Neurotoxic Lesions of the Lateral Nucleus of the Amygdala Decrease Conditioned Fear But Not Unconditioned Fear of a Predator Odor: Comparison with Electrolytic Lesions

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The Journal of Neuroscience, May 15, 2001, 21(10):3619-3627

Neurotoxic Lesions of the Lateral Nucleus of the Amygdala Decrease Conditioned Fear But Not Unconditioned Fear of a Predator Odor: Comparison with Electrolytic Lesions
Karin J. Wallace and Jeffrey B. Rosen
Department of Psychology and Neuroscience Program, University of Delaware, Newark, Delaware 19716

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Considerable evidence suggests that the lateral (LA) and basal (BA) nuclei of the amygdala are sites of plasticity and storageof emotional memory. Recent arguments, however, have seriouslychallenged this view, suggesting that the effects of amygdalalesions are attributable to interference with performance of fearbehavior and not learning and memory. One way to address thiscontroversy is to measure the same behavioral response duringboth conditioned and unconditioned fear. This is done in the presentstudy by measuring fear-related freezing behavior after electrolyticand neurotoxic lesions of the LA or LA/BA nuclei in rats in acontextual fear conditioning paradigm and unconditioned fear toa predator odor. Electrolytic LA lesions attenuated post-shockfreezing, retention test freezing, and freezing to the predatorodor trimethylthiazoline (TMT). In contrast, excitotoxic NMDAlesions of the LA had no effect on post-shock freezing but significantlyattenuated retention test freezing. Furthermore, excitotoxic LAlesions did not diminish freezing to TMT. Larger excitotoxic lesionsthat included the BA significantly reduced freezing in both thepost-shock and retention tests but did not appreciably decreasefreezing to TMT. The results suggest that the LA is importantfor memory of learned fear but not for generation of freezingbehavior. In addition, the BA plays a role in freezing in conditionedfear situations but not in unconditioned fear. The studies suggestthat the LA and BA play different roles in fear conditioning,but neither of them has a significant role in unconditioned freezingto a predatorodor.

Key words: fear conditioning; context conditioning; amygdala; basolateral nucleus of the amygdala; lateral nucleus of the amygdala; basal nucleus of the amygdala; unconditioned fear; fox odor; freezing

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Much progress in understanding the neuroanatomy of fear has resulted from using simple well defined paradigms that measurespecies-typical defense responses primarily in rodents (e.g.,freezing, fear-potentiated startle, and autonomic changes) duringboth cue-specific (e.g., light and tone) and contextual classicalfear conditioning (i.e., environment without specific cue). Itis generally accepted that the basolateral complex of the amygdala(BLC), consisting primarily of the lateral (LA) and basal (BA)amygdaloid nuclei, plays a major role in receiving and integratingconditioned and unconditioned stimuli for fear conditioning (Davis,1997; Fanselow and LeDoux, 1999; Maren, 1999a; LeDoux, 2000).Indeed, electrolytic or neurotoxic damage to the LA or BLC blockthe learning of conditioned fear (LeDoux et al., 1990a; Kim etal., 1993; Campeau and Davis, 1995; Maren et al., 1996a; Cousensand Otto, 1998). This evidence, together with electrophysiologicaldata demonstrating neural activity changes during fear conditioning(Quirk et al., 1995; Rogan et al., 1997; Collins and Pare, 2000;Maren, 2000; Pare and Collins, 2000) and blockade of fear learningafter pharmacological manipulation in the amygdala (Miserendinoet al., 1990; Campeau et al., 1992; Maren et al., 1996b; Mulleret al., 1997; Wilensky et al., 2000), suggest that the BLC isa site of plasticity and storage of emotional information (Fanselowand LeDoux, 1999).

Recently, serious challenge to the view that the BLC is a locus of conditioned fear has emerged (Cahill et al., 1999; Vazdarjanova,2000). One major argument for this challenge is that there islittle direct evidence that distinguishes between the effectsof BLC lesions on memory versus performance. Thus, reduction inbehavioral measures of conditioned fear (primarily freezing andfear-potentiated startle) in BLC-lesioned animals may be attributableto a reduction of learning or may simply be a consequence of aninability of the lesioned animal to perform the necessary behavior.Cahill et al. (1999) suggest that, until it is shown that BLClesions block conditioned but not unconditioned fear behavior,it is premature to conclude that the BLC is necessary for learningand memory of conditionedfear.

