Phasic Activation of Locus Ceruleus Neurons by the Central Nucleus of the Amygdala

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The Journal of Neuroscience, April 15, 2003, 23(8):3491

Phasic Activation of Locus Ceruleus Neurons by the Central Nucleus of the Amygdala
Sebastien Bouret¹, Adam Duvel², Selim Onat¹, and Susan J. Sara¹
¹ Neuromodulation and Memory Processes, Unité Mixte de Recherche 7102, Centre National de la Recherche Scientifique, Université Pierre & Marie Curie, 75005 Paris, France, and ² Department of Psychology, Beckman Institute for Advanced Science and Technology, University of Illinois, Urbana, Illinois 61801

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The role of the central nucleus of the amygdala (CeN) in modulating output of noradrenaline in the forebrain was evaluatedby recording extracellular, single-unit activity from the noradrenergicnucleus locus ceruleus (LC) during stimulation of the CeN. Shorthigh-frequency trains (200 Hz) delivered at 800 µA in the CeNevoked phasic responses in 90% of the neurons recorded in LC.Single pulses were also effective but less reliably. The responseswere complex, multiphasic with an initial latency of 10-20 msec.This early peak was diminished or, in some cases, completely blockedby local or intracerebroventricular application of the corticotrophinreleasing factor antagonist $alpha$ helical CRF (9-41). The later excitatorypeak and subsequent inhibition were not effected by the drug treatment.The results underline the reciprocal functional relationship betweenthe amygdaloid complex and the LC and suggest that the LC mightbe an important "effector" of CeN activation duringlearning.

Key words: amygdala central nucleus; locus ceruleus; noradrenaline; CRF; neuromodulation; electrophysiology

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The central nucleus of the amygdala (CeN) has a well established role in emotional learning (Applegate et al., 1982; Pascoeand Kapp, 1985). More recent evidence suggests that this nucleusplays an essential role in regulation of attention (for review,see Gallagher and Holland, 1994; Holland and Gallagher, 1999).Careful behavioral analyses after lesions led Gallagher and Holland(1994) to conclude that the CeN "regulates the processing of cueswhen predictive relationships between events are first noticedor altered." This precisely describes the cognitive context thatelicits a robust response of the whole population of cells inthe noradrenergic nucleus locus ceruleus(LC).

LC neurons are activated both tonically and phasically during a task requiring sustained attention, suggesting a role in vigilance(Aston-Jones et al., 1991). However, the most striking featureof the response patterns of these neurons is that they show phasicresponses to novel stimuli followed by rapid habituation and thenrenew responding whenever the associated reward contingenciesare modified, such as during reversal or extinction (Sara andSegal, 1991; Hervé-Minvielle and Sara, 1995; Vankov et al., 1995).Thus, the LC responds to the predictive value or meaning of thestimulus rather than to its physical properties (Sara et al.,1994). These LC response characteristics observed in the rat werelater confirmed in the behaving monkey (Aston-Jones et al., 1997).Thus, LC neurons respond "when predictive relationships betweenevents are first noticed or altered," in the words of Hollandand Gallagher describing the functional role of theCeN.

There is a small but potentially important afferent projection from CeN to LC (Wallace et al., 1989; Luppi et al., 1995).Fibers from CeN terminate in the rostrolateral periceruleus ondendrites identified immunohistochemically as noradrenergic (VanBockstaele et al., 1996b, 1998). Input from CeN to the LC couldbe important in regulating LC activity during behavior requiringhigh levels of attention and stimulus processing. LC might, then,participate in mediating the CeN role in attention, through itsubiquitous projections to the forebrain. The postsynaptic facilitoryeffects of norepinephrine (NE) on stimulus processing in all sensorymodalities are well documented (Manunta and Edeline, 1997; Waterhouseet al., 1998; Lecas, 2001; Bouret and Sara, 2002).

The role attributed by Gallagher and Holland to the CeN in attention processes, together with the recent anatomical descriptionof the projections of CeN to LC, encouraged us to examine thefunctional influence of CeN on LC by recording responses of LCneurons to electrical stimulation of the CeN. The role of corticotropin-releasingfactor (CRF) in mediating LC responses was evaluated, becauseit has been shown that a substantial portion of CeN terminalstargeting LC dendrites contain CRF (Van Bockstaele et al. 1996a,b)and CRF has an excitatory effect on LC neurons (Siggins et al.,1985).

