Visual Pathways Involved in Fear Conditioning Measured with Fear-Potentiated Startle: Behavioral and Anatomic Studies

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The Journal of Neuroscience, December 15, 2001, 21(24):9844-9855

Visual Pathways Involved in Fear Conditioning Measured with Fear-Potentiated Startle: Behavioral and Anatomic Studies
Changjun Shi and Michael Davis
Department of Psychiatry and Behavior Science and Center for Behavior Neuroscience, Emory University School of Medicine, Atlanta, Georgia 30322

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Visual pathways to the amygdala, a brain structure critical for classical fear conditioning, were investigated. Conditionedfear was measured in rats as increased acoustic startle amplitudein the presence versus absence of a light or an odor paired previouslywith foot shock (fear-potentiated startle). Post-training lesionsof both the lateral geniculate body (LG) and lateral posteriornucleus (LP) of the thalamus together, but not lesions of LG orLP alone, completely blocked the expression of fear-potentiatedstartle to a visual conditioned stimulus (CS) but not to an olfactoryCS. These lesions also did not block contextual fear conditioningusing startle or freezing as measures. Local infusion of 1,2,3,4-tetrahydro-6-nitro-2,3-dioxo-benzo[f]quinoxaline-7-sulfonamide disodium, an AMPA antagonist, into thevisual thalamus immediately before testing also blocked fear-potentiatedstartle to a visual CS, suggesting that the lesion effects werenot attributable to damage of fibers of passage. Iontophoreticinjections into the LP of the anterograde tracer biotinylateddextran amine resulted in heavy anterograde labeling in two amygdala-fugalcortical areas: area TE2 and dorsal perirhinal cortex (PR), andmoderate labeling in the lateral amygdaloid nucleus (L). Theseresults suggest that, during classical fear conditioning, a visualstimulus can be transmitted to the amygdala via either lemniscal(i.e., LG $right-arrow$ V1, V2 $right-arrow$ TE2/PR) or non-lemniscal (i.e., LP $right-arrow$ V2,TE2/PR) thalamo-cortico-amygdala pathways, or direct thalamo-amygdala(i.e., LP $right-arrow$ L)projections.

Key words: fear; conditioning; amygdala; visual thalamus; perirhinal cortex; startle

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acquisition of conditioned fear depends on the association of a conditioned stimulus (CS) and an unconditioned stimulus (US).It is widely believed that CS and US information converges inthe basolateral amygdala in which the association and possiblyplasticity occurs (LeDoux et al., 1990; LeDoux, 1992, 2000; Romanskiet al., 1993; Davis et al., 1994; Shi and Davis, 1999). The pathwaysthrough which acoustic CS information is transmitted to the amygdalahave been studied extensively. Auditory inputs to the amygdalaarise from both auditory thalamus and the auditory associationcortex and terminate exclusively in the lateral amygdaloid nucleus(L) (LeDoux et al., 1990; Mascagni et al., 1993; Romanski andLeDoux, 1993b; Shi and Cassell, 1997; McDonald, 1998; Doron andLeDoux, 1999). Fear conditioning to a simple auditory CS can bemediated by either of these thalamo-amygdala or thalamo-cortico-amygdalapathways (Romanski and LeDoux, 1992b; Campeau and Davis, 1995b).In parallel, recent behavioral studies from our laboratory suggestedthat foot shock US information can be transmitted to the amygdaladuring fear conditioning via either thalamic or cortico-amygdalapathways (Shi and Davis, 1999). Although the amygdala is alsocritical for conditioned fear to a visual CS (LeDoux et al., 1989;Sananes and Davis, 1992; Campeau and Davis, 1995a), the brainstructures and pathways by which a visual CS accesses the amygdalaremainunknown.

In the rat, the superficial layers of superior colliculus (SC) are the major targets of retinal inputs (Linden and Perry,1983), and these, in turn, project to the visual thalamus. However,studies from our laboratory found that lesions or chemical inactivationof the superficial layers of the SC, in which the retina projects,did not disrupt the expression of fear-potentiated startle toa visual CS (Tischler and Davis, 1983; Meloni and Davis, 1999).The dorsal lateral geniculate nucleus (LGD) and the lateral posteriornucleus (LP) of thalamus receive direct projections from the retinaas well as from the SC, and these structures in turn project toretinotopically organized areas within the occipital cortex. However,post-training lesions of the occipital cortex did not preventeither the expression or extinction of conditioned fear responsesusing a visual CS (Tischler and Davis, 1983; LeDoux et al., 1989;Rosen et al., 1992; Falls and Davis, 1994), suggesting that subcorticaland/or additional thalamo-cortical pathways must contribute visualinformation to the amygdala. Anatomic tract tracing studies inour laboratory (Shi and Davis, 1999) suggested that the LP mightproject directly and/or indirectly via the perirhinal cortex (PR)and caudal temporal cortex to the amygdala in rat. Thus, thesethalamo-amygdala and thalamo-cortico-amygdaloid pathways couldallow a visual CS to activate the amygdala during visual fearconditioning.

The present experiments were designed to assess whether the visual thalamus, in particular the LP, is crucial in fear conditioningusing a visual CS and how this visual information is transmittedfrom LP to the amygdala. Rats were first trained to fear a lightby pairing it with foot shock. Electrolytic lesions restrictedto the LP, the dorsal lateral geniculate body (LG), or both structurestogether were performed after fear conditioning. Conditioned fearwas measured using fear-potentiated startle (increased acousticstartle amplitude in the presence vs absence of the visual CS)(Brown et al., 1951; Davis and Astrachan, 1978). To evaluate modalityspecificity, the effects of these lesions on fear-potentiatedstartle using an odor CS was performed. To evaluate the possiblecontribution of damage to fibers of passage, the effects on fear-potentiatedstartle of reversible inactivation of the visual thalamus usingpretest infusions of the AMPA receptor antagonist 1,2,3,4-tetrahydro-6-nitro-2,3-dioxo-benzo[f]quinoxaline-7-sulfonamidedisodium (NBQX) were also assessed. Anterograde tract tracingwith biotinylated dextran amine (BDA) was then used to identifythe potential thalamo-cortical and/or thalamo-amygdala connectionsthat may relay visual information to theamygdala.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects
Adult male albino Sprague Dawley rats (Charles River Laboratories, Portage, MI) weighing 350-400 gm were used. Animals forlesion or tract tracing studies were housed in groups of two orthree in plastic cages (20 × 26 × 48 cm), and those for infusionstudies were housed individually in wire cases (17 × 15 × 15 cm)with water and laboratory chow available ad libitum. They weremaintained on a 12 hr light/dark cycle (lights on at 7:00 A.M.).Behavioral procedures occurred during the light period. Rats wereacclimated to the colony rooms for 3 weeks before behavioralexperiments.