The present study directly addresses this issue. Presentation of a predator odor, trimethylthiazoline [(TMT) originally isolatedfrom fox feces] has been shown to elicit a number of fear-associatedresponses in rats (Cattarelli and Chanel, 1979; Vernet-Maury etal., 1984, 1992; Heale et al., 1994; Hotsenpillar and Williams,1997; Morrow et al., 2000a,b; Wallace and Rosen, 2000). Most relevantto our application is the demonstration that rats reliably displayrobust unconditioned freezing behavior to TMT (Wallace and Rosen,2000). Thus, it is possible to measure the same fear-related behavior,freezing, during acquisition and retrieval of conditioned fearand during the presence of an ecologically relevant unconditionedfear stimulus in the same amygdala-lesioned rats. To determinewhether both types of fear are disrupted by specific amygdaladamage, the effects of both electrolytic and neurotoxic lesionsof the LA or combined LA and BA lesions on conditioned and unconditionedfear-related freezing wereanalyzed.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects
Male Sprague Dawley rats (Harlan Sprague Dawley, Indianapolis, IN) weighing 250-300 gm at surgery were used in these experiments.They were maintained on a 12 hr light/dark cycle, and food andwater were available ad libitum. All experiments were approvedby the University of Delaware Institutional Animal Care and UseCommittee.

Apparatus
During fear conditioning, rats were placed in a Plexiglas cylindrical chamber (8.6 cm diameter, 20 cm long; SR-Lab animalenclosure; San Diego Instruments, San Diego, CA). Plexiglas doorsdropped into slots at each end of the cylinder kept the rat inthe chamber. The rat was confined but not restrained and couldmove and turn around in the chamber, but when not turning facedone of the two doors. The cylinder was mounted on a Plexiglasplatform inside a cabinet of particleboard covered with Formica(30 × 30 × 60 cm; S-R chambers; San Diego Instruments). A gridfloor (San Diego Instruments) consisting of seven parallel stainlesssteel rods, each measuring 4 mm in diameter and spaced 1.3 cmapart (center to center), was placed on the floor of the cylinderand was attached to a scrambled shocker. A 25 W light bulb locatedin the roof of the cabinet was on at all times, and a fan in thecabinet provided a background noise of 70dB.
The same Plexiglas cylinders without the grid floors were used in the predator odor experiment but were placed in a fume hoodrather than the Formica-particleboard chambers. The fume hoodwas used to prevent the volatile odorant TMT from spreading intothe experimental room. TMT was presented to the animal by pipettingit onto a piece of Kimwipe that was taped to the inside of eachdoor. In both fear conditioning and presentation of the predatorodor, the chamber was cleaned with 5% ammonium hydroxide afterrunning each animal. In the TMT experiments, residual odor wasalso allowed to dissipate in the fume hood before another animalwas brought into the experimental room and placed in thechamber.

Procedure
Electrolytic lesions. Rats were anesthetized with a ketamine (100 mg/kg, i.p.) and xylazine (6.7 mg/kg, i.p.) solution forsurgery. Bilateral lesions of the LA were made in three locationsalong the rostrocaudal extent of the nucleus ~0.6 µm apart. Lesionswere made in four squads of rats with slightly different coordinatesand duration of current (Table 1). Stainless steel electrodesof 250 µm diameter, insulated except for 500 µm at the tip, wereused (model NE-300; Rhodes Medical Instruments, Woodland Hills,CA). Lesions were generated by passing a 0.1 mA anodal currentthrough the electrode tip. The cathode was attached to the rat'sfoot with an alligator clip. Rats were allowed 7-10 d to recover,during which time they were also handled.


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Table 1. Electrolytic lesion parameters

NMDA lesions. Rats were anesthetized as described for electrolytic lesions. Bilateral lesions of the LA were made by a singleinjection of NMDA (Sigma, St. Louis, MO) in each amygdala. Lesionswere made in three squads of animals using different amounts ofNMDA to obtain different sizes of damage. The needle of a 1.0µl Hamilton syringe (Hamilton Company, Reno, NV) was lowered tothe target site (from bregma: posterior, 3.3 mm; lateral, ±4.9mm; and ventral, 7.8 mm) and left in place for 2 min before injection.NMDA (20 mg/ml) was then infused at 0.05 µl/min, for a total injectionof 0.1, 0.15, or 0.2 µl. After infusion, the Hamilton syringewas left in place for an additional 5 min before removal, andthe same procedure was followed for the other amygdala. Rats wereallowed 7-10 d to recover, during which time they were alsohandled.