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Animals. Electrophysiological recordings were taken from 41 male Sprague Dawley rats obtained from IFFA Credo (L'Arbresle,France). The rats, weighing 320-420 gm at the time of the recordingsession, were housed for at least 1 week before the experimentin a temperature-controlled vivarium on a 12 hr light/dark cycle.They were weighed and handled regularly and had access to foodand water ad libitum.

Surgery. Rats were anesthetized with urethane, 1.2 gm/kg, which was usually sufficient for the entire recording session, butit was supplemented if there was any sign of discomfort. The ratswere mounted in a stereotaxic apparatus with the head positionedso that bregma was 2 mm below lambda, making an angle of approximately $-$ 14° from the head level position. Burr holes were drilled overthe CeN and LC, the dura was removed, and electrodes were implantedunder electrophysiological control. A bipolar stimulating electrodeassembly consisted of two tungsten electrodes glued together (0.1-0.5M $Omega$ ) with 500 µm separating the tips. This was aimed at the CeN: $-$ 1.8 mm posterior to bregma, 3.8 mm lateral to the midline, and~7.6 mm ventral to the surface of the brain. The LC electrodewas lowered at $-$ 3.9 mm posterior to the lambda suture and 1.15mm lateral to the midline. LC neurons were usually found at 5.2-5.8ventral to the surface of the brain, just under the fourth ventricle.They were identified by their broad action potentials, slow firingrate (1.2 Hz), and distinctive excitatory-inhibitory responseto contralateral pawpinch.

Pharmacology. In five experiments, the effect of the CRF antagonist $alpha$ helical CRF (9-41) ( $alpha$ hCRF) (Sigma, St. Quentin Fallavier,France) was examined. In two experiments, $alpha$ hCRF was injected intothe ventricles (intracerebroventricular injection). A 26 gaugeguide cannula was implanted above the lateral ventricle contralateralto the recording site (~1 mm posterior to bregma and ~1.5 mm lateralto midline), 1 mm dorsal to the ventricle (3.4 mm below brainsurface), and cemented in place with dental cement. Injectionwas made through a 33 gauge cannula extending 1 mm ventrally fromthe edge of the guide to reach the ventricle. In three subsequentexperiments, a 33 gauge cannula was glued to the recording electrodeso that the edge of the cannula was ~200 µm anterolateral to thetip of the recording electrode. The cannula was attached to flexibletubing into which a 2 µl Hamilton microsyringe was inserted. Theelectrode-cannula assembly was lowered into the LC as describedabove.

Two hundred micrograms of $alpha$ hCRF was dissolved in 190 µl of distilled water and stored as 10 aliquots of 19 µl at $-$ 20°C. Justbefore the injection, the solution was completed with 1 µl ofhypertonic saline to make an isotonic solution at a concentrationof 1 µg/µl with a neutral pH. For intracerulear injections, 1µl of this solution was slowly infused into the LC. Three to 4µl were injected in intracerebroventricularexperiments.

Stimulating and recording. The electrophysiological signal was filtered (400-3000 Hz bandpass), amplified (10,000×) (amplifiermodel # P511; Grass Instruments, West Warwick, RI), and displayedon an oscilloscope and an audio monitor. Wave forms were discriminatedonline using the Cambridge Electronic Design (CED) (Cambridge,UK) CED1401 digital converter and Spike2 software (CED). Datawere stored on a personal computer for additional offline analysis.Stimulation was delivered through an isolation unit in singlepulses (200 µsec) or in trains of three pulses at 200 Hz. Stimulationintensities included 200, 500, and 800 µA. Each series consistedof 40-60stimulations.

Data analysis. Single units were isolated wherever possible, using the Spike2 software. If the spikes were not clearly separable,the file was treated as a multiunit recording. Poststimulus timehistograms (PSTHs) and raster displays were generated for neuronalactivity 500 msec before and 500 msec after the stimulation, using2 msec bins. The mean and SD of neuronal firing activity was calculatedfor the 500 msec prestimulation baseline. A firing rate increaseto 2 SDs above the mean of the base line, sustained over at leastfour bins, was considered an excitatory response. A decrease to2 SDs below the mean was considered an inhibitory response. Responselatencies were thus calculated for each unit or multiunitrecord.