Apparatus
Animals were trained and tested in stabilimeter devices that have been described previously (Cassella and Davis, 1986). Briefly,each stabilimeter consisted of an 8 × 15 × 15 cm Plexiglas andwire mesh cage suspended within a steel frame. The floor of eachstabilimeter consisted of four 6.0-mm-diameter stainless steelbars spaced 18 mm apart through which shock could be delivered.Within the steel frame, the cage was compressed between four springsabove and a 5 × 5 cm rubber cylinder below, with an accelerometer(model 2217E; PCB Piezotronics, Depew, NY) located between thecage and the rubber cylinder. Cage movement resulted in displacementof an accelerometer in which the resultant voltage was proportionalto the velocity of the cage displacement. Startle amplitude wasdefined as the maximum accelerometer voltage that occurred duringthe first 0.2 sec after the startle stimulus was delivered. Theanalog output of the accelerometer was amplified (model 104; Endevco),digitized on a scale of 0-4096 units by a MacADIOS II board (GWInstruments, Somerville, MA) and stored on a Macintosh IImicrocomputer.
In the visual CS chamber, each of five stabilimeters was enclosed in a ventilated, light- and sound-attenuating box (68.5× 35.5 × 42 cm). This inner isolation box was located within anadditional outer ventilated plywood isolated box (76 × 47 × 51cm). The five wooden boxes, in turn, were housed in a larger ventilated,light- and sound-attenuating chamber (2.5 × 2.5 × 2.0 m; IndustrialAcoustic Co., Bronx, NY). A television camera (Ikegami, Maywood,NJ) for observing the behavior of the rats during the experimentwas positioned behind the stabilimeter within the inner isolationbox and was connected to a television monitor located outsideof the chamber. A red light bulb (7.5 W) was located on the floorof the inner isolation box to provide illumination for the camerasin the otherwise darkbox.
In the odor conditioning chamber, all training and testing occurred in two identical stabilimeter cages located within a soundattenuating chamber (inside dimensions of 56 × 56 × 81 cm; IndustrialAcoustics Co.). The Industrial Acoustics box was modified so thatthe top and inner walls were lined with 6.3 mm Plexiglas. In addition,the fiberglass material in the ventilation unit was removed toavoid absorption of odors. The odor CS was delivered through anolfactometer (model E15-03; Coulbourne Instruments, Allentown,PA) mounted outside of the sound-attenuating chamber. It consistedof three solenoid valves with three independent input ports mixingto a common output port. The output was routed into the chamberwith PharMed (Miami, FL) Tygon tubing (3.2 mm inner diameter ×6.3 mm outer diameter; Norton Plastics, Fisher Scientific, Houston,TX). Inside the chamber, the tubing was split with a "y" connector,and each end was attached to a 15 cm length of tubing that fittightly onto a tube that protruded through an opening in the topof each cage. To deflect any direct airflow onto the animal'sback, a 2.54 cm square metal shield bent in the form of a "V"was placed underneath the tube that delivered the airstream.
A compressed air tank (10 psi) was connected to a flowmeter (Fraser Harlake, Orchard Park, NY). From the flowmeter, the tubingwas split with a "y" connector to two separate check values toprevent back flow. Tubing from each check valve was connectedto activated carbon filter devices (Whatman Carbon-Cap 150; FisherScientific). Tubing from one filter was attached directly to oneof the input ports of the olfactometer ("air" solenoid). Tubingfrom the second filter was fitted with a check valve, and tubingfrom the valve was attached to a brass inlet connector in thelid of the jar containing 20 ml of the olfactant (I-CHEM100, 100ml glass jars with Teflon-lined polypropylene lids; VWR Scientific,West Chester, PA). The outlet connector in the lid was connectedto a second flowmeter, which connected to a second input portof the olfactometer ("odor 1" solenoid). The inlet and outletconnectors were sealed in the lid with 100% silicone adhesive(Dow Corning, Midland, MI) to avoid anyleakage.
After the rats were placed in the test cages, the air solenoid valve was opened to provide a clean air stream continuouslyduring all training and testing sessions at a rate of 2.00 l/minto clear the tubing both before and after odor presentations.Between individual training-testing sessions, once the animalswere removed from the cages, clean air was delivered through thetubing for an additional 5 min to further clear any residual odor.For the odor cue presentations, the odor 1 solenoid valve containingthe olfactant was opened for 4 sec and blended into the air streamat a flow rate of 0.75 l/min. When the odor solenoid was opened,the clean airflow rate dropped to 1.25 l/min, making the finalstimulus flow rate 2.00 l/min. Hence, the introduction of theodor did not lead to any net change in airflow.
A blower fan (McMaster-Carr, Atlanta, GA) provided a continuous influx of clean air into the chamber, and an exhaust fan (McMaster-Carr)continually exhausted air from the chamber to minimize any odorlingering between CS presentations. Air was exhausted througha 7.62-cm-diameter opening at a rate of 10.16 cubic feet per secondas measured by a Kestrel 1000 wind meter (Nielsen-Kellerman, Chester,PA). The stabilimeter cages and chamber were cleaned daily aftertraining-testing sessions with warm tap water and 95% alcoholand were air dried for at least 8hr.

Stimuli
All sound level measurements were made with a Precision Sound Level Meter (A scale, model 2235; Brüel & Kjær, Norcross, GA).Background noise (0-20 kHz, 55 dB) was produced by a white-noisegenerator (model 15800; Lafayette, Lafayette, ID) and deliveredthrough high-frequency speakers (Radio Shack Supertweeters; range,5-40 kHz) located 2 cm from the front of each stabilimeter. Thisplus the noise of the ventilating fan attached to the sidewallof each wooden box produced an overall background noise levelof 64 dB. The startle stimulus was a 50 msec burst of white noise(5 msec rise-decay time) of various intensities generated by awhite-noise generator (Model 15800; Lafayette) and delivered throughthe same speakers as the backgroundnoise.
The visual CS was a 3.7 sec light produced by an 8 W fluorescent bulb (100 µsec rise time, 700 feet lamberts) attached tothe back of each stabilimeter. The US was a 0.4-0.6 mA foot shockwith a duration of 0.5 sec, generated by five LeHigh Valley (Beltsville,MD) constant-current shockers (model SGS-004) located outsideof the chamber. Shock intensity was measured with a 1 k $Omega$ resistoracross a differential channel of an oscilloscope in series witha 100 k $Omega$ resistor connected between adjacent floor bars withineach stabilimeter. Current was defined as the root mean squarevoltage across the 1 k $Omega$ resistor, in which milliamperes is 0.707× 0.5 × peak-to-peakvoltage.
The odor CS was created by the air stream passing through a 5% solution of amyl acetate (Sigma, St. Louis, MO) diluted inpropylene glycol. The odor CS was freshly prepared each day beforetraining-testing sessions. The presentation and sequencing ofall stimuli were under the control of the Macintoshcomputer.

