Neuronal Adaptations to Changes in the Social Dominance Status of Crayfish

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Volume 17, Number 2, Issue of January 15, 1997 pp. 697-708
Copyright ©1997 Society for Neuroscience

Neuronal Adaptations to Changes in the Social Dominance Status of Crayfish

Shih-Rung Yeh, Barbara E. Musolf, and Donald H. Edwards
Department of Biology, Georgia State University, Atlanta, Georgia 30302-4010

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

The effect of superfused serotonin (5-HT; 50 µM) on the synaptic responses of the lateral giant (LG) interneuron in crayfishwas found to depend on the social status of the animal. In sociallyisolated animals, 5-HT persistently increased the response ofLG to sensory nerve shock. After social isolates were paired ina small cage, they fought and determined their dominant and subordinatestatus. After 12 d of pairing, 5-HT reversibly inhibited the responseof LG in the social subordinate and reversibly increased the responseof LG in the social dominant crayfish. The effect of 5-HT changedapproximately linearly from response enhancement to inhibitionin the new subordinate over the 12 d of pairing. If, after 12d pairing, the subordinate was reisolated for 8 d, the responseenhancement was restored. If the subordinate, instead, was pairedwith another subordinate and became dominant in this new pair,the inhibitory effect of 5-HT changed to an enhancing effect overthe next 12 d of pairing. If, however, two dominant crayfish werepaired and one became subordinate, the enhancing effect of 5-HTpersisted in the new subordinate even after 38 d pairing. Thesedifferent effects of serotonin result from the action of two ormore molecular receptors for serotonin. A vertebrate 5-HT₁ agonisthad no effect on social isolates but reversibly inhibited theresponse of LG in both dominant and subordinate crayfish. Theinhibitory effects of the agonist developed approximately linearlyover the first 12 d of pairing. A vertebrate 5-HT₂ agonist persistentlyincreased the response of LG in isolate crayfish and reversiblyincreased the response of the cell in dominant and subordinatecrayfish. Finally, although neurons that might mediate these effectsof superfused 5-HT are unknown, one pair of 5-HT-immunoreactiveneurons appears to contact the LG axon and initial axon segmentin each abdominal ganglion in its projection caudally from thethorax.
Key words: serotonin; 5-HT receptors; agonistic behavior; escape; lateral giant interneuron; social dominance

INTRODUCTION

Behavioral differences associated with dominant and subordinate animals often appear during the first agonistic encounter,when one animal begins to win and the other to lose the firstfight. Subsequent fights are usually decided more quickly, untilfighting is avoided altogether by the retreat of the subordinatein the face of the dominant's advance. The transition betweenthe similar behavior of two strangers to the bipolar differencein the behavior of the new dominant and subordinate can occurvery quickly, within minutes or hours of their first encounter.These different behavioral states can persist for variable periodsof time, from a few minutes or hours to a lifetime.

The nervous system of an animal that participates in a plastic social hierarchy must be able to mediate rapid behavioral transitionsin either direction as well as to mediate indefinite periods ofbehavior appropriate to each social status. The neural mechanismsfor change and maintenance of social status are unknown, but neuromodulatorsubstances have been linked to both. Immediate changes in socialbehavior have been seen in some animals after injection with aneuromodulator. Flank marking, a sign of social dominance in hamsters,occurs within moments of the injection of arginine vasopressinin the superior chiasmastic nucleus of the hypothalamus of freelybehaving hamsters (Ferris et al., 1986; Albers and Rawls, 1989).Similarly, injected serotonin evokes a dominant posture and promotesaggression in crayfish and lobsters (Livingstone et al., 1980;Kravitz, 1988; Huber, 1995). Slower changes in social behaviorand the maintenance of social status have been correlated withchanged serum levels of androgens, serotonin, and serotonin metabolites.Elevated levels of serotonin or serotonin metabolites have beenfound to correlate with dominance in some primates (Steklis etal., 1986; Brammer et al., 1987; Raleigh et al., 1991; Shivelyet al., 1991) and with aggression in mice (Cases et al., 1995;Nelson et al., 1995). Reductions in serotonin metabolites havebeen correlated with dominance or aggression in fish, rodents,and other primates, and with violent aggression in humans (Yodyingyuardet al., 1985; Bronson and Winter, 1992; Coccaro, 1992; Linnoilaand Virkkunen, 1992; Winberg et al., 1992, 1993; Brunner et al.,1995).

These results indicate that one mechanism of neural modulation of social behavior controls the levels of neuromodulatory substancesavailable to interact with neuronal targets. Another possiblemechanism would control the receptors for neuromodulators in thetarget neurons. Here we present evidence that the modulatory effectof serotonin on a command neuron for escape in crayfish changesin response to new social experience and changes in social status.These slow but reversible modulatory changes appear to resultfrom changes in the population of serotonin receptors. The modulatoryand receptor changes appear to be part of a larger but reversibleprocess of neuronal and behavioral adaptation to persistent changesin social status (Krasne and Shamasian, 1996). A preliminary reportof some of this work has appeared previously (Yeh et al., 1996).