To quantify baseline and evoked activity, the firing rate was calculated by summing the number of spikes per bin for two 50msec windows on each PSTH, from 60 to 10 msec before stimulusonset and from 20 to 70 msec after stimulus onset. The mean firingrate in Hertz during these two periods was obtained by multiplyingeach count by 20 and dividing it by the number of trials (40-60).

To quantify the effect of CRF antagonist injections, spike counts during a baseline and two response windows were computedfor successive trials, before and after injection. These windowswere 15 msec in duration, starting 15 msec after stimulus onsetfor the early response window and 30 msec after stimulus onsetfor the late response window. The 15 msec baseline window ended10 msec before stimulation. Spike counts obtained before and after $alpha$ hCRF injection were compared with two-way ANOVA or with a nonparametricmultiple comparison (Newman-Keuls analog test) when necessary(when spike counts were very low or not normally distributed).One factor was defined as CeN stimulation with two levels: baselineand response (either early or late). The other factor was $alpha$ hCRFinjection with two levels: before and after injection. A significantinteraction between these two factors or a significant effectof the response factor in only one condition (before or afterinjection) was used as statistical criteria to define an influenceof $alpha$ hCRF on the response to CeN stimulation. For each cell, meanspike count within the defined window, before and after injection,was calculated. The magnitude of early and late phases of theresponse after $alpha$ hCRF injection could then be expressed as a differencefrom the baseline and converted to Hertz. To compare the effectof $alpha$ hCRF on early and late phases of the response, an averagevalue (across trials) of spike count difference was obtained foreach cell for early and late response counts, respectively. Atwo-way ANOVA was applied to the population of recorded cells,with one factor being defined as response phase (two levels, earlyand late). The other factor was $alpha$ hCRF injection with two levels:before and afterinjection.

Histology. At the end of the stimulation session, the rats were injected with the noradrenergic $alpha$ 2 receptor agonist clonidine(40 µg/kg, i.p.) as a pharmacological control for the recordingelectrode placement. Clonidine binds to inhibitory autoreceptorsin the LC, and this systemically administered dose completelyinhibits firing of the noradrenergic neurons with a latency ofonset of ~10 min (Dyon-Laurent et al., 1994). Thirty minutes afterinjection of clonidine, electrolytic lesions were made in thestimulating and recording sites by passing constant current (9V) between the tips and the ground for 5 sec. Rats were perfusedintracardially with saline and then Formalin (10%). Brains wereremoved and stored in Formalin. Sixty micrometer sections werecut, stained with cresyl violet, and examined for lesions in theappropriatestructures.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Histology

Placement of the stimulating electrode in the CeN is shown in Figure 1A. Placement of the recording electrode in the LC wasdetermined by inspection of the histology as shown in Figure 1B,and the response to clonidine is illustrated in Figure 1C. Thirty-fiverats had recording electrodes in the LC, and all of the cellswere inhibited after clonidine injection. Of these, 27 also hadstimulating electrodes correctly positioned in the CeN. Four stimulatingelectrodes were situated in the internal capsule, just lateralto CeN, two in the basolateral nucleus of the amygdala (BLA),one in the striatum, and one in the ventral hippocampus.

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Figure 1. Histological and pharmacological control of electrode placement. A, Histological verification of the recording site in the CeN (arrow). The small lesion (arrowhead) in the CeN was made by passing DC current between the tips of the stimulating electrodes. Note the descending tract of the electrode through the internal capsule (ic) and the globus pallidus (GP). ST, Striatum. B, Histological verification of the recording site in LC. Note on the left the intact LC, the darkly stained nucleus just under the fourth ventricle (IV), as indicated by the arrow. On the contralateral side is the lesioned site of the LC (arrowhead) made by passing DC current between the tip of the recording electrode and the ground. The electrode tract can be seen above the lesion in the cerebellum. C, Example of a pharmacological verification of the recording from a noradrenergic neuron. Note the total inhibition of activity of the unit after systemic injection of clonidine (40 µg/kg) indicated by the arrow. All LC units and multiunit activity responded with total but transient inhibition after clonidine injection. The peak reflects the phasic activation of LC neurons during the injection.