Behavioral procedures
Matching. On the first 2 d of all experiments, rats were placed in the startle cages, and baseline activity was sampled onceevery 10 sec for the first 5 min. An activity sample was definedas the peak accelerometer voltage that occurred during a 500 msecsampling period. Then, animals were presented with 30 startlestimuli at a 30 sec interstimulus interval (ISI). Intensitiesof 90, 95, and 105 dB were used with 10 startle stimuli at eachintensity. Startle stimuli were presented in a balanced, irregularsequence with the restriction that each of the three intensitieshad to occur once in each trial block. The mean startle amplitudeacross the 30 startle stimuli on the last matching day was usedto assign rats into sham or lesion groups, such that the meanstartle level for each group before training wascomparable.
Training. Rats were placed in the stabilimeter cages and, 5 min later, were presented with the first of 10 visual or fiveodor CS-shock pairings. The shock was delivered during the last0.5 sec of the CS at an average intertrial interval of 4 min (range,3-5min).
Testing. Rats were placed in the same startle cages in which they were trained, and baseline activity was sampled once every10 sec for the first 5 min. Then, for the visual CS, animals werepresented with 18 startle-eliciting stimuli in the dark (six ateach of three intensities: 90, 95, or 105 dB). These initial startlestimuli (hereafter called "leaders") were used to evaluate fear-potentiatedstartle to the context compared with baseline startle during secondday matching. Thirty seconds after the last leader stimulus, eachanimal received 60 startle stimuli (20 at each of three intensities:90, 95, or 105 dB), with half of the stimuli presented alone (noise-alonetrials) and the other half presented 3.2 sec after the onset ofthe 3.7 sec CS (light-noise trials). The six trial types werepresented in a computer-generated randomized order with the restrictionthat each trial type had to occur once within each block of sixtrials. All startle stimuli were presented at a 30 secISI.
For testing with the odor CS, the animals were placed individually into the two test cages within the olfactory chamber. Aftera 5 min acclimation period, animals were presented with 30 95dB startle stimuli at a 30 sec interstimulus interval. Thirtyseconds after the last leader trial, the animals were presentedwith the first of 10 odor plus startle stimulus trials (odor-noisetrials). On these test trials, the odor was delivered for 4 sec,and then the 50 msec startle stimulus was delivered 3.5 sec afterthe onset of the CS. After each odor-noise trial, three noise-alonetrials were presented at a 30 sec intertrial interval so thatnoise-alone trials occurred 30, 60, and 90 sec after eachodor.

Statistical analyses
Freezing to the context was defined as the mean activity before training minus the mean activity after training. Fear-potentiatedstartle to the context was defined as the mean startle amplitudeof leaders during testing minus the mean startle amplitude (acrossthe first 18 trials) during the second day of matching. Fear-potentiatedstartle to an explicit CS was defined as the difference in startleamplitude on the light-noise or odor-noise minus the noise-alonetrials. ANOVAs were conducted using trial type (light-noise orodor-noise versus noise-alone) as a within-subjects factor andlesion or drug infusion as between-subjects factors. These analyseswere complemented, when required, by ttests.

Surgery
Stereotaxic surgical procedures were performed under anesthesia with sodium pentobarbital (50 mg/kg, i.p.). All coordinateswere based on the rat atlas of Paxinos and Watson (1997).
Electrolytic lesions. Lesions were made with stainless steel electrodes (0.25 mm in diameter) insulated except for the 0.5mm at the tip. A constant-current source generated DC anodal currentfor all electrolytic lesions at an intensity of 1.0 mA. Lesionsof LG or LP were performed by making two lesions at differentanteroposterior coordinates on each side of the brain. Combinedlesions of LG and LP were produced by making four lesions at differentanteroposterior coordinates on each side of the brain. Detailedcoordinates for each lesion are shown in Table 1. The anteroposterior(AP) and lateromedial (LM) coordinates are relative to bregma;the dorsoventral (DV) coordinates are relative to the surfaceof the brain above the targets. For sham lesions, the electrodewas lowered 1.0 mm above the dorsoventral lesion coordinate withoutpassing current.


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Table 1. Coordinates of electrode placements for electrolytic lesions

Cannulations. Rats were stereotaxically implanted with guide cannulas (22 gauge, 11 mm length; Plastics One Inc., Roanoke,VA) aimed bilaterally at the visual thalamus at the followingcoordinates: AP, $-$ 4.6 mm; ML, ±3.0 mm; and DV, $-$ 4.6 mm (to dura).The implanted cannulas were held in place using jewelers screwsattached to the skull and a crown of dental acrylic. Cannula patencywas maintained using internal stylets that protruded 1 mm beyondcannulatips.
Tract tracing. The anterograde tracer BDA (10,000 molecular weight; 10% in 0.1 M PBS; Molecular Probes, Eugene, OR) was iontophoreticallyinjected via a glass micropipette (tip diameter of 20-35 µm) atvarious locations of the target areas. After placement of themicropipette, a constant positive current of 4 µA was appliedfor 5-10 min using a constant-current generator. The micropipettewas then slowly removed, and the scalp incision was closed. Animalswere allowed to survive for 4-7 d beforeperfusion.

