Chronic Stress Induces Contrasting Patterns of Dendritic Remodeling in Hippocampal and Amygdaloid Neurons

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The Journal of Neuroscience, August 1, 2002, 22(15):6810-6818

Chronic Stress Induces Contrasting Patterns of Dendritic Remodeling in Hippocampal and Amygdaloid Neurons
Ajai Vyas^*, Rupshi Mitra^*, B. S. Shankaranarayana Rao, and Sumantra Chattarji
National Centre for Biological Sciences, Tata Institute of Fundamental Research, Bangalore 560065, India

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The hippocampus and the amygdala are essential components of the neural circuitry mediating stress responses. The hippocampus,which provides negative feedback regulation of the stress response,is particularly vulnerable to degenerative changes caused by chronicstress. Unlike the hippocampus, relatively little is known abouthow stress affects the amygdala and the nature of its role inthe stress response. Hence, we examined the effects of two differentmodels of chronic stress on hippocampal and amygdaloid neuronalmorphology in rats. In agreement with previous reports, chronicimmobilization stress (CIS) induced dendritic atrophy and debranchingin CA3 pyramidal neurons of the hippocampus. In striking contrast,pyramidal and stellate neurons in the basolateral complex of theamygdala exhibited enhanced dendritic arborization in responseto the same CIS. Chronic unpredictable stress (CUS), however,had little effect on CA3 pyramidal neurons and induced atrophyonly in BLA bipolar neurons. These results indicate that chronicstress can cause contrasting patterns of dendritic remodelingin neurons of the amygdala and hippocampus. Moreover, CIS, butnot CUS, reduced open-arm activity in the elevated plus-maze.These findings raise the possibility that certain forms of chronicstress, by affecting specific neuronal elements in the amygdala,may lead to behavioral manifestations of enhanced emotionality.Thus, stress-induced structural plasticity in amygdala neuronsmay provide a candidate cellular substrate for affective disorderstriggered by chronicstress.

Key words: stress; anxiety; immobilization; rat; hippocampus; CA3; basolateral amygdala; atrophy; hypertrophy; dendritic remodeling

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A growing body of evidence has demonstrated that chronic stress can cause hippocampal damage (Uno et al., 1989; McEwen, 1999).Pioneering studies on how stress and stress hormones affect therat hippocampus revealed that repeated restraint stress producessignificant dendritic remodeling in CA3 pyramidal neurons (Watanabeet al., 1992; Magarinos et al., 1996; Sousa et al., 2000). Thisdendritic remodeling is characterized by a reversible shorteningand debranching of apical dendrites (Conrad et al., 1996) andis mediated by mechanisms involving high levels of glucocorticoidsecretion and activation of excitatory amino acid release (Magarinosand McEwen, 1995b). These findings have contributed to rodentmodels of stress-induced neuronal atrophy that may provide onepotential explanation for the hippocampal shrinkage associatedwith post-traumatic stress disorder, recurrent depressive illness,and Cushing's syndrome (Starkman et al., 1992, 1999; Bremner etal., 1995, 1997; Sheline et al., 1996; Lupien et al., 1998).

Over the past decade many studies on stress have focused primarily on the hippocampus, not only because of its susceptibilityto stress-related damage but also because of its negative feedbackregulation of the stress response via the hypothalamic-pituitary-adrenal(HPA) axis (Herman et al., 1989; Jacobson and Sapolsky, 1991;Sapolsky et al., 1991; Herman and Cullinan, 1997). Although thehippocampus is one of the most intensely studied structures inthe stress-inhibitory circuit, other limbic inputs, which areinvolved in regulating the HPA axis through excitatory inputs,have received less attention. In particular, there is increasingevidence supporting a critical role for the amygdala in fear,anxiety, and activation of the HPA axis (Allen and Allen, 1974;Davis, 1992; Davis et al., 1994; LeDoux, 1994). Anatomical studiesindicate that limbic inputs impinging on the paraventricular nucleus(PVN) of the hypothalamus and hypothalamic GABAergic neurons canbe either excitatory from the hippocampus, and thereby enhancingGABAergic tone, or inhibitory from the amygdala, and thereby reducingGABAergic tone (Herman et al., 1989; Jacobson and Sapolsky, 1991;Sapolsky et al., 1991; Pitkanen and Amaral, 1994; Herman and Cullinan,1997). This in turn implies that although enhanced hippocampalinput would suppress the HPA axis, enhanced amygdaloid input couldhave the opposite effect on HPAactivity.

