6) ml. Hence, both BLA- and sham-lesioned rats drank less of solution A than of solution B; if anything, the aversion to A was slightly more marked in the BLA-lesioned animals. A two-way mixed ANOVA was conducted on these data, with the variables of lesion (BLA, sham) and flavor (A, B). This revealed a significant main effect of flavor (F(1,13) = 4.94), no significant main effect of lesion (F < 1), and no lesion x flavor interaction (F < 1). Thus, both BLA- and sham-lesioned rats showed a sensory preconditioning effect, drinking less of a flavored solution that had previously been paired with a flavor to which they had developed an aversion, than of a flavored solution that had been paired with a neutral flavor.
Discussion
Experiment 1 confirmed that rats with BLA lesions show normal acquisition of appetitive Pavlovian conditioning. Both sham- and BLA-lesioned animals acquired autoshaped lever pressing with both sucrose and food pellet rewards. A satiety test was carried out to examine the BLA-lesioned rats' sensitivity to reinforcer devaluation. The CRs of the BLA-lesioned rats were insensitive to sensory-specific satiety, in both single-lever and choice tests, but a consumption test confirmed the success of the satiety treatment itself. This complements previous findings (Hatfield et al., 1996Experiment 2 sought to determine whether BLA-lesioned animals have a general deficit in adjusting responding according to the current motivational value of an associatively activated outcome representation. Rats were presented with two compound flavor stimuli, each made up of two different flavors. Subsequently, one of these flavors was devalued by pairing its consumption with nausea-inducing injection of LiCl. Both BLA- and sham-lesioned rats acquired the conditioned flavor aversion and also subsequently rejected the neutral flavor that had previously been paired with this newly devalued flavor. That is, they showed no deficit in outcome devaluation in a sensory preconditioning task, demonstrating that BLA-lesioned rats can alter their responding in accordance with the current motivational value of an associatively retrieved outcome representation.
Comparison of the designs of experiments 1 and 2 reveals that they are very similar in structure. In experiment 1, a CS was paired with a US, which in turn was devalued; lesions of the BLA interfered with expression of the devaluation in performance to the CS. In experiment 2, flavor A was paired with flavor X, which in turn was devalued; lesions of the BLA were without effect on expression of the devaluation in performance to flavor A. Comparing parameters in experiments 1 and 2, both the CS and US and flavors A and X were novel. The methods of devaluation (specific satiety and injection of LiCl) were different, but Hatfield et al. (1996
One interpretation of these contrasting results is that BLA lesions are without effect on neutral S-S learning. Hence, performance at test in experiment 2 is mediated by intact S1-S2 associations in both sham and lesioned animals. This complements recent findings suggesting that S-S associations in second-order conditioning are intact after BLA lesions (Setlow et al., 2002
One plausible account of the current data is that the BLA is only part of a wider limbic-cortico-striatal circuitry responsible for the representation of rewards. That is, there are extra-amygdala representations of associative outcomes that are capable of representing and updating their current motivational value. A substantial body of work has highlighted the role of connectivity between the amygdala, prefrontal cortex, and nucleus accumbens in the development of such representations (Balleine et al., 2003
Recent work (Blundell et al., 2001
In fact, the more conservative hypothesis that the BLA is responsible for the representation of the sensory properties of outcomes, regardless of their motivational salience, could also provide an explanation of these results. If we assume, contrary to the position above, that there is no representational difference between motivationally significant and neutral outcomes (for example, although the flavors presented in experiment 2 were neutral, they were presented in aqueous solution to thirsty animals), then a crucial difference could be that experiment 1 required formation of visual-taste (lever-food) associations, whereas experiment 2 required taste-taste associations. Failures in devaluation might, therefore, be because of deficits in cross-modal association rather than in reward representation. Although this hypothesis still requires that the BLA is responsible for associations involving the sensory, hedonic aspects of the US (i.e., the selective taste components of the reward), this explanation would be in line with previous interpretations of BLA function (Hatfield et al., 1992
In summary, we have demonstrated that BLA-lesioned animals can remain sensitive to post-training changes in the motivational value of outcomes. We have suggested (Blundell et al., 2001
Footnotes
Received Mar. 17, 2003; revised Jun. 30, 2003; accepted Jul. 2, 2003.This work was supported by a United Kingdom Medical Research Center (MRC) Career Establishment Grant to S.K. and by an MRC studentship to P.B.
Correspondence should be addressed to Dr. Pam Blundell, Department of Psychology, University of York, Heslington, York YO10 5DD, UK. E-mail: p.blundell{at}psych.york.ac.uk.
Copyright © 2003 Society for Neuroscience 0270-6474/03/237702-08$15.00/0
References
Balleine BW (2001) Incentive processes in instrumental conditioning. In: Handbook of contemporary learning theories (Mowrer RR, Klein SB, eds), pp 307-366. Hillsdale, NJ: Erlbaum.