Behavior
Contextual fear conditioning. The simplest version of contextual fear conditioning was used in these experiments in whicha rat receives a foot shock after being placed in a novel environment(Fanselow, 2000). Rats were placed in the chamber for 3 min beforea 1.5 mA, 1 sec foot shock. Freezing was measured for 4 min immediatelyafter the foot shock (post-shock period). Freezing was definedas a characteristic crouch position with cessation of all movementexcept that associated with breathing (Blanchard and Blanchard,1969). Freezing was measured as a sample of freezing or not freezingevery 10 sec, for a total of 25 observations. The number of observationsof freezing was divided by 25 and then multiplied by 100 to obtaina percent of time spentfreezing.
A retention test of fear conditioning was conducted 24 hr after the foot shock by placing the animals back into the same chamberand recording freezing for 4 min as described above. In both thepost-shock and the retention tests, the observer was blind tothe condition (lesion group of each rat). Freezing data were statisticallyanalyzed with a mixed-model ANOVA (lesion group as a between-subjectsmeasure and freezing tests as a within-subjects measure), followedby a Scheffe's S post hoc test. $alpha$ values were set at p < 0.05.
Presentation of predator odor. After contextual fear conditioning, rats freezing behavior in the cylinders was extinguishedin the fume hood before presentation of TMT until they froze <20%of the time (no odor, but a Kimwipe on the door). This requiredfour to six 10 min sessions in the chamber once or twice per day,before being tested for freezing to TMT. On the testing day, ratswere placed in the chamber for a 3 min acclimation period, afterwhich the odorless doors were exchanged with doors containing150 nmol of TMT (19.4 µl) on each door. Freezing was recordedfor the following 11 min and was scored as a percent of time spentfreezing as described for context conditioning. This amount ofTMT was reported previously to elicit freezing ~75-80% of thetime (Wallace and Rosen, 2000) and at similar levels as foundafter a 1 sec, 1.5 mA foot shock in normal rats (Malkani and Rosen,2000; Thompson and Rosen, 2000).

Histology
After the conclusion of each experiment, rats were overdosed with sodium pentobarbital and perfused transcardially with 0.1M PBS, followed by 4% formaldehyde in 0.1 M PBS. Brains were removed,post-fixed, and cryoprotected (4% formaldehyde, 30% sucrose, and0.1 M PBS) for 4-10 d. Brains were frozen and sliced (Jung CM3000cryostat; Leica, Deerfield, IL) at 40 µm, mounted onto microscopeslides (Micro Slides, Selected, Precleaned Superfrost Plus; VWRScientific, West Chester, PA), and stained with cresyl violetto determine lesionlocations.
Lesions were located using a light microscope and mapped onto computerized coronal brain drawings from the Paxinos and Watsonrat brain atlas (1998) using NIH Image 1.59 on a 7600/132 PowerMacintosh (Apple Computers, Cupertino, CA). This was done forsix brain sections in each animal, covering the anteroposteriorextent of the amygdala. Analysis of lesion size in four nuclei[LA, BA, amygdalostriatal transition region (ASTR), and caudateputamen (CPu)] was conducted. For analysis of each lesion, thearea of each nucleus and the area of the lesion in the nucleuswere measured. Only the ventral half of the CPu was used as thearea of the nucleus measured because damage was confined to theventral CPu. A percent of each nucleus lesioned was calculatedby dividing the area of the lesion in the nucleus by the totalarea of the nucleus and multiplying by 100. These scores fromthe six drawings were then averaged to get a total percent ofthe nucleusdamaged.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrolytic lesions

Histology
Subjects were divided into three groups based on histology (LA, LA/ASTR, and no lesion). Most of the LA rats were from squads2 and 4, whereas ASTR rats were mostly from squad 3 (Table 1).Rats were included in the LA group if the lesion was centeredin the LA with only minor damage to the surrounding nuclei. LAlesions were bilateral and always included the dorsolateral divisionof the LA. Rats with lesions of the LA that included extensivelesions of surrounding areas were excluded. Based on these criteria,14 rats were included in the LA lesion group (Figs. 1A, 2). Themean ± SEM percentage of the LA destroyed was 56 ± 4%. In somerats, there was also slight damage to the dorsal endopiriformnucleus (11 ± 2% of the nucleus), the BA (7 ± 2% of the nucleus),the ASTR (9 ± 1% of the region), and/or the CPu (9 ± 2% of theventral half of the nucleus). The LA/ASTR group (n = 9) includedanimals with lesions of both the LA and the adjacent ASTR (Fig.2). This group generally had smaller lesions of the LA (41 ± 7.5%of the nucleus) but larger lesions of the ASTR (32 ± 4% of theregion) compared with the LA group. One animal included in thisgroup had very minor damage to the LA but significant damage tothe ASTR (Fig. 1B). All rats in the LA/ASTR group also had somedamage to the CPu (29 ± 3% of the ventral half of the nucleus).Damage to the LA was primarily concentrated in the dorsolateralportion, and damage to the ASTR tended to be located laterallyand close to the LA. The final no-lesion group consisted of animalswith sham lesions of the amygdala (n = 4) and no surgery (n =11). The behavior of these two subgroups did not differ and sowere combined for analysis. Fifteen rats were not included inthe analysis because their lesions were asymmetrical, unilateral,or not in the LA and could not be placed in a group. One of theserats was excluded from analysis because the lesion of the LA wassmall (24%), although it did have attenuated freezing.