As outlined above, one potential difference between the hippocampus and amygdala with respect to the neural circuitry underlyingstress comes from their disparate roles in the regulation of theHPA axis. Evidence for another difference comes from behavioralstudies demonstrating how stress affects hippocampal- or amygdala-dependentlearning and memory. In rodents, stress facilitates aversive learningbut impairs spatial learning (Shors et al., 1992; Luine et al.,1994). Although repeated stress that produces dendritic remodelingin the CA3 region impairs hippocampal-dependent learning (Conradet al., 1996), the basolateral amygdala has been shown to be essentialfor stress-induced facilitation of aversive learning (Liang etal., 1994; Shors and Mathew, 1998).

In view of the potentially contrasting impact of chronic stress on the hippocampus and amygdala at the behavioral level, andthe different roles played by these two structures in the neuralcircuitry of stress, it is important to examine the effects ofchronic stress at the level of single neurons. Therefore, we haveinvestigated the effects of two models of chronic stress on themorphology of hippocampal and amygdaloid neurons inrats.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experimental animals. Male Wistar rats were used for chronic unpredictable stress (CUS) and chronic immobilization stress(CIS) protocols. At the beginning of the experiments, CUS animalsweighed 200-250 gm (2-2.5 months old) and CIS animals weighed300-350 gm (3-3.5 months old). All animals (National Centre forBiological Sciences, Bangalore, India) were housed in groups ofthree with ad libitum access to food and water, unless specifiedotherwise in stress protocols. Control animals, which were littermatesof the stress-treated animals, were housed in separate cages.Animals were maintained in a temperature-controlled room, witha light/dark cycle of 12 hr (lights on at 7:00 A.M.). All proceduresrelated to maintenance and experimentation were in accordancewith National Institutes of Health guidelines and approved bythe Institutional Animal EthicsCommittee.

Experimental treatment groups. Rats, randomly assigned to experimental groups, were subjected to either CIS or CUS for 10consecutive days. CIS consisted of complete immobilization (2hr/d, 10 A.M.-noon) in rodent immobilization bags without accessto either food or water (Nibuya et al., 1999). CUS involved exposingrats to several types of stressors, which varied from day to day,for a period of 10 d (Ortiz et al., 1996). Thus, for the CUS paradigm,rats were subjected each day to two stressors that were randomlychosen from eight different stressors. The eight stressors wereforced swim for 3-4 min, lights on overnight, lights off for 3hr during the light period of the light/dark cycle, cold stress,social isolation overnight, food and water deprivation overnight,cage movement for 1 hr, and immobilization for 1 hr. Control animalswere not subjected to any type of stress. The following additionalparameters were measured to monitor the overall effects of thestress paradigms: percentage gain in body weight (net change inweight after experiment × 100/weight at the beginning of experiment),relative adrenal weight (wet weight of adrenal glands in mg ×100/body weight in grams), and presence of ulcers on gastricmucosa.

Morphological data analysis. After completion of stress protocols, all groups of rats were killed under deep anesthesia. Thebrain was removed quickly, and blocks of tissue containing thehippocampus and amygdala were dissected and processed for rapidGolgi staining technique as described earlier (ShankaranarayanaRao et al., 2001). One hemisphere from each brain was used forpreparing transverse sections from the dorsal hippocampus, andthe other hemisphere was prepared for obtaining coronal sectionsfrom the amygdala. For both the hippocampus and amygdala, 120-µm-thicksections were obtained using a rotary microtome (Jung RM 2055,Leica). Sections were collected serially, dehydrated in absolutealcohol, cleared in xylene, and coverslipped. Slides were codedbefore quantitative analysis, and the code was broken only afterthe analysis was completed. To be selected for analysis, Golgi-impregnatedneurons had to satisfy the following criteria: (1) presence ofuntruncated dendrites, (2) consistent and dark impregnation alongthe entire extent of all of the dendrites, and (3) relative isolationfrom neighboring impregnated neurons to avoid interfering withanalysis.

For morphological quantification of hippocampal neurons, 10 pyramidal neurons (five long-shaft and five short-shaft) fromeach animal were analyzed from area CA3 of the dorsal hippocampus(Fitch et al., 1989). Three major classes of neurons (pyramidal,stellate, and bipolar/bitufted) from the basolateral complex ofthe amygdala (BLA) were selected for analysis on the basis ofmorphological criteria described in the literature (McDonald,1982; McDonald, 1992). Our analysis of BLA neurons was restrictedto those located between bregma $-$ 2.0 mm and $-$ 3.2 mm, and thesewere observed to be evenly distributed across theBLA.