Balleine BW, Dickinson A (2000) Effect of lesions of the insular cortex on instrumental conditioning: evidence for a role in incentive memory. J Neurosci 20: 8954-8964.
[Abstract/Free Full Text] Balleine BW, Killcross AS, Dickinson A (2003) The effect of lesions of the basolateral amygdala on instrumental conditioning. J Neurosci 23: 666-675.
[Abstract/Free Full Text] Berridge KC (1991) Modulation of taste affect by hunger, caloric satiety, and sensory-specific satiety in the rat. Appetite 16: 103-120.[ISI][Medline]
Berridge KC (1996) Food reward: brain substrates of wanting and liking. Neurosci Biobehav Rev 20: 1-25.[ISI][Medline]
Berridge KC (2001) Reward learning: reinforcement, incentives, and expectations. In: The psychology of learning and motivation—advances in research and theory, Vol 40 (Medin DL, ed), pp 223-278. San Diego: Academic.
Blundell PJ, Hall G, Killcross AS (2001) Lesions of the basolateral amygdala disrupt selective aspects of reinforcer representation in rats. J Neurosci 21: 9018-9026.
[Abstract/Free Full Text] Corbit L, Muir J, Balleine BW (2001) The role of the nucleus accumbens in instrumental conditioning: evidence for a functional dissociation between accumbens core and shell. J Neurosci 21: 3251-3260.
[Abstract/Free Full Text] Davey GCL, Cleland GG (1981) Topography of signal-centered behavior in the rat: effects of deprivation state and reinforcer type. J Exp Anal Behav 38: 291-304.
Dunn LT, Everitt BJ (1988) Double dissociations of the effects of amygdala and insular cortex lesions on conditioned taste-aversion, passive-avoidance, and neophobia in the rat using the excitotoxin ibotenic acid. Behav Neurosci 102: 3-23.[ISI][Medline]
Gallagher M, McMahan RW, Schoenbaum G (1999) Orbitofrontal cortex and representation of incentive value in associative learning. J Neurosci 19: 6610-6614.
[Abstract/Free Full Text] Goulet S, Murray EA (2001) Neural substrates of crossmodal association memory in monkeys: the amygdala versus the anterior rhinal cortex. Behav Neurosci 115: 271-284.[Medline]
Hall G (1996) Learning about associatively activated stimulus representations: implications for acquired equivalence and perceptual learning. Anim Learn Behav 24: 233-255.
Hatfield T, Graham PW, Gallagher M (1992) Taste-potentiated odor aversion learning: role of the amygdaloid basolateral complex and central nucleus. Behav Neurosci 106: 286-293.[ISI][Medline]
Hatfield T, Han JS, Conley M, Gallagher M, Holland P (1996) Neurotoxic lesions of basolateral, but not central, amygdala interfere with Pavlovian second-order conditioning and reinforcer devaluation effects. J Neurosci 16: 5256-5265.
[Abstract/Free Full Text] Holland PC, Gallagher M (2003) Double dissociation of the effects of lesions of basolateral and central amygdala on conditioned-stimulus potentiated feeding and Pavlovian-instrumental transfer. Eur J Neurosci 17: 1680-1694.[ISI][Medline]
Holland PC, Rescorla RA (1975) Second-order conditioning with food unconditioned stimulus. J Comp Physiol Psychol 88: 459-467.[ISI][Medline]
Howell DC (1997) Statistical methods for psychology, Ed 5. Belmont, CA: Wadsworth.
Jenkins HM, Moore BR (1973) The form of the auto-shaped response with food or water reinforcers. J Exp Anal Behav 20: 163-181.[ISI][Medline]
Killcross AS, Blundell P (2002) Associative representations of emotionally significant outcomes. In: Emotional cognition (advances in consciousness research) (Moore S, Oaksford M, eds), pp 35-73. Amsterdam: Benjamins.
Killcross AS, Everitt BJ, Robbins TW (1997) Different types of fear-related behaviour mediated by separate nuclei within amygdala. Nature 388: 377-380.[Medline]
Konorski J (1967) Integrative activity of the brain: an interdisciplinary approach. Chicago: University of Chicago.
Malkova L, Murray EA (1996) Effects of partial versus complete lesions of the amygdala on cross-modal associations in cynomolgus monkeys. Psychobiology 24: 255-264.
Malkova L, Gaffan D, Murray EA (1997) Excitotoxic lesions of the amygdala fail to produce impairment in visual learning for auditory secondary reinforcement but interfere with reinforcer devaluation effects in rhesus monkeys. J Neurosci 17: 6011-6020.