Histology
For perfusions, animals were given an excessive dose of chloral hydrate and then exsanguinated with 100 ml of physiologicalsaline and perfused through the ascending aorta with 500 ml offixative containing 4% paraformaldehyde in 0.1 M PBS, pH 7.4,for 30 min. Brains were removed and stored in a solution of 30%sucrose in formalin for at least 2 d. Sections (50-µm-thick) werecut through lesion or cannulation sites on a frozen microtomeand mounted on gelatin-coated slides. After drying, the slideswere stained with cresyl violet, and the extent of the lesionor location of the cannula tip was evaluated under amicroscope.
The brains with BDA injections were sectioned into 30-µm-thick coronal sections using a freezing microtome. Serial sectionswere collected and stored in cold PBS. BDA was visualized by incubatingsections for 2 hr at room temperature in ABC reagent (Vector Laboratories,Burlingame CA) diluted in 0.1 M PBS (1:100) containing 0.3% TritonX-100, followed by a second incubation in biotinylated goat anti-avidin(Vector Laboratories) diluted in 0.1 M PBS (1:200) containing0.3% Triton X-100 for 2 hr. Sections were then reincubated inABC for 1 hr. Between each incubation, sections were washed for15 min in three changes of PBS. Peroxidase histochemistry wasperformed by reacting the sections for 10 min in a solution containing0.05% diaminobenzidine and 0.01% hydrogen peroxide in 0.1 M phosphatebuffer. Sections were mounted on chrome alum-gelatin-coated slidesand mounted in Eukitt after dehydration and clearing. Alternatesections were counterstained with cresyl violet. The distributionof anterograde labeling in the cortex was analyzed using dark-fieldillumination. The position and density of labeled fibers and terminalswere imaged with a digital camera (model DXC5000; Sony, Tokyo,Japan) of representativesections.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effects of post-training lesions of LG and/or LP on expression of fear-potentiated startle to a visual CS

This experiment evaluated the effects of lesions of dorsal LG and/or LP on expression of fear-potentiated startle in whichanimals were lesioned after training. A total of 52 rats werematched into six groups of 8-10 rats each. On the following 2d, all animals were conditioned by pairing the light with footshock. One or 2 d after training, rats received electrolytic orsham lesions aimed at the LG alone, the LP alone, or both. Oneweek after surgery, animals were tested for fear-potentiatedstartle.

Histology
Figure 1 shows histological reconstructions of representative cases with the LP or LG nucleus lesions. Figure 2 shows histologicalreconstructions depicting the smallest and largest LP-LG lesionsincluded in the analysis. From the 10 rats that received bilateralelectrolytic lesions aimed at LP, two were excluded because ofincomplete damage to the LP. Because the dorsal part of the suprageniculatethalamic nucleus (SG) shares similar connectivity as mediocaudalLP (see Discussion), we considered this area as a part of LP andincluded it in the lesion sites. In the other rats (n = 8), therewas also inconsistent damage to the adjacent posterior nucleusof thalamus, anterior pretectal nucleus, and dorsal portion ofthe medial geniculate body. However, no case had significant damageto LG. In the nine animals with intended LG lesions, six had acomplete lesion of the LGD without significant damage to the adjacentLP and were included in the analyses. Most of these cases alsohad complete bilateral damage to the ventral lateral geniculatenucleus (LGV). In the combined lesion group, three animals hadincomplete damage to the LGD and/or LP, and their data were thusexcluded from the statistical analyses. In the animals with completeLG-LP damage (n = 6), there was also variable damage to the LGV,lateral dorsal, posterior, ventroposterior, peripeduncular, andanterior pretectal thalamic nuclei, as well as to the medial geniculatebody.

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Figure 1. Histological reconstructions of representative cases with post-training lesions of lateral posterior (left column) and lateral geniculate (right column) thalamic nuclei on coronal plates from the atlas of Paxinos and Watson (1997). The numbers to the right indicate rostrocaudal levels relative to bregma. Shaded areas indicate lesion sites. See Table 2 for abbreviations.


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Table 2. Abbreviations list

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Figure 2. Histological reconstructions of the smallest (left column) and largest (right column) combined lesions of lateral geniculate and lateral posterior nuclei of thalamus transcribed on coronal plates from the atlas of Paxinos and Watson (1997). The numbers to the right indicate rostrocaudal levels relative to bregma. Shaded areas indicate area lesion extent. See Table 2 for abbreviations.

Fear-potentiated startle
Figure 3A-C shows the mean startle amplitude on noise-alone and light-noise trials and the difference scores between thesetwo trial types for animals with sham, LP, LG, or LG-LP lesions.Figure 3A shows that startle amplitudes during light-noise trialswere significantly greater than startle amplitudes during noisealonetrials in both sham (t₍₇₎ = 6.16; p < 0.01) and LP-lesioned (t₍₇₎= 7.39; p < 0.01) animals, indicative of fear-potentiated startleto visual CS in both groups. A repeated-measures ANOVA found notreatment × trial type interaction (F_(1,14) = 0.24; p > 0.05),indicating that the LP lesion did not significantly alter themagnitude of fear-potentiated startle. Figure 3B shows that theLG-lesioned groups also exhibited significant fear-potentiatedstartle to a visual CS (t₍₅₎ = 2.87; p < 0.05), as did the shamanimals (t₍₇₎ = 3.24; p < 0.05), indicative of conditioned fear.There was no significant treatment × trial type interaction (F_(1,12)= 0.38; p > 0.05), indicating equivalent levels of fear-potentiatedstartle in the sham versus lesioned groups.

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Figure 3. Mean amplitude startle response on noise-alone trials (black bars) and light-noise trials (white bars) and the difference (+SEM) between these two trial types (gray bars) in sham-operated and lesioned animals (A-C) and in rats infused with PBS or NBQX in the chemical inactivation experiment (D). A, LP lesions; B, LG lesions; C, combined LG and LP lesions; D, chemical inactivation of visual thalamus with NBQX. The post-training lesions of LP or LG alone had no significant effect on fear-potentiated startle, but either combined post-training lesions of LG and LP or pretesting chemical inactivation of the visual thalamus completely blocked expression of fear-potentiated startle to a visual CS.