Camera lucida tracings (500×) were obtained (Leitz Orthoplan) from selected neurons and then scanned (eight-bit grayscaleTIFF images with 1200 dpi resolution; HP Scan Jet 6200C) alongwith a calibrated scale for subsequent computerized image analysis.Custom-designed macros embedded in Object Image software (ftp://simon.bio.uva.nl/pub/,an extended version of NIH Image) were used for morphometric analysisof digitized images. Using the center of the soma as referencepoint, dendritic length and branch points were measured as a functionof radial distance from the soma by adding up all values in eachsuccessive concentric segment (Sholl's analysis; segment diameter:50 µm for CA3 pyramidal neurons, 20 µm for BLA neurons) (ShankaranarayanaRao et al., 2001).

Elevated plus-maze. The elevated plus-maze, consisting of two opposite open arms (60 × 15 cm, surrounded by 1-cm-high transparentwall) and two enclosed arms (60 × 15 cm, surrounded by a 15-cm-highopaque wall), was elevated 75 cm from ground. Individual trialslasted for 5 min each and were recorded with a video camera foroff-line analysis. At the beginning of each trial, animals wereplaced at the center of the maze, facing an enclosed arm. Alltrials were conducted between 10 A.M. and 2 P.M., and the mazewas cleaned with 5% ethanol solution (v/v) after eachtrial.

Statistical analysis. Statistical significance for the effects of CUS and CIS on dendritic branch points and dendritic lengthof CA3 pyramidal neurons were analyzed by one-way ANOVA. Becausevalues for dendritic branch points and dendritic length of BLAneurons did not conform to a normal distribution, a more rigorousand stringent nonparametric statistical analysis involving a distribution-freerandomized Mann-Whitney test (Potvin and Roff, 1993) was appliedto evaluate levels of significance of morphological changes intheamygdala.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effects of chronic immobilization stress on dendritic morphology of hippocampal CA3 pyramidal neurons

CIS caused a significant decrease in the dendritic length (p < 0.01) and the number of branch points (p < 0.01) in hippocampalCA3 pyramidal neurons as compared with neurons in control animals(Table 1). Both long-shaft and short-shaft CA3 pyramidal cellsshowed significant dendritic atrophy after CIS. Moreover, thedecrease in total dendritic length and number of branch pointswas evident in both apical as well as basal dendrites of CA3 pyramidalcells. The atrophy of basal dendrites, however, was not as pronouncedas that observed in apical dendrites (Table 1). Representativecamera lucida drawings of control and CIS long-shaft CA3 neuronsare depicted in Figure 1B.


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Table 1. Effects of CIS and CUS on total dendritic length (µm) and number of branch points in hippocampal CA3 neurons

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Figure 1. CIS is more effective compared with CUS in causing dendritic atrophy in hippocampal long-shaft CA3 pyramidal neurons. A, Effects of CIS on mean dendritic length (top) and number of branch points (bottom) for each successive 50 µm segment as a function of the radial distance of the corresponding segment from the soma (control cells, n = 50; CIS cells, n = 45). Changes in apical (left) and basal (right) dendrites are shown separately. B, Camera lucida drawings of representative Golgi-impregnated hippocampal CA3 pyramidal neurons from control and CIS-treated animals. Scale bar, 50 µm. C, Effects of CUS on mean dendritic length (top) and number of branch points (bottom) for each successive 50 µm segment as a function of the radial distance of the corresponding segment from the soma (control cells, n = 45; CUS cells, n = 50). Changes in apical (left) and basal (right) dendrites are shown separately. *p < 0.05, **p < 0.01; one-way ANOVA. Filled circle, black line: Control; open circle, gray line: CIS or CUS.

To investigate the effects of CIS in greater detail, a segmental analysis was performed to track the changes in dendriticlength and branch points as a function of radial distance fromthe cell soma (Fig. 1A). This analysis demonstrates that CIS inducedthe most pronounced reduction in both apical dendritic lengthand number of apical branch points of long-shaft CA3 neurons withina distance of 150-250 µm from the soma. Basal dendritic lengthwas reduced most significantly within the first 150 µm from thesoma, whereas the most significant decrease in number of basalbranch points (Fig. 1A, bottom right panel) occurred within 50µm of the soma. Short-shaft CA3 neurons exhibited a similar patternof atrophy after CIS (data notshown).