[Abstract/Free Full Text] Morris R, Frey S, Kasambira T, Petrides M (1999) Ibotenic acid lesions of the basolateral, but not the central, amygdala interfere with conditioned taste aversion: evidence from a combined behavioral and anatomical tract-tracing investigation. Behav Neurosci 113: 291-302.[ISI][Medline]
Nicholson DA, Freeman Jr JH (2000) Lesions of the perirhinal cortex impair sensory preconditioning in rats. Behav Brain Res 112: 69-75.[ISI][Medline]
Parkinson JA, Robbins TW, Everitt BJ (2000) Dissociable roles of the central and basolateral amygdala in appetitive emotional learning. Eur J Neurosci 12: 405-413.[ISI][Medline]
Rizley RC, Rescorla RA (1972) Associations in second-order conditioning and sensory preconditioning. J Comp Physiol Psychol 81: 1-11.[ISI][Medline]
Rolls ET (2000) The orbitofrontal cortex and reward. Cereb Cortex 10: 284-294.
[Abstract/Free Full Text] Setlow B, Gallagher M, Holland PC (2002) The basolateral complex of the amygdala is necessary for acquisition but not expression of CS motivational value in appetitive Pavlovian second-order conditioning. Eur J Neurosci 15: 1841-1853.[ISI][Medline]
Simbayi LC, Boakes RA, Burton MJ (1986) Effects of basolateral amygdala lesions on taste aversions produced by lactose and lithium chloride in the rat. Behav Neurosci 100: 455-465.[ISI][Medline]
Swanson LW (1998) Brain maps: structure of the rat brain. Amsterdam: Elsevier.
This article has been cited by other articles:
S. B. Ostlund and B. W. Balleine
Differential Involvement of the Basolateral Amygdala and Mediodorsal Thalamus in Instrumental Action Selection
J. Neurosci., April 23, 2008; 28(17): 4398 - 4405.
[Abstract] [Full Text] [PDF]
A. R. DELAMATER
The Role of the Orbitofrontal Cortex in Sensory-Specific Encoding of Associations in Pavlovian and Instrumental Conditioning
Ann. N.Y. Acad. Sci., December 1, 2007; 1121(1): 152 - 173.
[Abstract] [Full Text] [PDF]
S. B. Ostlund and B. W. Balleine
Orbitofrontal Cortex Mediates Outcome Encoding in Pavlovian But Not Instrumental Conditioning
J. Neurosci., May 2, 2007; 27(18): 4819 - 4825.
[Abstract] [Full Text] [PDF]
J. E. HADDON and S. KILLCROSS
Contextual Control of Choice Performance: Behavioral, Neurobiological, and Neurochemical Influences
Ann. N.Y. Acad. Sci., May 1, 2007; 1104(1): 250 - 269.
[Abstract] [Full Text] [PDF]
J.-C. Dreher, P. J. Schmidt, P. Kohn, D. Furman, D. Rubinow, and K. F. Berman
Menstrual cycle phase modulates reward-related neural function in women
PNAS, February 13, 2007; 104(7): 2465 - 2470.
[Abstract] [Full Text] [PDF]
D. M. Dwyer and S. Killcross
Lesions of the basolateral amygdala disrupt conditioning based on the retrieved representations of motivationally significant events.
J. Neurosci., August 9, 2006; 26(32): 8305 - 8309.
[Abstract] [Full Text] [PDF]
S. B. Ostlund and B. W. Balleine
Lesions of Medial Prefrontal Cortex Disrupt the Acquisition But Not the Expression of Goal-Directed Learning
J. Neurosci., August 24, 2005; 25(34): 7763 - 7770.
[Abstract] [Full Text] [PDF]
L. L. Wellman, K. Gale, and L. Malkova
GABAA-Mediated Inhibition of Basolateral Amygdala Blocks Reward Devaluation in Macaques
J. Neurosci., May 4, 2005; 25(18): 4577 - 4586.
[Abstract] [Full Text] [PDF]
S.-H. Wang, S. B. Ostlund, K. Nader, and B. W. Balleine
Consolidation and Reconsolidation of Incentive Learning in the Amygdala
J. Neurosci., January 26, 2005; 25(4): 830 - 835.
[Abstract] [Full Text] [PDF]
A. Izquierdo and E. A. Murray
Combined Unilateral Lesions of the Amygdala and Orbital Prefrontal Cortex Impair Affective Processing in Rhesus Monkeys
J Neurophysiol, May 1, 2004; 91(5): 2023 - 2039.
[Abstract] [Full Text] [PDF]
C. L. Pickens, M. P. Saddoris, B. Setlow, M. Gallagher, P. C. Holland, and G. Schoenbaum
Different Roles for Orbitofrontal Cortex and Basolateral Amygdala in a Reinforcer Devaluation Task
J. Neurosci., December 3, 2003; 23(35): 11078 - 11084.