Figure 3C shows that, in the combined LG-LP-lesioned group, there was no increase in startle amplitude on the light-noiseversus noise-alone trials (t₍₅₎ = 0.11; p > 0.05). In contrast,sham animals exhibited a significant increase in startle amplitudeon the light-noise versus noise-alone trials (t₍₇₎ = 6.13; p <0.01). A repeated-measures ANOVA showed a significant treatmentcondition × trial type interaction (F_(1,12) = 25.42; p < 0.01)between the two groups. An ANOVA on the noise-alone scores showedno significant differences in startle amplitude (F_(1,12) = 0.67;p > 0.05). These data indicate that post-training electrolyticlesions of the LG or LP alone had no effect on the expressionof fear-potentiated startle, but combined lesions of both completelyblocked the expression of fear-potentiated startle to a visualCS

Lesions of visual thalamus did not interrupt expression of fear-potentiated startle to either an olfactory or a context cue

To test that the above lesion effects were specifically interrupting transmission of visual information to the amygdala ratherthan a general failure of memory retrieval or failure of enhancementof startle, this experiment evaluated the expression of fear-potentiatedstartle using an olfactory cue as a CS. Conditioned fear to thecontext was also measured in the test chamber in which the animalstrained and tested with the visual CS. A total of 16 rats werematched into two groups of eight rats each. After matching tests,animals were first conditioned by pairing the light with footshock for 2 d. On the following day, all animals were conditionedby pairing an odor with foot shock in a novel chamber. One or2 d after training, rats received electrolytic or sham lesionsof visual thalamus. After recovery, animals were first testedfor freezing to the context and fear-potentiated to the contextas well fear-potentiated startle to the visual CS in the samechamber used for light-shock pairing training (see Materials andMethods). On the second day, animals were retested for fear-potentiatedstartle to the odor CS in the odor conditioningchamber.

Histology
From the eight rats that received bilateral electrolytic lesions aimed at LP and LG, three were excluded because of incompletedamage to the targets. In the other rats (n = 5), the lesion extentwas similar to the combined lesion group described above. Oneof eight animals in the sham-lesioned group exhibited extremelylow baseline startle after surgery, and its data were excludedfrom the statisticalanalyses.

Fear-potentiated startle
Lesions of visual thalamus totally blocked fear-potentiated startle to visual CS but not to the odor CS. Figure 4, A and B,shows the mean startle amplitude on noise-alone and light-noiseor odor-noise trials and the difference scores between these twotrial types for animals with sham or LG-LP lesions. Consistentwith the previous results, the visual thalamus-lesioned animalsdid not exhibit any increase in startle amplitude on the light-noiseversus noise-alone trials (t₍₄₎ = 0.335; p > 0.05), whereas shamanimals exhibited a significant increase in startle amplitudeon the light-noise versus noise-alone trials (t₍₆₎ = 4.153; p< 0.01). A repeated-measures ANOVA showed a significant treatmentcondition × trial type interaction [F_(1,10) = 11.782; p < 0.01)between the two groups. In contrast, both sham (t₍₆₎ = 2.634;p < 0.05) and lesion (t₍₄₎ = 2.527; p < 0.05) animals exhibitedsignificant increases in startle amplitude on the odor-noise versusnoise-alone trials. A repeated-measures ANOVA showed no significanttreatment condition × trial type interaction (F_(1,10) = 1.023;p > 0.05) between the two groups.

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Figure 4. Fear-potentiated startle responses (FPS) to the visual (A), olfactory (B), and contextual (C) CSs, and freezing responses to the context (D) in sham-operated and visual thalamus-lesioned animals. Combined lesions of the LG and LP specifically blocked expression of fear-potentiated startle to the visual CS but had no effect on fear-potentiated startle to the odor CS, as well as startle or freezing to the context.

Furthermore, post-training lesions of visual thalamus had no effect on expression of conditioned fear responses to the trainingcontext using both fear-potentiated startle (Fig. 4C) and freezing(Fig. 4D) as measures compared with shams. A repeated-measuresANOVA showed a significant overall difference of activity (F_(1,10)= 31.43; p < 0.01) and startle amplitude (F_(1,10) = 13.982; p< 0.01) between the pretraining and post-training trials, indicativeof significant freezing and fear-potentiated startle to contextCS. However, there was no treatment × trial type interaction (F_(1,10)= 0.147 for activity; F_(1,10) = 0.455 for startle; p > 0.05).These data indicate that post-training electrolytic lesions ofthe LG and LP had no effect on the expression of conditioned fearto either the olfactory cue or context CS, although it completelyblocked the expression of fear-potentiated startle to a visualCS.

Pretesting infusion of NBQX into visual thalamus blocks expression of fear-potentiated startle to a visual cue

Because electrolytic lesions damage both neurons and passing fibers, this experiment reevaluated the role of dorsal lateralgeniculate and lateral posterior nuclei on expression of fear-potentiatedstartle using local infusion of NBQX, an AMPA receptor antagonist,to temporarily block local glutamate transmission at AMPA receptorswithin thesestructures.

After cannula implantation, animals recovered for 1 week before being matched into two groups. On the next 2 d, the rats weregiven fear conditioning and tested for potentiated startle thenext day. Immediately before behavioral testing, rats were infusedwith 6 µg of NBQX (dissolved in a 1 µl volume of PBS; ResearchBiochemicals, Natick, MA) or with PBS alone. Infusions (0.25 µl/min)were made through 28 gauge injection cannulas attached by polyethylenetubing to a Hamilton microsyringe. After the infusion was completed,the injection cannulas were left in place for 2 min before beingwithdrawn.

Histology
Ten of the 33 animals did not have bilateral cannulation of the visual thalamus or lost their head caps before testing, andtheir data were excluded from additionalanalyses.

Fear-potentiated startle
As shown in Figure 3D, startle amplitude during light-noise trials was significantly greater than startle amplitude duringnoise-alone trials for PBS-infused rats (t₍₁₁₎ = 3.86; p < 0.01).Infusion of NBQX into the visual thalamus had no effect on baselinestartle (i.e., noise-alone trials) (F_(1,21) = 0.02; p > 0.05)compared with PBS-infused rats but completely blocked fear-potentiatedstartle to a visual CS, as shown by the lack of difference betweenstartle amplitude on the light-noise versus noise-alone trialsafter infusion of NBQX (t₍₁₀₎ = 0.47; p > 0.05), as well as asignificant difference in fear-potentiated startle (i.e., differencescores) for PBS- versus NBQX-infused rats (t₍₂₁₎ = 3.04; p < 0.01).These data indicate that glutamate transmission via AMPA receptorsin the visual thalamus is crucial for the expression of fear conditioningusing a visual CS. Furthermore, these data suggest that the blockadeof fear-potentiated startle by electrolytic lesions of the visualthalamus was not attributable to damage of the optic track and/orbrachium of superior colliculus, which carry efferents from retinaand SC to visual thalamus and the pretectum. Finally, these datastrongly suggest that visual transmission within the visual thalamusis mediated by glutamate acting on AMPAreceptors.

Anterograde tract tracing with BDA from LP

Because the LP proved to be critical for the expression of fear-potentiated startle using a visual CS and because the amygdalaalso is critical in this test (LeDoux et al., 1989; Sananes andDavis, 1992; Campeau and Davis, 1995a; Lee et al., 1996), we usedthe anterograde tracer BDA to map the pathways that connect theLP to the amygdala. Because the caudal boundary of LP with medialgeniculate body is very difficult to determine on Nissl-stainedcoronal sections, we used the termination of superior colliculusafferents to define the extent of LP based on BDA injections intothe superficial layers of superior colliculus in several additionalanimals.