Effects of chronic unpredictable stress on dendritic morphology of CA3 pyramidal neurons

In contrast to CIS, CUS was not as effective in causing dendritic atrophy in CA3 pyramidal neurons (Table 1). We observedseveral points of difference between the effects induced by CISand CUS. First, the magnitudes of the reduction in total dendriticlength and the number of branch points in CUS-treated long-shaftCA3 neurons were considerably smaller compared with those elicitedby the CIS paradigm. For example, the average percentage changein total apical dendritic length ( $-$ 13% from control) (Table 1)and number of apical branch points ( $-$ 13% from control) (Table1) induced by CUS was less than half of their corresponding valuesafter CIS (total apical dendritic length: $-$ 29% from control; numberof apical branch points: $-$ 31% from control) (Table 1). Second,these changes did not have the same degree of statistical significancecompared with CIS-induced changes in the same variables. Third,only apical, but not basal, dendrites of long-shaft CA3 cellsshowed a significant (p < 0.05) reduction in both total dendriticlength and number of branch points. Finally, although short-shaftCA3 neurons exhibited atrophy in both apical and basal dendrites,the magnitudes of the reduction in total dendritic length andnumber of branch points were almost identical (Table 1). In contrast,CIS-induced atrophy in apical dendrites was relatively greatercompared with basal dendrites (Table 1).

The relatively smaller effects induced by CUS compared with CIS become clearly evident in the more detailed segmental analysispresented in Figure 1C. Unlike the significant CIS-induced atrophyobserved at radial distances of 150-250 µm, CUS failed to elicita comparable effect at any distance from thesoma.

Effects of chronic immobilization stress on dendritic morphology of amygdala neurons

Having established the overall efficacy of our chronic stress protocols in eliciting patterns of dendritic atrophy in hippocampalCA3 pyramidal neurons that are qualitatively similar to thosereported previously, we next analyzed morphological effects ofCIS on Golgi-impregnated amygdala neurons in the same animals.Changes in dendritic length and number of branch points in controland CIS-treated neurons in the BLA were analyzed using the samemethods applied to the hippocampalneurons.

Previous morphological studies have revealed that the cortex-like BLA contains two main cell-types: spiny pyramidal (or modifiedpyramidal) neurons and spine-sparse nonpyramidal neurons (McDonald,1982, 1992). Amygdaloid "pyramidal neurons" constitute a broad,continuous morphological spectrum, from neurons that are virtuallyidentical to cortical pyramidal neurons at one end to neuronsthat more closely resemble cortical spiny stellate cells at theother end of the spectrum. These studies also suggest that asin the cerebral cortex, it is possible to recognize bitufted/bipolarvarieties of nonpyramidal cells on the basis of dendritic arborizationpatterns. Our analysis, therefore, used this framework (McDonald,1982, 1992) to analyze morphological effects of the CIS paradigmon three classes of BLA neurons: pyramidal, stellate, and bitufted/bipolar.

The same CIS paradigm that caused dendritic atrophy in CA3 pyramidal neurons in the hippocampus induced the opposite effectin BLA pyramidal neurons (Table 2). We observed a significant(p < 0.05) increase in dendritic length of CIS-treated pyramidalneurons [median(inter-quartile range) = 1666(761) µm] comparedwith control pyramidal neurons [median(inter-quartile range) =1330(699) µm] (Fig. 2C). This increase (25% compared with control)in median dendritic length was investigated further using segmentalanalysis, and the results are presented in Figure 2A. Segmentalanalysis in incremental steps of 20 µm from the soma clearly showsthat dendritic length of CIS-treated BLA neurons underwent themost pronounced increase within a distance of 60-160 µm from thesoma (Fig. 2A). In this particular range of radial distance fromthe pyramidal cell soma, all dendritic length median values forthe CIS-treated neurons were above the 75th percentile value forcontrol neurons. The total number of branch points was also greaterin CIS-treated pyramidal neurons [median(inter-quartile range)= 15.0(3.2)] compared with control neurons [median(inter-quartilerange) = 13.5(4.2)] (Fig. 2C). Representative camera lucida drawingsof BLA pyramidal neurons for control and CIS animals are depictedin Figure 2B.