Two recording electrodes were located anterior and medial to LC in the lateral dorsal tegmental nucleus (LDT), three wereanterior and dorsolateral to LC in the parabrachial nucleus, andone was in the cerebellum. None of the cells recorded from thesesites responded to clonidine. All six of these rats had accuratelyplaced stimulating electrodes in theCeN.

Responses of LC neurons to stimulation of CeN

Fifty-three single LC units and 13 multiunit recordings were taken from the 27 rats that had both stimulating electrodes inthe CeN and recording electrodes in the LC. Ninety percent (48of 53) of isolated single units showed a significant responseto the CeN stimulation; 44 of these were orthodromically driven.Responses were seen to single pulses at 500 and 800 µA in 20 of53 single units (38%), with a mean latency of 11.7 ± 0.7 msec,latency being determined as described in Materials and Methods.More reliable responses were elicited by the short train of threepulses delivered at 200 Hz at an intensity of 800 µA. Forty-eightsingle units responded to the train, with a latency of mean 20.3± 0.5 msec from the first pulse. Figure 2 shows an example oftwo single units recorded from the same electrode (Fig. 2A), oneresponse being clearly biphasic, with a latency of 17 msec (Fig.2B), and the other short lasting, monophasic, with a latency of20 msec (Fig. 2C).

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Figure 2. Responses to a train of 800 µA, of two single units in LC recorded simultaneously from the same electrode. A shows superimposed waveforms of the two units. The unit depicted in B shows biphasic response with the initial phase latency at 17 msec. In the unit depicted in C, the initial latency is 20 msec, and second phase is absent. Top, Raster display of trial-by-trial responses to the stimulation. Bottom, Cumulative PSTH with 2 msec bins.

All 13 multiunit recordings taken from LC showed an excitatory response to train, with a latency of 21.3 ± 0.4 msec. An exampleof a multiunit response is shown in Figure 3.

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Figure 3. Multiunit response LC to a train of 800 µA applied to CeN. Note the relatively low baseline activity, which suggests that only a few neurons are included in this recording. The response consists of a biphasic excitation followed, 200 msec after stimulus, by a long-lasting inhibition. This postexcitation inhibition is probably attributable to an $alpha$ 2 receptor-mediated autoinhibition.

Antidromic responses were seen in four neurons. Response latency ranged from 21 to 24 msec, with a response to every stimulationtrial and within cell response latencies being the same on everytrial.

One unit responded with a total inhibition lasting for nearly 300 msec; this was the only purely inhibitory response seenin the entire series, and it should be noted that a neighboringunit, recorded from the same electrode, was antidromically drivenby the stimulation. Thus, the inhibition seen in the other neuronwas probably attributable to release of NE by the antidromicallydriven cell, which responded to everystimulation.

Responses of LC neurons to stimulation outside of the CeN

Stimulation of the BLA produced excitatory responses in two LC multiunit recordings with latencies of 28 and 32msec.

In four experiments, the stimulating electrode was located in the internal capsule, and, in two of four multiunit records,there was a response in LC to the 800 µA train with a 28 mseclatency. There was no response to the stimulation of the striatum(n = 1) or the ventral hippocampus (n =1).

Responses to CeN stimulation in non-LC recordings

Verified placements in parabrachial nucleus in three rats (two single units and two multiunit) revealed reliable excitatoryresponses to CeN stimulation at 500 µA with a variable latency(range of 18-31msec).

Two multiunit recordings were taken from the LDT, both showing excitatory responses with 25 and 18 mseclatencies.

One recording electrode was located in the cerebellum, and there was no response to the CeNstimulation.

Effect of CRF antagonist on LC response to CeN stimulation

Intraventricular (n = 2) and intracerulear (n = 3) injections of $alpha$ hCRF were made. Eleven single units were recorded from thefive animals. The spontaneous firing rate of LC neurons was notaffected by either intracerebroventricular or local injection,(Fig. 4, Table 1), enabling a clear comparison of the phasicresponses to CeN stimulation before and after $alpha$ hCRF injection.

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Figure 4. Local injection does not alter the firing rate of LC neurons. The firing rate of a single unit is shown as a function of time. Neither local $alpha$ hCRF application (arrow) nor CeN stimulation (lines) modify the baseline activity of the cell.