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Figure 1. Coronal brain sections of electrolytic lesions from the LA group (A) and LA/ASTR group (B). The lesions are outlined in black. In A, the LA lesions had only slight damage of the ASTR, basal nucleus of the amygdala, and central nucleus of the amygdala. The lesions of the rat shown in B were primarily located in the ASTR, sparing much of the LA. This rat was unique because other rats in the LA/ASTR group had lesions of both the LA and ASTR. Behaviorally, attentuation of freezing in this rat was similar to the rest of the group. Ba, Basal nucleus of the amygdala; Ce, central nucleus of the amygdala; La, lateral nucleus of the amygdala.

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Figure 2. Schematic representations of largest and smallest electrolytic lesions in the amygdala at four rostral to caudal coronal levels (numbers indicate millimeters posterior from bregma). The sections are of the left ventral quadrants of coronal drawings containing the amygdala from the atlas of Paxinos and Watson (1998). Relevant structures are labeled in the left row of drawings. Lesions of the LA and LA/ASTR are in the middle and right rows, respectively. The gray areas represent the animals with smallest lesion and the black areas represent the largest lesion of each group. DEn, Dorsal endopiriform nucleus.

Effects of electrolytic lesions on contextually conditioned freezing
Once three groups were formed based on the lesions, context conditioning was analyzed using a 3 (groups LA, LA/ASTR, and nolesion; between measure) × 2 (post-shock vs retention; withinmeasure) mixed-model ANOVA. The data are presented in graphicform in Figure 3. There was an overall difference between thegroups during context conditioning (F_(2,31) = 53.1; p < 0.0001).Scheffe's S post hoc test demonstrated that rats with lesionsof the LA and LA/ASTR froze significantly less than rats in theno-lesion group. A difference in freezing between the LA/ASTRand the LA-lesioned rats failed to reach statistical significance(p < 0.063). There was also an overall difference between thepost-shock and the retention tests (F_(1,31) = 15.2; p < 0.0005).However, there was no interaction effect between the groups andtheir levels of freezing during the post-shock and retention tests(F_(2,31) = 0.23), indicating that the effects of LA and LA/STRlesions were an overall effect on a reduction in freezing in boththe post-shock and retention tests compared with the no-lesiongroup.

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Figure 3. Effects of electrolytic lesions on short-term and long-term memory of conditioned fear as measured by the percent of time spent freezing in the post-shock period and retention test, respectively. Freezing in the post-shock period was significantly more than during the retention test for all groups. Overall freezing (both post-shock and retention) in the LA and LA/ASTR groups was significantly less that the no-lesion group. There was no interaction effect.

These results of a significant attenuation of freezing complements a previous study of electrolytic lesions of the LA demonstratingdeficits in cue-specific conditioned freezing during a retentiontest (LeDoux et al., 1990a). Post-shock freezing was not analyzed.Together, the results of the two studies indicate that the LAplays a role in both cue-specific and contextual fear conditioningparadigms. In addition, our study indicates that larger lesionsthat contain both the LA and ASTR, or even lesions of the ASTRalone (Fig. 1B), contribute only a slight nonsignificant additiveeffect to lesions confined to the LA. Although the present resultsand those of LeDoux et al. (1990a) seem to support a role of theLA in fear conditioning, a decrease of freezing in both the post-shockand retention test without a differential effect on these testscompared with the no-lesion group confounds this interpretation.An alternative interpretation is that the LA simply reduced theability of the animals to freeze without affecting learning (fora detailed argument of this interpretation, see Cahill et al.,1999). This problem is addressed in the section on the effectsof NMDA lesions on fear conditioning. Those data are presentedafter presentation of the effects of electrolytic lesions of theLA and LA/ASTR on unconditioned freezing to a predatorodor.

Effects of electrolytic lesions on unconditioned freezing to TMT
On the day of TMT testing, rats froze on average <10% of the 3 min period before TMT was introduced into the chamber, andthere was no difference between the groups (mean ± SEM; LA, 6.8± 1.6%; LA/ASTR, 9.1 ± 1.8%; no lesion, 9.2 ± 2.5%). Differencesin freezing behavior before and during TMT presentation betweenthe groups were analyzed using a 3 (groups LA, LA/ASTR, and nolesion; between measure) × 2 (pre-TMT vs during TMT; within measure)mixed-model ANOVA. The data are presented in graphic form in Figure4. There was less freezing before TMT than during TMT presentation(F_(1,2) = 149.4; p < 0.0001) and an overall difference in freezingbetween the LA, LA/ASTR, and no-lesion groups (F_(2,32) = 27.2;p < 0.0001). A Scheffe's S post hoc test showed that all groupswere significantly different from each other, in which the no-lesiongroup had the highest and the LA/ASTR group had the lowest levelsof freezing. In addition, there was an interaction between thegroups freezing in the pre-TMT and during TMT periods (F_(2,32)= 33.0; p < 0.0001). This is attributable to a difference in freezingbetween pre-TMT and during TMT for the LA lesion and the no-lesiongroups but not the LA/ASTR group. A paired t test on the pre-TMTand during TMT freezing data in the LA/ASTR group was not significant(t₍₁₀₎ = 1.81; p > 0.1).