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Table 2. Effects of CIS and CUS on total dendritic length (µm) of BLA neurons

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Figure 2. CIS increases dendritic arborization in BLA pyramidal neurons. A, Median values (horizontal line within each vertical bar) of total dendritic length for each successive 20 µm segment as a function of the radial distance of the corresponding segment from the soma (control cells, n = 18; CIS cells, n = 22). Inter-quartile ranges are represented by the lower (25th percentile) and upper (75th percentile) bounds of each vertical bar. B, Camera lucida drawings of representative Golgi-impregnated BLA pyramidal neurons from control and CIS-treated animals. Scale bar, 50 µm. C, Plots of median values and inter-quartile ranges for total dendritic length (top) and total number of branch points (bottom) for control (n = 18) and CIS (n = 22) neurons. *p < 0.05, **p < 0.01; randomized Mann-Whitney test.

Similar to the morphological changes exhibited by pyramidal neurons after CIS, BLA stellate neurons (Fig. 3B) also showedan increase in both total dendritic length and total number ofbranch points (Table 2). Segmental analysis (Fig. 3A) revealsthat the most significant and pronounced increase in dendriticlength occurred within a distance of 60 µm from the soma. Furthermore,even in segments that did not exhibit a statistically significantdifference, the CIS-treated stellate neurons tended to have highermedian values relative to control neurons. In contrast to pyramidaland stellate neurons, bipolar/bitufted neurons were not affectedby CIS (Table 2). The overall efficacy of the CIS protocol ininducing dendritic remodeling was also analyzed by assessing itsimpact on the entire population for each of the three classesof BLA neurons. Cumulative frequency plots (see Fig. 5A) of theentire database obtained from all three classes of BLA neuronsclearly demonstrate that neurons with a wide range of dendriticlengths showed the same trends as their respective median values.This is particularly evident in BLA pyramidal neurons, where theincrease in total dendritic length was evenly distributed acrossneurons with a wide range of dendritic lengths and was comparableto the increase shown by the median value for the distribution.Thus, in contrast to the lack of effect in the bipolar/bituftedneurons, CIS-induced increase in dendritic length appears to beoccurring across the entire population of pyramidal neurons analyzedfor the present study.

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Figure 3. CIS increases dendritic arborization in BLA stellate neurons. A, Median values (horizontal line within each vertical bar) of total dendritic length for each successive 20 µm segment as a function of the radial distance of the corresponding segment from the soma (control cells, n = 43; CIS cells, n = 39). Inter-quartile ranges are represented by the lower (25th percentile) and upper (75th percentile) bounds of each vertical bar. B, Camera lucida drawings of representative Golgi-impregnated BLA stellate neurons from control and CIS-treated animals. Scale bar, 50 µm. C, Plots of median values and inter-quartile ranges for total dendritic length (top) and total number of branch points (bottom) for control (n = 43) and CIS (n = 39) neurons. *p < 0.05, **p < 0.01, ***p < 0.001; randomized Mann-Whitney test.

Effects of chronic unpredictable stress on dendritic morphology of amygdala neurons

The same three classes of BLA neurons that were studied in the CIS experiments were also analyzed after CUS. In contrast tothe CIS-induced effects, the morphological changes exhibited byBLA neurons following the CUS paradigm were quite different. First,the CUS paradigm only affected bipolar/bitufted neurons in theBLA (Table 2). Second, unlike the increase observed in dendriticparameters of pyramidal and stellate neurons after CIS, CUS causeda significant decrease (p < 0.05) in total dendritic length (Table2). Table 2 also shows a significant difference in median dendriticlength between control neurons of the CIS and CUS groups. Thismay be attributed to the age difference between animals used inthe two stressprotocols.

Segmental analysis of CUS-induced dendritic atrophy of bipolar/bitufted neurons (Fig. 4A) reveals that throughout the entireextent of the dendritic tree, the median values for the dendriticlength for any particular segment were always smaller than thecorresponding control values. The most significant reduction indendritic length was evident within a distance of 40 µm from thesoma, as well as at a distance of 140-180 µm from the soma (Fig.4A). The lack of any CUS-induced effects on BLA pyramidal andstellate neurons was borne out across the entire range of valuesfor total dendritic length (Fig. 5B).