MATERIALS AND METHODS
Dominant and subordinate crayfish. Juvenile (1-3 cm) crayfish (Procambarus clarkii) were hatched and raised in the laboratory.The animals were isolated for >1 month after they became free-swimmingby placing them individually in 6-cm-diameter cylindrical plasticmesh cages within a larger aquarium. Socially dominant and subordinateanimals were created by pairing previously isolated crayfish withoutregard to sex for 12 d or longer. Pairs were placed in 6-cm-diametermesh cages in groups of 8 in a 20 gallon aquaria. Crayfish fightimmediately after pairing, and the fighting results in establishmentof a stable dominant/subordinate relationship. Dominant/subordinaterelationships are dependent on size and experience, rather thanon sex (Bovbjerg, 1953). The two animals are both active and moveabout the cage, frequently climbing over each other. The dominantanimal initiates most and wins all of the agonistic interactionsbetween the pair. During these interactions, the subordinate avoidscontact with the dominant, either by retreating when approachedor by staying as far away from the dominant as possible, oftenup on the wall of the container.

Experimental animals were chosen from among the population of crayfish that had been individually housed for 1 month or longeror from the pairs of animals that had been together for at least12 d. Each pair was observed for 10-15 min, the social dominantand social subordinate were identified, and one was selected forexperimentation, whereas the other was not used.

Dissection and experimental procedure. A crayfish of known social status (isolate, subordinate, or dominant) was chilled toimmobility, and the abdomen was removed, pinned out in a Petridish, and dissected dorsally to expose the ventral nerve cord.The nerve cord and isolated abdomen preparation was maintainedat room temperature in 10 ml of crayfish saline continuously replacedat ~1.2 ml/min (Van Harreveld, 1936). The axon of the lateralgiant (LG) interneuron was identified visually in the terminalconnective and penetrated proximally (Fig. 1). Four shocks [0.3msec, 90 sec interstimulus interval (ISI)] at each of four stimuluslevels between 3 and 7.5 V were applied to the ipsilateral thirdand fourth nerves of the terminal ganglion and evoked both sub-and superthreshold LG EPSPs. The stimulus series was presentedonce, and then the stimuli at the two lowest levels were repeated.The preparation was then superfused with serotonin (100 µM in7 preparations at the outset of these experiments, and 50 µM forthe remaining 93 preparations) or with a 5-HT agonist [ $alpha$ -methyl-5-HTor 1-(3-chlorophenyl)piperazine (mCPP) at 50 µM, 67 preparations],all at 1.2 ml/min. If perfect mixing had occurred, the continuousreplacement of the bath with 50 µM 5-HT would have brought thebath concentration to 95% of 50 µM in ~25 min. Stimuli at a constantsubthreshold voltage level were presented at 3 min ISI duringthe first 45 min of superfusion. The previous stimulus serieswas then repeated during continued superfusion. The effects onthe LG response produced by the two concentrations of serotoninwere indistinguishable. A saline wash followed; responses to afinal set of stimuli were recorded after 1 hr wash. Although theelectrophysiology was performed with knowledge of the animal'sdominance status, the effects of serotonin on the responses ofall three types of animals were unmistakable and immediately distinguishable:the responses of isolate and dominant animals were always increasedfrom control levels, whereas those of subordinates were alwaysdecreased.
Fig. 1. The tailflip circuit in crayfish, showing convergence of mechanosensory afferents and interneurons on the LG command neuronfor tailflip. Hairs and other mechansoreceptors on the abdominalsurface project primary afferents into the ventral nerve cordwhere they excite the LG directly ( $alpha$ ) and indirectly through mechanosensoryinterneurons ( $beta$ ). EPSPs were recorded in the initial axon segmentof the LG neuron.
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The same experiments were performed on a set of adult (8-12 cm) crayfish that were obtained commercially and maintained communallyuntil they were separated into pairs for at least 2 weeks. Theeffects of serotonin and serotonin agonists on the responses ofthe LG neurons in these adult dominant and subordinate animalswere no different from the responses of the dominant and subordinatejuveniles.

5-HT immunocytochemistry and Lucifer yellow (LuY) injection. Crayfish were anesthetized by cooling them gradually over 20min to 4°C. The complete ventral nerve cord was removed undercold saline and pinned out in a Petri dish lined with SYLGARD(Dow Corning, Midland, MI), and the cord was desheathed in onesegment to expose the LG axon. LG was penetrated with a micropipettefilled with LuY, which was injected iontophoretically with $-$ 2nA continuous current for 1 hr. The nerve cord was transferredto another dish, repinned, and fixed in 4% paraformaldehyde in0.1 M phosphate buffer (PB) for 6 hr at room temperature. Thetissue was then rinsed in 0.1 M PB containing 0.4% Triton X-100,0.2% bovine serum albumin (BSA), and 0.1% sodium azide over 6hr at 4°C on a shaker. Six solution changes occurred over thistime. Published immunocytochemical procedures to stain for serotoninin the crayfish CNS were then followed (Beltz and Kravitz, 1983;Real and Czternasty, 1990), using a secondary antibody conjugatedto Texas Red.