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Table 1. LC unit firing rate (in Hertz) around CeN stimulation before and after $alpha$ hCRF injection

All cells showed a significant response to CeN stimulation (500 µA trains). There were no differences in effect of the CRFantagonist whether it was injected into the ventricle or intoLC. Figure 5 (left) shows a response of a cell having very littlespontaneous activity and a reliable phasic response to the stimulation.The response was significantly decreased after the intracerebroventricularadministration of the CRF antagonist (Fig. 5, right).

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Figure 5. Intracerebroventricular injection of CRF antagonist decreases LC response to CeN stimulation. PSTHs (2 msec bin) and rasters constructed around CeN stimulation (500 µA trains) for an LC unit with very little spontaneous activity. Before $alpha$ hCRF injection (left), the cell exhibits a clear response to CeN stimulation. After intracerebroventricular injection of $alpha$ hCRF (right), the response is greatly decreased (nonparametric Newman-Keuls analog test; p < 0.05).

When the whole response window (50 msec) was considered, the injection of $alpha$ hCRF had no significant effect on response magnitude(Table 1), because the treatment only affected the early phaseof the response. For four of the six units that had only presentedan early response, this response was completely blocked (Fig.6A). This early response was significantly decreased for the othertwo units. Five units showed a biphasic response that consistedof an early peak at ~18 msec and a later peak at ~30 msec fromstimulus onset; an example is seen in Figure 6B. For these cells,clearly only the early phase of the response was altered by $alpha$ hCRF,the late phase being unaffected.

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Figure 6. Effects of local injection of CRF antagonist on LC response to CeN stimulation. A, PSTHs and rasters constructed around CeN stimulation (Ce stim) (500 µA trains; horizontal bar) for an LC unit showing a monophasic response (top). This response is completely blocked by the CRF antagonist (bottom; nonparametric Newman-Keuls analog test; p < 0.05). B, Same representation for another single unit showing a biphasic response to CeN stimulation. Before $alpha$ hCRF injection (top), the cell exhibits a biphasic response with an early (shaded area) and a late phase. After the injection (bottom), the early response is greatly attenuated (30% of its preinjection value; nonparametric Newman-Keuls analog test; p < 0.05), whereas the late phase is spared.

This differential effect of $alpha$ hCRF on early and late phases of the response is clearly seen when the entire sample is takeninto consideration. Figure 7 depicts the mean early and late responses,before and after drug treatments. The drug × phase interactionwas significant (F_(20,1) = 6.4; p = 0.02), confirming that effectwas limited to the early phase of the response.

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Figure 7. Mean ± SEM early and late responses of 11 LC units to CeN stimulation before and after injection of $alpha$ hCRF. Only the early phase of the response was affected by the treatment. Triangles, Control; squares, $alpha$ hCRF. An ANOVA reveals a significant interaction between response phase and treatment factors (F_(20,1) = 6.4; p = 0.02).

For those cells (n = 7) that still responded to CeN stimulation after $alpha$ hCRF injection, a significant increase in latency wasobserved as a consequence of the effect on the early phase ofthe response (t₍₆₎ = $-$ 2.6; p = 0.04) (Table 1).

  Discussion

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Responses of LC units and multiunits to CeN stimulation were consistent and present in the large majority of recorded cells.Although the anatomical projections of CeN to LC have been welldescribed, with some neurochemical definition (Van Bockstaeleet al., 1996a,b), this is the first direct demonstration of afunctional influence of CeN on LC activity in vivo. The responseselicited were for the most part excitatory, with little variabilityin initial latency, but most responses were complex, with biphasicexcitation (Fig. 2) or excitation followed by inhibition (Fig.3).