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Figure 4. CUS causes dendritic atrophy in BLA bipolar/bitufted neurons. A, Median values (horizontal line within each vertical bar) of total dendritic length for each successive 20 µm segment as a function of the radial distance of the corresponding segment from the soma (control cells, n = 34; CUS cells, n = 39). Inter-quartile ranges are represented by the lower (25th percentile) and upper (75th percentile) bounds of each vertical bar. B, Camera lucida drawings of representative Golgi-impregnated BLA bipolar/bitufted neurons from control and CUS-treated animals. Scale bar, 50 µm. C, Plots of median values and inter-quartile ranges for total dendritic length (top) and total number of branch points (bottom) for control (n = 34) and CUS (n = 34) neurons. *p < 0.05, **p < 0.01, ***p < 0.001; randomized Mann-Whitney test.

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Figure 5. Cumulative frequency plots summarizing the data for total dendritic length illustrating the contrasting effects of CIS (A) and CUS (B) on all BLA neurons. Pyramidal, left column; stellate, middle column; bipolar/bitufted, right column. The 50% mark (dashed line) for the total n in each plot represents the median value for the total dendritic length for the corresponding neuronal class. For clarity, the median values are marked with a solid vertical line (control: black; CIS or CUS: gray) in only those cases where there is a statistically significant difference relative to control. CIS induces a significant increase (right arrow) in total dendritic lengths of pyramidal and stellate neurons, without significant effect on bipolar/bitufted neurons. CUS causes a significant decrease (left arrow) in total dendritic length of bipolar/bitufted neurons, without affecting pyramidal and stellate neurons. Filled circle and black line: Control; open circle and gray line: CIS or CUS.

Effects on body and adrenal weights

To compare the indices of dendritic remodeling with other measures of the effects of chronic stress, we monitored relativegain in body weight and relative adrenal weight. Percentage bodyweight gain was significantly (p < 0.001; Student's t test) reducedafter completion of the 10 d stress protocol for both CIS (CIS: $-$ 0.2 ± 1.2%, n = 34; control: 6.4 ± 1.2%, n = 36) and CUS (CUS:2.7 ± 2.0%, n = 32; control: 15.1 ± 1.3%, n = 25) animals. Interestingly,only CIS caused significant adrenal hypertrophy (relative adrenalweight, CIS: 15.9 ± 0.8, n = 34; control: 13.6 ± 0.7, n = 34;p < 0.05; Student's ttest).

Anxiety response after chronic immobilization and unpredictable stress

Previous studies suggest that repeated restraint stress can have powerful enhancing effects on emotionality (Conrad et al.,1999). Animals display distinct behavioral changes suggestiveof an anxiety response after exposure to stress. Therefore, thebehavioral response of CIS and CUS animals in an anxiogenic environmentwas investigated using the elevated plus-maze and compared withcontrol animals. CIS animals exhibited a significant (p < 0.05;Student's t test) reduction in both percentage open-arm entries(CIS: 24.9 ± 5.9%, n = 10; control: 40.9 ± 3.6%, n = 10) and percentagetime in open arms (CIS: 12.2 ± 4.6%, n = 10; control: 21.6 ± 3.3%,n = 10). Thus, the CIS animals made fewer entries and spent lesstime in the open arms of the maze than control animals, indicativeof an enhanced anxiety response. In contrast, no significant effectswere observed in CUS animals for percentage open-arm entries (39.2± 6.4%; n = 10) and percentage time in the open arms (25.5 ± 5.5%;n = 10). We conclude that CIS induced significantly greater anxietycompared with CUS and control animals (Vyas et al., 2001).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study explored two aspects of how chronic stress affects the hippocampus and amygdala. First, our goal in these experimentswas to see whether chronic stress induces morphological changesin the amygdala and how they compare with those observed in thehippocampus (Watanabe et al., 1992). Second, we tested whetherthese stress-induced morphological changes follow the same generalpattern across two very different regimens of chronic stress,CIS and CUS (Ortiz et al., 1996; Nibuya et al., 1999). Our findingsdemonstrated that chronic stress induces contrasting patternsof dendritic remodeling in hippocampal and amygdaloid neurons.CIS elicited significant dendritic atrophy in hippocampal CA3pyramidal neurons, but caused dendritic hypertrophy in BLA neurons.This CIS-induced enhancement in dendritic arborization was restrictedonly to BLA pyramidal and stellate neurons, which are presumablyexcitatory projection neurons (McDonald, 1982, 1992). Moreover,these patterns varied, depending on the type of chronic stressused. CUS, which only caused atrophy, was relatively less effectivein remodeling CA3 pyramidal neurons and specifically affectedBLA bipolar/bitufted neurons. Finally, CIS and CUS also differedin terms of their anxiogenic properties because CIS, but not CUS,reduced open-arm activity in the elevated plus-maze.