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Figure 4. Percentage of time rats with electrolytic lesions of the amygdala spent freezing to TMT. Freezing before TMT presentation (Pre TMT) did not differ between the groups. The three groups differed from each other on the percentage of freezing during TMT. Only the LA/ASTR lesions completely blocked freezing (there was no significant difference in freezing before and during TMT).

The data demonstrate that rats with lesions of the LA froze less than rats without lesions, although the lesions did not completelyblock freezing. In contrast, freezing was blocked with combinedlesions of the LA/ASTR and in one rat with lesions of the ASTR,suggesting that either the ASTR or some combination of the LAand ASTR is important for contextually conditioned freezing andfreezing to TMT. The ASTR is a small poorly characterized regionbetween the LA ventrally and laterally, the central nucleus medially,and the caudate putamen dorsally, but it is usually included aspart of the central nucleus of the amygdala because of cell morphology(McDonald, 1998). However, LeDoux et al.(1990b) have shown thatthalamic areas, including the posterior intralaminar nucleus andthe medial posterior complex, which project to the LA, also projectto the ASTR. Shi and Cassell (1999) reported recently that fibersfrom the perirhinal cortex, a region that projects to the LA,also terminate in the ASTR. Therefore, it is possible that theLA/ASTR lesions eliminated more of the afferent sensory fieldsimportant for conditioned and unconditioned freezing than didLA lesions alone. Nevertheless, what remains unresolved is thequestion of whether the effects produced by electrolytic lesionsare attributable to cells in the LA and ASTR or to fibers passingthrough these regions. The results from excitotoxic NMDA lesionspresented below address thisquestion.

NMDA lesions

Histology
Groups were determined by histological analysis of the area destroyed. Of the 67 rats infused with NMDA, only 25 had sufficientdamage to assign them to a group. Rats with lesions on only oneside of the brain were excluded because the interest was in theoverall effects of LA lesions on freezing. In addition, some animalswere excluded based on lesion placement outside of the amygdala.The remaining animals were divided into two lesion groups (Figs.5, 6) and one no-lesion group based on location and extent ofthe lesions. One lesion group was formed with lesions in the LA(n = 8). Rats in this group had 48.1 ± 6.2% (mean ± SEM) of theLA destroyed bilaterally, with the entire dorsolateral divisionof the LA destroyed in all animals except for two, in which themost dorsal tip of the nucleus was left undamaged. Animals withsignificant damage to the basal nucleus were not included in theLA group [only 3.9 ± 1.1% (mean ± SEM) of BA was lesioned]. Lesionsfrequently extended somewhat beyond the LA laterally and dorsallyand included parts of the dorsal endopiriform nucleus [32.1 ±5.8% (mean ± SEM) of the nucleus was damaged], the CPu (19.4 ±5.4% was damaged), and/or the ASTR (17.0 ± 4.1% was damaged).The central nucleus of the amygdala was not damaged. Another group[LA lesion plus damage to surrounding areas (LA+); n = 17] (Figs.5, 6) consisted of larger lesions of the LA (78.1 ± 4.9% was damaged),as well as more damage to other nuclei: the BA (34.4 ± 6.1% wasdamaged), ASTR (63.2 ± 4.0% was damaged), caudate putamen (37± 2.4% was damaged), and piriform cortex (specific amount of damagewas not determined). Again, the central nucleus of the amygdalawas not damaged. A final group did not have a visible lesion oneither side of the brain (no lesion; n = 8). Some of the casesin the no-lesion group had cannula tracks that were discernablenear the caudal end of the amygdala but did not appear to havea lesion surrounding the track. An additional group was addedto the analysis for behavioral comparison that did not have surgery(n = 9). Because their amount of conditioned freezing was no differentfrom the no-lesion group they were included in the no-lesion group,which increased the total number of subjects to 17. Unfortunately,a separate group with NMDA lesions confined to the ASTR couldnot be formed.

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Figure 5. Representative NMDA lesions in the amygdala. On the left is a low-magnification cresyl violet-stained coronal section of the amygdala. On the right are magnified regions (50×) of the lateral and basal nuclei of a single coronal section from each of the three experimental groups. The No Lesion specimen demonstrates normal cell morphology in lateral and basal nuclei. In the LA Lesion samples, gliosis dominates the lateral nucleus, but normal neuronal cell morphology is found the basal nucleus. The LA+ Lesion samples have only gliosis in both the lateral and basal nuclei.