Van Bockstaele et al. (1998) provided strong evidence that a substantial portion of the CeN terminals in the periceruleusregion make asymmetric, excitatory synaptic specializations ontarget cells staining positively for tyrosine hydroxylase. Thereare abundant synapses on unidentified cells and dendritic processesas well. This region contains a large population of GABAergicneurons that locally regulate LC activity, thus providing an additionalmediating mechanism for CeN influence on LC. A substantial numberof CeN axon terminals located in the periceruleus region are CRFimmunoreactive (Van Bockstaele et al., 1998). Previous studiesshowed a marked decrease in CRF in LC region after lesions ofthe CeN, suggesting that this nucleus is a major source of CRFin LC (Koegler-Muly et al., 1993). Moreover, recent studies usinga combination of cellular and molecular techniques clearly confirmthe existence of CRF receptors in LC neurons (Fox et al., 2002).Electrophysiological studies, in vivo and in vitro, have indicatedthat CRF has an excitatory effect on LC neurons (Siggins et al.,1985; Curtis et al., 1995), so CRF should be a strong candidatefor mediating at least part of the LC response to CeN stimulation.The present results confirm this by showing that the short latencyearly part of the response is significantly attenuated or completelyblocked after local application of the CRF antagonist in the LC.The presence of vesicles in these terminals that were not CRFimmunoreactive suggests that other peptides and neurotransmittersare likely to be colocalized with CRF in CeN terminals (Van Bockstaeleet al., 1998). Indeed, immunohistochemical studies revealed largepopulations of neurotensin, enkephalin, somatostatin, substanceP, cholecystokinin, and vasoactive peptide containing neuronswithin the CeN (Cassell et al., 1986). The residual early responsesometimes seen after the CRF antagonist could be mediated by anyof these. The late part of the response, spared by the injection,is most likelypolysynaptic.

The majority of extrinsic projections from CeN are GABAergic (Swanson and Petrovich, 1998); their short-latency inhibitoryinfluence might delay expression of the excitatory response inLC. It should be noted that the stimulus artifact associated withthe train stimulation had a duration of 13 msec, so it could bemasking an early inhibitoryresponse.

Specificity of CeN stimulation

Stimulating electrodes located in BLA and the internal capsule evoked responses in LC. The BLA does not project to LC butdoes have a small direct projection to the CeN and another viathe lateral amygdala (LA) (Pitkanen et al., 1997). Thus, the polysynapticinfluence would account for the longer-latency response of LCcells to this stimulation. Responses in LC were also elicited,less reliably, from the internal capsule. Data from our laboratorysuggest that fibers originating in the FR2 region of frontal cortexand projecting to the region of the LC pass via the internal capsule.Electrical stimulation of the FR2 produces an excitatory responsein LC (Briois and Sara, 1997; Jodo et al., 1998) that is abolishedby cutting this fiber system (L. Briois and S. J. Sara, unpublishedobservations). It is important to note that stimulation of otherelectrode placements, near but outside of the CeN, namely in theventral hippocampus or the ventral striatum, did not evoke responsesinLC.

It is possible that there is current spread to other structures in the vicinity that could mediate the effect of the CeN stimulation.The most likely candidate is the bed nucleus of the stria terminalis(BNST), just adjacent to the CeN and a major output pathway fromthe amygdala. This nucleus does send a large projection to thepericeruleus region. Recent studies by Van Bockstaele et al. (1996a)have shown that, like CeN projections, BNST terminals synapseon both noradrenergic and non-noradrenergic dendrites in the region.The major difference is that the BNST synapses are mostly symmetrical,i.e., of the inhibitory type. Thus, current spread to the BNSTcould be contributing to the response in LC, but it most likelydoes not account for the consistent excitatory responses observed.In fact, current spread to the BNST might account for the puzzlingobservation that LC responses to short trains had significantlylonger latencies than responses to single pulses of the same intensity.According to the ultrastructural studies of Van Bockstaele, activationof the BNST, more likely during a train than during a brief pulse,would provide a competing inhibitory influence to LC, delayingthe appearance of the excitatoryresponse.

The relatively sparse number of antidromically driven responses was initially unexpected, because the CeN receives a substantialnoradrenergic input. A recent report has shown, however, thatthe majority of the noradrenergic fibers in the CeN originate,not in LC as originally suggested by Fallon et al. (1978), butin the medulla oblongata catecholamine cell groups (Asan, 1998).This corroborates a previous study using double labeling to showthat only ~5% of LC neurons were retrogradely labeled from theCeN (Petrov et al., 1993).

Parabrachial and LDT responses to CeN stimulation

Responses to CeN stimulation in the parabrachial nucleus and in the LDT are not surprising, because the CeN projects directlyto both of these regions (Hopkins and Holstege, 1978); the responseshad slightly longer latencies than those in LC, but there werenot enough data to evaluate the reliability of thisdifference.