CIS is more effective than CUS in inducing dendritic atrophy in CA3 pyramidal neurons

Previous studies of the hippocampus as a target of stress and stress hormones have characterized essential features of structuralremodeling in CA3 pyramidal neurons. The earliest reports establisheda rat model that demonstrated that 21 d of chronic restraint stress(6 hr/d) or 21 d of corticosterone treatment caused apical dendritesof CA3 pyramidal neurons to decrease in length and branching (Watanabeet al., 1992; Magarinos and McEwen, 1995b). This pattern of apicaldendritic atrophy was also observed in the tree shrew after chronicpsychosocial stress (Magarinos et al., 1996). The present studydemonstrates that CIS for 10 d (2 hr/d) is capable of inducinga pattern of shortening and debranching of dendrites in hippocampalCA3 pyramidal neurons that is consistent with previous findings.Interestingly, although earlier studies have reported atrophyonly in apical dendrites, our results indicate that CIS causedsignificant atrophy in basal dendrites as well. Complete immobilization,considered to be more severe compared with restraint stress, maybe more effective in eliciting structural changes in both apicaland basal dendrites. However, the degree of shortening and debranchinginduced by CIS was generally more pronounced in apical dendritesrelative to basal dendrites (Table 1).

Our findings also suggest that CUS was less effective compared with CIS in its ability to elicit dendritic atrophy (Table1). Although repeated restraint stress has commonly been usedin past studies, there is a growing appreciation of the fact thatrepeated application of the same stressor can lead to habituationin the stress response (Melia et al., 1994). Therefore, stressprotocols, comprising a combination of different stressors, havebeen used to reduce such adaptive effects (Ortiz et al., 1996).Studies using repeated unpredictable stress have been shown toelicit behavioral and biochemical changes that have not been observedwith repeated predictable stress (Sapolsky et al., 1984), butthere is also evidence (Magarinos and McEwen, 1995a) indicatingthat repeated restraint stress and a chronic multiple stress paradigmproduced the same degree of apical dendritic atrophy in CA3 pyramidalneurons despite differences in terms of the degree and time courseof non-neural measures, e.g., habituation of the corticosteroneresponse to acute restraint stress, body weight gain, thymus atrophy,and adrenal gland hypertrophy. This suggests that mediators inaddition to adrenal steroids can influence the time course ofan array of stress indices in a complex manner. It may well bethat not all of the individual stressors used in our CUS paradigmwork in concert to trigger similar temporal variations in stressindices that can lead to a robust morphological phenotype. Inthe present study, although both CIS and CUS were comparable interms of reduced body weight gain, the CIS paradigm produced greateradrenal hypertrophy. This, in turn, is consistent with the greatermagnitude of dendritic atrophy induced byCIS.

CIS enhances dendritic arborization in BLA pyramidal and stellate neurons

Having established the efficacy of our CIS regimen in producing morphological effects that match previous reports on the hippocampus,the novel and interesting observations of the present study camefrom our analyses of stress-induced morphological changes in theamygdala. The observed dendritic growth in the BLA is particularlyinteresting for several reasons. First, although pyramidal neuronsappear to be one of the prime targets of the CIS-induced morphologicalchanges in both hippocampus and amygdala, the changes were inopposite directions (atrophy vs hypertrophy). Second, the enhanceddendritic arborization in the BLA was not manifested uniformlyacross all neuronal classes (Fig. 5) because bipolar/bituftedneurons remained unaffected by CIS. Third, only the bipolar/bituftedBLA neurons were affected by CUS, and that too in the oppositedirection compared with the CIS-induced hypertrophy. In otherwords, there are multiple levels of dissociation in our observationsleading us to conclude that the two regimens of chronic stresshave rather specific and contrasting effects within the hippocampaland amygdaloidcircuitry.

On the basis of morphological studies, the BLA, which is described as a cortex-like nucleus of the amygdala (Swanson and Petrovich,1998), has been shown to contain a large number of spiny excitatoryprojection neurons, which are "pyramidal-like" (McDonald, 1982,1992). According to recent studies characterizing the electrophysiologicalproperties of morphologically identified amygdala neurons, pyramidal-likeBLA neurons display some form of spike frequency adaptation oraccommodation (Washburn and Moises, 1992; Rainnie et al., 1993;Chapman and Chattarji, 2000). Interestingly, this accommodatingfiring pattern in BLA pyramidal-like neurons is also a salientfeature of the firing patterns observed in hippocampal and neocorticalpyramidal neurons (Connors and Gutnick, 1990).