Figure 5 shows a representative BDA injection (A) into the superior colliculus and the termination pattern in the visual thalamus(B-D). The injection was centered in the superficial layers inwhich retinal inputs are distributed. Heavy anterograde labelingwas present in the midcaudal two-thirds of the LP, covering themost caudal part of laterorostral LP and the whole extent of itslaterocaudal (LPLC) and mediocaudal (LPMC) subdivisions. In contrast,the most rostral LP exhibited only scattered labeled axon fibersand terminals. As shown in Figure 5D, very dense labeling in caudalLP extended ventromedially into the dorsal half of the SG, whichis generally included in the auditory thalamus. Thus, at leastthis dorsal portion of SG, which was targeted by visual inputsfrom superior colliculus like the rest of the caudal LP, shouldbe considered as a subdivision of the visual thalamus (LPSG).Finally, as expected, injections into superficial layers of theSC produced a dense and topographically organized distributionof anterograde labeling in LGD and LGV.

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Figure 5. Digital dark-field photomicrographs of representative coronal sections through midcaudal levels of the visual thalamus showing the distribution of labeled tecto-thalamic fibers and terminals (B-D) after a BDA injection into the superficial layers of the superior colliculus (A). Note the continuity of labeling between the dorsal SG and LPMC in D. Scale bars, 200 µm. See Table 2 for abbreviations.

Injections of BDA into different subdivisions of LP produced topographically organized anterograde labeling in associationwith visual cortex and medial and lateral V2. Because the detailsof this visual cortical projection are not the focus of this study,they will be presented elsewhere. The animals with injectionsinto medial and caudal LP exhibited heavy anterograde labelingin temporal cortical area TE2, dorsal PR, and the lateral nucleusof the amygdala. Two representative cases (3 and 47) are illustratedand describedhere.

In case 47, the injection site was located in the most caudomedial part of LP, involving the medial part of LPMC and adjacentLPSG (Fig. 6A). This injection produced heavy anterograde labelingin dorsal PR (Fig. 6B) and moderate labeling in lateral amygdaloidnucleus, amygdalostriatal transition zone, and posterior striatum(Fig. 6C,D). The labeling in PR extended rostrally from ~3.8 mmbehind bregma to the caudal end of the rhinal sulcus, with a predominancein its rostral half. In coronal sections, terminal labeling inPR was densest in the middle layers (III and IV) and layer I.The layer I labeling of PR extended dorsally into TE3 but withmuch lower density and was restricted to the superficial portion.There was no labeling in the middle layers of TE3, indicatingthat the effective injection site did not invade dorsal medialgeniculate body, which projects mainly to the middle laminas ofTE3 (our unpublished observation). Subcortically, anterogradelabeling was present in the L, the amygdalostriatal transitionzone, and the caudal caudate-putamen. Labeling in the L was moderatein density and extended to its midcaudal two-thirds. In coronalsections, labeling was mostly distributed in the dorsolateralsubdivision, with highest density in the ventromedial portion,similar to the projection pattern of visual association cortexarea TE2. This contrasts with the termination pattern of acousticinputs from auditory thalamus and cortex (area TE3), which mainlytargets the most dorsal portion of the lateral nucleus (Romanskiand LeDoux, 1993b; Shi and Cassell, 1997; Linke et al., 2000).Dense anterograde labeling was also present in area TE2, but nolabeling was observed in the primary and secondary visual corticesV1 and V2.

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Figure 6. Digital photomicrographs showing the distribution of labeled axon fibers and terminals in representative coronal sections through rostral levels of the perirhinal cortex (B) and midcaudal levels (C, D) of the amygdaloid complex after a BDA injection into the mediocaudal part of LP (A). See Table 2 for abbreviations.

The other animal (case 3) had an injection also in the LPMC (Fig. 7A) but relatively rostral. In contrast to the most caudalinjections, this injection produced heavy anterograde labelingin the caudal part of lateral association visual cortex and areaTE2 (Fig. 7C,D). The cortical labeling was primarily distributedin the middle lamina and superficial portions of the molecularlayer. The dorsal PR (Fig. 7B-D) and the L exhibited light tomoderate density of labeling, with a similar pattern as that ofthe last animal.

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Figure 7. Digital bright-field photomicrograph showing a BDA injection site in the rostral part of LPMC (A) and dark-field photomicrographs showing distribution of labeled axon fibers and terminals in three representative levels of the temporal cortex. See Table 2 for abbreviations.

Thus, consistent with previous retrograde data, the present anterograde tracing data clearly show that the LP provides directprojections to the amygdala. This subcortical visual pathway exclusivelytargets the L. The results also show that the LP provides heavythalamo-cortical projections to area TE2 and dorsal PR, both ofwhich give rise to direct projections to the amygdala, specifically,the lateral amygdaloidnucleus.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present studies investigated visual CS pathways to the amygdala during the expression of conditioned fear. The lesionexperiments demonstrated that bilateral electrolytic lesions ofboth LGD and LP of the thalamus applied after training completelyblocked the expression of fear-potentiated startle to a visualCS but not to an olfactory CS or to context cues. In contrast,bilateral lesions of either structure alone had no effect on theexpression of fear-potentiated startle. Furthermore, local infusionof NBQX into visual thalamus immediately before testing preventedexpression of conditioned fear to a visual CS. Discrete injectionsof the anterograde tracer BDA into the LP revealed direct thalamo-amygdalapathway and indirect thalamo-cortical connections via dorsal PRand caudal temporal cortex area TE2. Considered with previousstudies, the present results suggest that the LP transmits visualCS to the basolateral amygdala via both cortical (LP-TE2/PR-amygdala)and subcortical (LP-amygdala)pathways.