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Figure 6. Schematic representations of largest and smallest NMDA lesions in the amygdala at four rostral to caudal coronal levels (numbers indicate millimeters posterior from bregma). The sections are of the left ventral quadrants of coronal drawings containing the amygdala from the atlas of Paxinos and Watson (1998). Relevant structures are labeled in the left row. Lesions of the LA and LA+ groups are in the middle and right rows, respectively. The gray areas represent the animals with smallest lesion and the black areas represent the largest lesion of each group. DEn, Dorsal endopiriform nucleus.

Effects of NMDA lesions on contextually conditioned freezing
For statistical analysis of the effects of NMDA lesions on contextual fear conditioning, a 3 (groups LA, LA+, and no lesion;between measure) × 2 (post-shock vs retention; within measure)mixed-model ANOVA was conducted. There was an overall differencebetween the groups (F_(2,39) = 22.8; p < 0.0001). Scheffe's S posthoc analysis revealed that the difference was attributable toa lower level of freezing in rats in the LA+ group compared withLA and no-lesion groups. This indicates that, overall, there wasnot an effect of NMDA lesions of the LA on freezing, but the largerlesions in the LA+ animals produced significant decreases in freezing.There was also a significant overall post-shock versus retentiondifference (F_(1,2) = 48.8; p < 0.0001) attributable to lower freezingscores on the retention test compared with freezing in the post-shockperiod. Most importantly, there was a significant interactioneffect between the groups and testing period (F_(2,39) = 4.2; p< 0.02) (Fig. 7A).

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Figure 7. NMDA lesion of the LA and LA+ on conditioned fear. A, Effects of NMDA lesions on short-term and long-term contextually conditioned fear as measured by the percentage of time spent freezing in the post-shock period and retention test, respectively. Freezing in the post-shock period was significantly more than during the retention test for all groups. The LA+ group had significantly less overall freezing than the no-lesion and LA groups. The post-shock freezing of the no-lesion and LA groups did not differ; however, there was significantly less freezing during the retention test in the LA group compared with the no-lesion group. B, The percentage of decrease in freezing in the retention test compared with the post-shock period. Both the LA and LA+ groups had a significantly greater percentage decrease of freezing in the retention test from the post-shock period than the no-lesion group.

To further analyze this significant interaction, two additional analyses were performed. Post-shock freezing between the groupswas compared using a one-way ANOVA, followed by a Scheffe's Stest. The significant difference in post-shock freezing (F_(2,39)= 20.0; p < 0.0001) was attributable to diminished freezing inthe LA+ groups compared with the no-lesion and LA groups. Theanalysis demonstrates that NMDA lesions confined to the LA hadno detrimental effects on freezing behavior per se, whereas largerlesions did. Because the post-shock freezing levels were differentbetween the groups, an analysis of differences in retention ofconditioned fear had to be corrected for these differential levelsin initial freezing. To standardize freezing scores across thegroups, a percent decrease in freezing score in the retentiontest and the post-shock period was derived for each subject bythe following formula: (retention test freezing/post-shock freezing× 100 $-$ 100. This results in a percent decrease in freezing inthe retention test compared with the post-shock period (Fig. 7B).A one-way ANOVA (F_(2,37) = 4.80; p < 0.01) followed by a Student-Newman-Keulspost hoc test was performed on these derived scores. There wasa significant difference (p < 0.05) between the LA and no-lesiongroups and between the LA+ and no-lesion groups but not betweenthe LA and LA+ groups. The analysis indicates that both lesionsconfined to the LA and larger lesions that destroyed the LA plusconsiderable portions of the BA, endopiriform nucleus, and ASTRproduced significant decrements in freezing during the retentiontest compared with the no-lesion group. Furthermore, when post-shockfreezing in the two lesion groups was compared with the no-lesiongroup (Fig. 7A), only freezing of the LA+ group, but not the LAgroup, was diminished. This indicates that NMDA lesions confinedto the LA had no detrimental effects on freezing behavior perse but did have specific effects on long-term memory of fear.In addition, because post-shock freezing is a measure of short-termmemory, the results suggest that short-term memory for fear conditioningoccurs independent of the LA. Lesions also including the ASTRand BA did decrease post-shock freezing, and possibly short-termmemory, but did not contribute more to the deficits in long-termmemory than lesions confined to the LA (Fig. 7B).

Effects of NMDA lesions on unconditioned freezing to TMT
A one-way ANOVA was conducted to determine differences in freezing to TMT between the groups (LA, LA+, and no lesion). Therewas a significant difference in freezing (F_(2,39) = 8.2; p < 0.001).A Scheffe's S post hoc analysis revealed a statistical differencebetween the no-lesion group and the LA+ group but no differencebetween the no-lesion group and lesions of just the LA. However,although there was a statistical difference between these groups,the drop in the amount of freezing to TMT was small. The LA+ groupstill froze ~63% of the time compared with 79% for the no-lesiongroup and was not statistically different from the LA group freezingof 67% of the time (Fig. 8).