Our findings raise a particularly interesting issue concerning the cellular mechanisms by which CIS produced contrasting effectsin CA3 and BLA pyramidal neurons that appear to be otherwise similarin terms of their action potential firing patterns and morphologicalproperties. There is evidence for the involvement of excitatoryamino acids and NMDA receptors, as well as serotonin, in hippocampaldendritic remodeling (Magarinos and McEwen, 1995b; Magarinos etal., 1999; McEwen, 1999). Serotonin has also been shown to modulateexcitatory transmission in the amygdala in a corticosterone-dependentmanner (Stutzmann et al., 1998). Moreover, glucocorticoids enhancecalcium currents in the hippocampus (Kerr et al., 1992; Joelsand Vreugdenhil, 1998). Hence, it is quite likely that increasedlevels of intracellular calcium can act on the dendritic cytoskeletonto trigger structural changes. Thus, the observed differencesin dendritic remodeling in BLA neurons may reflect a fundamentaldifference in the spatiotemporal dynamics of intracellular calciumafter stress-induced physiological changes. Indeed, recent electrophysiologicalstudies of amygdaloid long-term potentiation also point to somekey differences in mechanisms of synaptic plasticity in the hippocampusand amygdala (Weisskopf and LeDoux, 1999; Weisskopf et al., 1999;Chapman and Chattarji, 2000). These differences in synaptic physiologyand plasticity, in turn, can alter the cellular response to thesame stressful stimulus and lead to contrasting forms of structuralplasticity in the twoareas.

Functional implications

What may be the behavioral consequences of the observed stress-induced morphological changes in the hippocampus and amygdala?Although some studies have reported spatial memory deficits afterstress (Luine et al., 1994) or chronic corticosterone treatment(Bodnoff et al., 1995), other studies (Conrad et al., 1999) suggestthat stress might also impair memory through non-hippocampal mechanisms,such as enhanced emotionality. Furthermore, stress facilitatesclassical eye-blink conditioning (Shors et al., 1992), and thisfacilitation requires activation of NMDA receptors in the BLA(Shors and Mathew, 1998). Corticosterone injections have alsobeen shown to potentiate fear conditioning (Corodimas et al.,1994). A recent interesting study (Conrad et al., 1999), whichpostulated that chronic stress would enhance cued conditioningbut not context conditioning, showed that repeated restraint stressfacilitates fear conditioning to both context and tone independentlyof causing hippocampal CA3 dendritic atrophy. The particularlyrelevant finding of this study was that the atypical antidepressant,tianeptine, failed to prevent enhanced fear conditioning and reducedopen-field exploration after stress, although it did prevent neuronalatrophy in the hippocampus. This led the authors to conclude thatchronic stress may have a powerful effect on the amygdala, whichcould override any influence of the hippocampus. Interestingly,CIS, in our study, also caused a significant increase in anxiety-likebehavior in the elevated plus-maze. Recent studies have also ledto the idea that aversive information relayed from the BLA toa part of the extended amygdala, i.e., the bed nucleus of thestria terminalis, may be involved in anxiety-like behavior (Davisand Shi, 1999). Thus, stress hormones released as a result ofstress-induced amygdala activity can strengthen the excitatorydrive within the BLA and thereby influence subsequent informationprocessing by the amygdala and its downstream targets. This suggeststhat chronic stress could lead to an imbalance in HPA axis functionthrough a gradual loss of hippocampal inhibitory control as wellas a gain in excitatory control exerted by the amygdala. Therefore,our observations on stress-induced dendritic remodeling in theamygdala may provide a potential cellular substrate for exploringstress-induced disorders that are characterized by diminishedcognitive capabilities and abnormally high fearresponse.

  FOOTNOTES

Received Feb. 12, 2002; revised May 2, 2002; accepted May 15, 2002.

^* A.V. and R.M. contributed equally to thiswork.

This work was supported by research grants from the National Centre for Biological Sciences and Council of Scientific andIndustrialResearch.

Correspondence should be addressed to Dr. Sumantra Chattarji, National Centre for Biological Sciences, UAS-GKVK Campus, Bangalore560065, India. E-mail: shona{at}ncbs.res.in.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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