Functional significance

There has been much discussion concerning the relative roles of the various nuclei of the amygdala in learning and memoryprocesses. There is a general consensus that the amygdala playsan important role in pavlovian fear conditioning and inhibitoryavoidance conditioning (Kapp et al., 1979; Pascoe and Kapp, 1985;Davis, 1994; McGaugh et al., 1996; LeDoux, 2000) and that theLA is involved in processing information concerning the conditionedstimulus (CS), whereas the CeN governs reactive responses (Amorapanthet al., 2000). There is, however, disagreement as to whether theamygdala is the site of plasticity underlying the associativefear learning or whether the role of the amygdala is to modulatememory formation in other brain regions (Fanselow and LeDoux,1999; Cahill et al., 1999; Vazdarjanova and McGaugh, 1999; Wilenskyet al., 2000). Consideration of the functional consequences ofthe CeN influence on LC might put the question in a new light.Activation of CeN during conditioning will cause an increase infiring of LC cells, which in turn will release NE in the BLA andLA, because there is a projection from LC to both of these regions(Fallon et al., 1978). As we know from the extensive work of McGaughet al. (1996), this increase in NE in the amygdala will enhancememory consolidation by interaction with hormones and neurotransmitters.The CeN excitation of LC will also release NE in forebrain regions.This should result in increased vigilance and attention (Berridgeand Foote, 1991) and enhanced sensory processing (Manunta andEdeline, 1997; Waterhouse et al., 1998; Lecas, 2001; Bouret andSara, 2002), thereby facilitatinglearning.

Several studies have shown that stimulation of the amygdala enhances synaptic transmission, plasticity, and long-term potentiationin the dentate gyrus (DG) of the hippocampus (Ikegaya et al.,1995, 1996; Akirav and Richter-Levin, 1999). The activation ofLC by stimulation of CeN directly or via BLA should result ina massive release of NE from LC terminals, found profusely inthe DG. There is a large literature showing noradrenergic-inducedenhancement of cellular excitability (Harley and Sara, 1992),synaptic transmission, (Sara and Bergis, 1991; Kitchigina et al.,1997), and synaptic plasticity (Neumann and Harley, 1983) in vivoin the rat DG. If activation of the amygdala occurs during learning,then its influence on LC should promote synaptic plasticity inthe hippocampus, thought to be necessary for memoryformation.

There are surprisingly few electrophysiological studies of the involvement of CeN in learning to lend support to the viewof CeN function put forth by Gallagher and Holland (see Introduction).The extensive work of Kapp et al. (1994) has, however, clearlyshown that this nucleus is activated by CSs in pavlovian aversiveconditioning (Kapp et al., 1994). It is evident that CeN activityduring learning can influence forebrain structures through severaldifferent pathways. Gallagher and Holland (1994) have, indeed,provided evidence from lesion and pharmacological studies thatthe cholinergic system is involved in mediating the CeN role inattention. In those studies, however, the conditioned orientatingresponse, suppressed after CeN lesion, was spared by lesions ofthe cholinergic system (Holland and Gallagher, 1999), suggestingthe involvement of other outputs. Our electrophysiological studiesshowing that responses are evoked in LC cells under similar cognitiveconditions as for CeN (see Introduction) together with the presentresults showing the strong excitatory influence of CeN on LC makesa strong case for considering LC to be another effector of CeNactivity. The widespread LC projections on both sensory and limbicareas, particularly the BLA and the hippocampus, should facilitateneuronal processing across these areas, as well as the formationof a distributed memorytrace.

  FOOTNOTES

Received Oct. 21, 2002; revised Jan. 27, 2003; accepted Jan. 29, 2003.

This work was supported by Centre National de la Recherche Scientifique (CNRS) Unité Mixte de Recherche 7102. S.B. was supportedby a predoctoral grant from the French Ministère de l'EducationNationale, Recherche et Technologie. A bilateral grant from theCNRS-Beckman Institute to S.J.S and M. Gabriel supported A.D.We recognize the essential contribution of Y. Moricard in providingexcellent histology. Prof. E. Thomas and Dr. E. Yadin participatedin some of the preliminaryexperiments.

Correspondence should be addressed to Dr. Susan J. Sara, Neuromodulation and Memory Processes, Unité Mixte de Recherche 7102,Université Pierre & Marie Curie, 9 Quai St. Bernard, 75005 Paris,France. E-mail: sjsara{at}ccr.jussieu.fr.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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