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Figure 8. Percentage of time rats with NMDA lesions of the amygdala spent freezing to TMT. Freezing before TMT presentation did not differ between the groups. There was a slight but statistically significant decrease in freezing in the LA+ group compared with the no-lesion group.

To ensure that the lack of a reduction in freezing to TMT in the NMDA lesion rats was not attributable to an effect of beingtested after fear conditioning, two rats were tested for freezingto TMT before fear conditioning. These rats displayed the samereduction of fear conditioning freezing without an effect on freezingto TMT (73 and 67% of the time spent freezing toTMT).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results of the present study demonstrate that electrolytic lesions of the LA or the LA/ASTR substantially diminish freezingin a contextually conditioned fear paradigm. These lesions alsoreduced unconditioned freezing to a predator odor. The data tendto support Cahill et al.'s (1999) hypothesis that amygdala lesionsinterfere with freezing instead of learning and memory. In contrast,excitotoxic lesions of the LA had no effect on post-shock- orpredator odor-induced freezing but significantly reduced freezingduring the retention test for contextually conditioned fear. Theseresults suggest that the cells of the LA play a role in learningand memory of fear conditioning, whereas fibers passing throughthe LA and/or ASTR play a role in the expression of freezing behavior.Larger excitotoxic lesions that also included part of the BA andASTR produced deficits in both shock-induced freezing and freezingduring the retention test but had negligible effects on freezingto a predator odor. Therefore, contrary to the suggestion of Cahillet al. (1999), our results strongly indicate that BLC is not necessaryfor production of freezing behavior. The data also suggest thefollowing: (1) the LA plays a specific role in long-term memoryof fear, (2) the BA and ASTR are involved in both short- and long-termmemory, and (3) the neuroanatomy of fear conditioning and unconditionedfear to a predator odor aredifferent.

Role of LA in fear conditioning

Auditory, visual, and somatic information from the cortex and thalamus enters the amygdala primarily via the LA (Pitkanenet al., 1997; McDonald, 1998; Swanson and Petrovich, 1998). Duringfear conditioning, association between conditioned and unconditionedstimuli is thought to occur in the LA (Davis, 1997; Maren, 1999a;LeDoux, 2000). Electrolytic lesions confined to the LA block auditorycue-specific fear conditioning (LeDoux et al., 1990a), and electrophysiologicalrecordings in the LA during emotional learning indicate neuralplasticity (Quirk et al., 1995; Collins and Pare, 2000; Maren,2000; Pare and Collins, 2000). Our findings demonstrate that electrolyticand, more importantly, excitotoxic lesions confined to the LAcan also substantially attenuate retention of contextually conditionedfear. Previous studies have demonstrated that both post-shockfreezing and freezing in the retention test of the simple contextualfear conditioning paradigm used in the present study are associativelyconditioned (Faneslow, 1990). Although some types of contextualfear conditioning may be hippocampal-dependent (Kim and Fanselow,1992; Phillips and LeDoux, 1992), it appears that learning inthe simple contextual conditioning paradigm is not (Phillips andLeDoux, 1994; Fanselow, 2000). Nonetheless, the present studydemonstrates that the LA is not just important in cue-specificfear conditioning (LeDoux, 2000) but also for conditioning ina paradigm lacking a specificcue.

The present study further indicates that LA neurons are not necessary for post-shock freezing indicative of short-term memorybut are important for long-term memory of fear conditioning. Thedecrease in freezing during both the post-shock and retentiontest periods after electrolytic lesions confounds the interpretationof the involvement of the LA in learning and memory of fear, whichcould be viewed as a performance deficit (Cahill et al., 1999).However, NMDA lesions clarify that cells of the LA are not necessaryfor short-term memory or freezing behavior per se but are importantfor normal levels of long-term memory of fear. Sparing of normallevels of post-shock freezing but substantially reducing retentiontest freezing with LA excitotoxic lesions indicates that the LAis necessary for long-term but not short-term memory of conditionedfear.

The effects on fear-conditioned freezing were different when neural damage also included the BA and ASTR. Freezing was severelyattenuated in both the post-shock period and in the retentiontest by larger NMDA lesions that damaged the LA, ASTR, and BA.Several studies have now demonstrated that post-shock freezingas well as freezing in a retention test of contextual fear aresignificantly diminished in rats with large excitotoxic lesionsof the BLC (Maren, 1999b; Cahill et al., 2000). The present studyindicates there is a difference in the role of the LA and BA inshort-term and long-term memory of fearconditioning.