Direct and indirect visual thalamo-amygdala connectivity

As in other sensory modalities, there is parallel processing of information reaching the rat's visual cortex. One main (lemniscal)pathway is via the LGD to the V1 and then from V1 to the V2, whereasthe other (non-lemniscal) pathway is via the LP to the associationvisual cortex. In rodents, V1 and V2 provide no direct projectionsto the amygdala. However, area TE2, which receives afferents fromboth V1 and V2 (Miller and Vogt, 1984; Vaudano et al., 1991; Cooganand Burkhalter, 1993; McDonald, 1998), provides substantial innervationto the amygdala (Mascagni et al., 1993; Shi and Cassell, 1997).Besides connecting with V1 and V2, TE2 also has direct reciprocalconnections with the LP. Early anatomic studies found that infusionof retrograde tracers into an area lateral to caudal peristriatecortex retrogradely labeled a group of neurons in the caudal portionof LP (Coleman and Clerici, 1980; Mason and Gross, 1981; Scheel,1988; Vaudano et al., 1991). In the present study, injectionsof the anterograde tracer BDA into the caudal LP, the tecto-recipientzone that receives bilateral superior collicular projections (Masonand Gross, 1981; present study), led to heavy axon and terminallabeling in area TE2. Thus, visual information can be transmittedto the basolateral amygdala via either LP-TE2 or LGD/LP-V1/V2-TE2pathways.

The PR is generally considered as a multimodal cortex, in which different modalities of sensory information converge via cortico-corticalconnections, which provide major projections to the amygdala andhippocampus (Deacon et al., 1983; Mascagni et al., 1993; Romanskiand LeDoux, 1993b; Shi and Cassell, 1997, 1999). Recent anatomicstudies show that injections of retrograde tracers into ventraltemporal cortex, including the PR, consistently labeled a groupof cells in LP, in addition to labeling in auditory thalamus (Namuraet al., 1997; Doron and LeDoux, 1999). Here we demonstrated thatthe cortical projections of LP go specifically to the dorsal partof perirhinal cortex, but very sparse or no projections go toadjacent auditory cortex or the ventral bank of the rhinal sulcus.Consistent with retrograde tracing findings (Doron and LeDoux,1999), anterograde labeling was seen in the PR after injectionsinto medial and caudal LP but not in cases with injections intorostrolateral part of LP. The heaviest labeling was seen in caseswith injections into caudomedial LP, the area that also sendsefferents to the amygdala (see below). Therefore, by receivingvisual inputs from both visual thalamus (LP) and cortex (V2 andTE2), the PR is another potential visual transmission route toamygdala.

The present anatomic data also confirmed a previous conclusion from retrograde tract tracing studies that there might be adirect visual thalamo-amygdala pathway (LeDoux et al., 1990a;Shi and Davis, 1996; Doron and LeDoux, 1999; Linke et al., 1999).Injections of BDA into caudal and medial LP produced a moderatedensity of axon and terminal labeling in the L and amygdalostriataltransition zone, in addition to cortical labeling in TE2 and PR.Besides LP, the dorsal part of SG is the other extrageniculatetarget of tecto-thalamic pathways and also projects to the amygdala(Doron and LeDoux, 1999; Linke et al., 1999; Linke et al., 2000).As shown in Figure 5D, the dense labeling from superficial layersof superior colliculus in dorsal SG is inseparable with that inLP, indicating homogeneity of the two areas. Electrophysiologicalrecording studies have also found that neurons in SG and LP havesimilar properties. Both have large receptive fields and respondvery reliably to fast moving visual stimuli (Hicks et al., 1984;Hutchins and Updyke, 1989; Casanova and Molotchnikoff, 1990).Furthermore, the present data show that the dorsal SG providesprojections to the PR and the L, as does the adjacent LP. Thus,we suggest that this dorsal part of SG should be considered asa part of LP (SG subdivision of LP), in contrast to the rest ofSG, which is a part of auditorythalamus.

Together, the suprageniculate and mediocaudal subdivisions of LP provide a subcortical visual pathway to the basolateral amygdala,in parallel with cortical visual pathways arising from the areaTE2 and dorsalPR.

Cortical versus subcortical visual CS pathways in fear conditioning

Previous anatomic and behavior studies have suggested that a foot shock US and an auditory CS can be relayed to the basolateralamygdala via both subcortical and cortical pathways (see introductoryremarks). The present anatomic data indicate that this schemeof parallel subcortical and cortical pathways seems also to applyto visual input to the amygdala. Thus, visual information maybe relayed to the basolateral amygdala via either thalamo-amygdalaor thalamo-cortico-amygdala pathways (seeabove).

However, conclusions about the participation or nonparticipation of cortical versus subcortical routes may depend on how theexperiments are performed. We believe that a disruption of conditionedfear produced by post-training lesions of a sensory pathway(s)indicates that this pathway(s) is normally used to mediate conditionedfear responses. However, if this pathway is damaged (e.g., bypretraining lesions), then other pathways may take over (Marenet al., 1996, 1997; Maren, 1999). Thus, the use of pretraininglesions or post-training lesions followed by retraining may identifypathways that can mediate fear conditioning, even if these pathwaysare not normallyused.

In the present study, post-training lesions restricted to the LP, which gives rise to subcortical visual inputs to the amygdala,did not block the expression of fear conditioning using a visualCS. In addition, post-training lesions of LG, which projects toboth primary and secondary visual cortices, did not block fear-potentiatedstartle using a visual CS. Because LP also projects to visualassociation cortices, this thalamo-cortical route might be expectedto mediate fear conditioning using a visual CS. However, previousstudies showed that extensive post-training visual cortical lesionsalso failed to block fear conditioning using a visual CS (Rosenet al., 1992; Falls and Davis, 1994). Thus, these data suggestthat neither the direct subcortical thalamo-amygdala pathway fromLP nor the LG and/or the LP to V1/V2 pathways appear to be criticalin mediating fear conditioning using a visual CS in intactanimals.

However, both TE2 and PR receive visual inputs from LP (present study) and visual cortices and in turn project to the amygdala.Thus, PR, together with the dorsally adjacent area TE2, representan area of convergence of thalamo-cortical and cortico-corticalvisual inputs that may provide information of visual CS to theamygdala during classical fear conditioning. In fact, previousstudies have shown that post-training chemical lesions of thetemporal cortex, including PR and area TE2 and TE3, totally blockedthe expression of conditioned fear using a visual CS (Campeauand Davis, 1995a). Consistent with this, the present study showedthat combined lesions of both LG and LP, which would cutoff boththalamic and cortical routes to TE2 and PR, also totally blockedthe expression of conditioned fear using a visual CS. Local infusionof the glutamate antagonist NBQX had the same effect, suggestingthat the lesion effect did not result from damage to fibers ofpassage. Furthermore, the lesioned animals exhibited a deficitof fear-potentiated startle specifically to the visual CS butnot to an olfactory or context CS, indicating that this lesioneffect was not attributed to a general failure of memory retrievalor to a deficit on enhancement of startle but by interruptingsensory transmission of visual information to the amygdala. Basedon these and other results, we conclude that visual input carriedby projections from LG and LP via connections through TE2 andPR to the amygdala normally are used in conditioned fear usinga visualCS.