Although the present study can dissociate the effects of LA lesions on short-term memory (no effect on post-shock freezing)from long-term memory (a reduction in freezing on the retentiontest), it does not discriminate between consolidation and retrievalprocesses. Other data suggest that the LA may be involved primarilyin late phases (consolidation) of learning and long-term potentiation.Although some studies have found an initial increase and thendecrease in activity in LA neurons during conditioning (Quirket al., 1995, 1997), several groups have demonstrated increasedcellular activity in LA neurons commensurate with classical fearconditioning in cats and rats (Collins and Pare, 2000; Maren,2000; Pare and Collins, 2000). Electrophysiological recordingduring discriminatory instrumental fear conditioning in rabbitsdemonstrates that LA cells respond robustly during late phasesof learning but not earlier phases (Gabriel and Talk, 2001). Incontrast, BA cells respond robustly during early phases and diminishas learning proceeds (Gabriel and Talk, 2001), possibly indicatingthat the BA is more important for short-term than long-term memory.The LA also shows a late, persistent phase of LTP that is dependenton protein kinase A and mitogen-activated protein kinase (Huanget al., 2000). Interestingly, the expression of one of the targetsof these kinases, the immediate-early gene egr-1, is increasedspecifically within the LA after contextual fear conditioning(Rosen et al., 1998; Malkani and Rosen, 2000), suggesting partof a molecular pathway in the LA for long-term memoryprocesses.

Role of the LA in unconditioned freezing to a predatory odor

Previous research has demonstrated that rats will freeze, avoid, and have physiological responses to predator odors (includingTMT) that are indicative of unconditioned fear (Cattarelli andChanel, 1979; Blanchard and Blanchard, 1989; Heale et al., 1994;Berton et al., 1998; Burwash et al., 1998; Perrot-Sinal et al.,1999; Morrow et al., 2000b; Wallace and Rosen, 2000). Becauselarge lesions of the entire amygdala blocked fear responses tothe presentation of a cat (Blanchard and Blanchard, 1972; Foxand Sorenson, 1994), we expected that amygdala lesions would alsoreduce freezing to TMT. Indeed, electrolytic lesions of the LAsignificantly reduced freezing to TMT, and larger LA/ASTR lesionsalmost totally abolished freezing. In contrast, NMDA lesions ofthe LA had no effect on freezing to TMT, whereas larger lesionsof the LA+ group produced only a slight reduction in freezingto TMT. The data suggest that fibers passing through the basolateralcomplex and ASTR, and not the cells of the LA, ASTR, and BA, areresponsible for the large reductions in freezing. Although itis possible that a larger reduction in unconditioned freezingwould occur with larger NMDA lesions, the strong effects of theselesions on contextually conditioned freezing compared with theweak effects on freezing to TMT suggest that conditioned and unconditionedfreezing to TMT rely on different amygdalacircuitry.

It may not be surprising that the NMDA lesions of the LA did not affect freezing to TMT. The main olfactory bulb or olfactorycortex does not project directly to the LA. Nevertheless, olfactoryinformation can enter the amygdala via the piriform cortex andsuperficial amygdaloid nuclei, which project to the insular cortexand then through insular efferents to the central nucleus of theamygdala (Shipley et al., 1995). TMT may also activate the accessoryolfactory bulb via the vomeronasal organ and enter the amygdalathrough a direct projection to the medial nucleus of the amygdala(Shipley et al., 1995). However, what is of interest from theresults of the present study is that excitotoxic lesions producedprofound effects on conditioned freezing but had minimal effectson unconditioned freezing to a predator odor, again strongly indicatingthat LA and BA are not necessary for production of freezing behaviorper se. Although these findings are exciting, more work needsto determine whether the results are unique to TMT and unconditionedfear inducing olfactory stimuli. Indeed, lesions of the BLC orLA only disrupt unconditioned fear responses to a brightly litenvironment (Walker and Davis, 1997), a loud auditory stimulus(Bellgowan and Helmstetter, 1996), and a large ball of cat fur(A. Vazdarjanova, personal communication). Furthermore, the BLCappears to be necessary for fear conditioning when an olfactorystimulus is paired with foot shock (Otto et al., 2000). Theseresults suggest that the BLC may process visual and auditory stimuliinvolved in unconditioned fear responses and may be necessaryfor olfactory fear conditioning as it is with other types of fearconditioning.

In summary, the role of the LA in fear conditioning appears unique to long-term memory processes because freezing immediatelyafter learning was unaffected by NMDA lesions, but long-term memorywas reduced. Furthermore, an interesting dissociation betweenthe effects of lesions of nuclei of the basolateral complex onconditioned and unconditioned fear suggests that these amygdaloidnuclei are important for learning and memory of fear but not forexpression of some types of unconditionedfear.

  FOOTNOTES

Received Oct. 23, 2000; revised Feb. 27, 2001; accepted Feb. 27, 2001.

This study was supported by National Science Foundation Grant IBN-9904623 (J.B.R.).
Correspondence should be addressed to Dr. Jeffrey B. Rosen, Department of Psychology, University of Delaware, 220 Wolf Hall,Newark, DE 19716. E-mail: jrosen{at}udel.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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