In parallel, the PR also receives potential auditory inputs from extraleminscal thalamic auditory areas (dorsal medial andmedial medial geniculate nuclei) (Namura et al., 1997; Doron andLeDoux, 1999) and from the dorsally located temporal neocorticalarea (TE3) (Deacon et al., 1983; Mascagni et al., 1993; Romanskiand LeDoux, 1993b; Shi and Cassell, 1997). Moreover, post-traininglesions of PR and TE3 also block the expression of conditionedfear using an auditory CS (Campeau and Davis, 1995b). Together,these data suggest that thalamo-cortical and cortico-corticalpathways to TE2/TE3 and/or PR are the primary visual and auditorytransmission routes to amygdala in emotional learning. However,at present, it cannot be determined whether both TE2/TE3 and PRor PR alone is criticallyinvolved.

The alternate interpretation of the present data are that subcortical and cortical pathways are equivalently involved in transmittinga simple light CS to the amygdala, as suggested by others (Romanskiand LeDoux, 1992b; Campeau and Davis, 1995b), and the blockadeof conditioned fear by post-training lesion of temporal cortex(i.e., TE2, TE3, and PR) was attributable to a failure of memoryretrieval. However, the later hypothesis is not supported by availabledata. First, the lack of an effect of pretraining lesions of thesame cortical area in previous studies is not consistent witha primary role of the PR in memory retrieval (Campeau and Davis,1995b), although admittedly other areas might subsume this functionafter damage to PR. Second, the post-training lesions of PR interruptconditioned fear only to visual and auditory CSs but not to contextualcues (Phillips and LeDoux, 1995), suggesting a specific involvementin sensory transmission rather than a general effect on learningandmemory.

Previous studies by Rosen et al. (1992) found that electrolytic lesions of so-called "rostral perirhinal cortex" (from ~1.8to 3.8 mm posterior to bregma) totally blocked fear-potentiatedstartle to a visual CS, suggesting that it was part of a visualCS pathway. However, recent anatomical studies found that thisportion of rhinal cortex has reciprocal connections with somatosensorycortex and thalamus rather than visual or auditory system andredefined it as a part of insular cortex, the so-called "parietalinsula" (Shi and Cassell, 1997, 1998a,b). Our behavioral studiesindicated that the parietal insular cortex appears to be partof a foot shock US pathway rather than a visual or auditory CSpathway (Shi and Davis, 1999). Consistent with this, the presenttracing data also show that the visual thalamus, specificallyLP, does not project to this part of insular cortex but to thedorsal PR caudal to it. Interestingly, post-training lesions ofparietal insular cortex [referred as the rostral perirhinal cortexby Rosen et al. (1992)] appear to disrupt fear conditioning notonly to a visual stimulus but to auditory (Campeau and Davis,1995b) and contextual (Corodimas and LeDoux, 1995) cues as well.So it has been suggested that this parietal insula may be involvedin some general learning process, such as memory storage or retrieval(Campeau and Davis, 1995b; Corodimas and LeDoux, 1995; Gewirtzand Davis, 2000).

The fact that unit conditioned responses to an auditory CS in the lateral nucleus of the amygdala occur with very short latenciesin normal, unlesioned rats (e.g., <15 msec) has been taken asevidence that the direct thalamo-amygdala connection must normallymediate conditioned fear (Quirk et al., 1995). Once again, itis difficult to reconcile this interpretation with the fact thatpost-training lesions of direct thalamo-amygdala pathways failto block the expression of conditioned fear. However, direct thalamo-PR-amygdalatransmission, bypassing the primary auditory cortex, might wellsupport these very short latency responses recorded in the amygdala,so that these unit data may be fully compatible with the lesiondata.

Although we believe that the subcortical visual and auditory pathways are not primary routes whereby CS information is transmittedto the amygdala during fear conditioning, it is clear they canbe recruited when the cortical CS pathways are not available duringtraining. Thus, pretraining lesions of cortical auditory and visualpathways did not prevent the development of conditioned fear toan auditory CS (DiCara et al., 1970; Romanski and LeDoux, 1992a,b;Campeau and Davis, 1995b), and animals could relearn conditionedfear using either an auditory or visual CS after cortical lesions(Campeau and Davis, 1995b). Both sets of data indicate that thesubcortical pathways are sufficient for transmitting CS informationto the amygdala after damage to the cortical pathways. On theother hand, combined lesions of cortical and subcortical auditorypathways, made before training, totally block fear conditioningto an auditory CS (Romanski and LeDoux, 1992b).

Overall, the present studies suggest that visual information necessary for the expression of conditioned fear can be transmittedto the amygdala via either lemniscal (i.e., LG $right-arrow$ V1/V2 $right-arrow$ TE2/PR)or non-lemniscal (i.e., LP $right-arrow$ V2, TE2/PR) thalamo-cortico-amygdalapathways or direct thalamo-amygdala (i.e., LP $right-arrow$ L) projectionsduring classic fear conditioning (Fig. 8). In normal, unlesionedanimals, the cortico-amygdala pathways may normally relay visualCS information to the amygdala. However, subcortical pathwaysmay be important when these cortical pathways are damaged.

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Figure 8. Schematic diagram summarizing thalamo-cortico-amygdala and thalamo-amygdala visual pathways involved in fear-potentiated startle. The pathway indicated by the dashed line may not be critical in normal visual fear conditioning paradigm. See Table 2 for abbreviations.

  FOOTNOTES

Received July 25, 2001; revised Sept. 14, 2001; accepted Sept. 25, 2001.

This work was supported by National Institute of Mental Health Grants MH-57250, MH-58922, MH-52384, MH 59906, and MH-47840,the Woodruff Foundation, and The Center for Behavioral Neuroscienceof the National Science Foundation under Agreement Number IBN-9876754.We are grateful to Dr. David Walker for reading and commentingon this manuscript and Dr. Gayla Paschall for her significantcontribution involving running the odor conditioning and testingexperiment.
Correspondence should be addressed to Dr. Changjun Shi, Department of Psychiatry and Behavioral Sciences, Emory UniversitySchool of Medicine, 1636 Pierce Drive, Suite 4000, Atlanta, GA30322. E-mail: cshi{at}emory.edu.

  REFERENCES

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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