RESULTS

Effect of 5-HT on LG responses in isolate, subordinate, and dominant juvenile crayfish
The LG neurons form a tightly coupled network of interneurons that together evoke an upward-directed tailflip escape responsewhen any one of them fires a single action potential (Wiersma,1947). An LG neuron is present in each abdominal hemiganglionwhere it is excited by local mechanosensory afferents and segmentaland multisegmental interneurons (Fig. 1) (Krasne, 1969; Kennedyet al., 1971; Zucker, 1972a). Stimulation of sensory afferentsin nerves 3 and 4 of the terminal abdominal ganglion (A6) evokesa biphasic EPSP in the LG neuron. The first depolarizing wave( $alpha$ ) is produced by monosynaptic connections from primary afferents,whereas the second wave ( $beta$ ) results from disynaptic inputs frommechanosensory interneurons (MSIs). Similar responses are seenin juvenile (2 cm) and adult (>8 cm) crayfish (Edwards et al.,1994).

The responses of the LG neuron to nerve shock in social isolates increased after 45 min superfusion of the exposed ventralnerve cord in the isolated abdomen with 50 or 100 µM serotonin(Figs. 2, 3A). Amplitudes of both $alpha$ and $beta$ EPSPs became larger,and this enhancement persisted, and even increased, after washingthe preparation with saline for 1 hr. The increase in responseoccurred at all stimulus levels and caused previously subthresholdstimulus levels to become superthreshold (Figs. 2B, 4). The responseincrease was accompanied by a small, persistent depolarizationof LG, along with a small increase in the input resistance ofthe cell, measured at the initial axon segment (Figs. 1, 3B).
Fig. 2. Responses of isolate, subordinate, and dominant juvenile crayfish to sensory nerve shock before (Control) and during bathapplication of 50 µM 5-HT and after 1 hr saline wash (Wash 1 Hr;see Materials and Methods). Top, EPSPs and spikes evoked by thestimulus level indicated and recorded under the three conditions,with the $alpha$ and $beta$ EPSP components labeled. Bottom, $beta$ EPSP amplitudesevoked by a range of stimulus intensities delivered to the sameanimals as in the top. Each value is the average of at least fourresponses to one stimulus level; the bars indicating ±1 SEM areobscured by the symbols. The Isolate crayfish was tested overthe range of stimulus intensities after 1 hr and after 5 hr ofsaline wash; the other animals were tested only after 1 hr wash.The average percent change in the response for each animal isgiven in the top left of each panel. The value is the percentchange in response produced by 5-HT from the control response,averaged over all subthreshold stimulus levels tested.
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Fig. 3. Changes in EPSPs, resting membrane potential, and input resistance of LG produced by superfused 5-HT and after 1 hr salinewash. A, Mean ± SEM percent change of the $alpha$ (top) and $beta$ (bottom)LG EPSPs produced by 5-HT (at either 50 or 100 µM) and by 1 hrsaline wash in isolate (left), subordinate (middle), and dominant(right) juvenile crayfish. B, Mean ± SEM change in resting membranepotential (top) and the percent change in input resistance (bottom)produced by 5-HT in isolate (left), subordinate (middle), anddominant (right) crayfish. The number of animals in each experimentis given in parentheses; the same animals were used for $alpha$ and $beta$ measurements in A. Responses that are significantly differentthan zero are indicated with an asterisk. Those differences aresignificant at p < 0.05, as indicated by the fact that the differencebetween the absolute value of the response mean and the absolutevalue of the 95% confidence limit is greater than zero.
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Fig. 4. Effect of 5-HT, 5-HT₁ agonist, and 5-HT₂ agonist on the stimulus threshold of LG in isolate, dominant, and subordinate juvenilecrayfish. The percent change in stimulus threshold was measuredas the difference between the stimulus voltage necessary to fireLG in the presence of the agonist and the stimulus voltage requiredbefore the drug was applied. Mean ± SEM percent change are shown;responses that are significantly different than zero are indicatedwith an asterisk. Those differences are significant at p < 0.05,as indicated by the fact that the difference between the absolutevalue of the response mean and the absolute value of the 95% confidencelimit is greater than zero. The number of animals used is givenin parentheses.
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The responses of the LG neuron in social subordinates were reduced by serotonin superfusion (Figs. 2, 3). $alpha$ and $beta$ EPSPs werereduced at all stimulus levels and caused previously superthresholdstimulus levels to become subthreshold (Figs. 2, 4). The reductionin response was accompanied by a small decrease in resting membranepotential and a decrease in input resistance. Saline wash (1 hr)eliminated the response reduction that occurred in the presenceof 5-HT.

The responses of the LG in social dominants were increased by serotonin at all stimulus levels but, unlike in the isolates,the response increase was eliminated by saline wash (Figs. 2,3). The stimulus threshold of the LG neuron was reduced duringserotonin superfusion in these animals (Fig. 4). As in the isolates,the response increase in the dominants was accompanied by a smalldepolarization and an increase in input resistance. The depolarizationwas removed by saline wash.

Concentration dependence of superfused serotonin on the response of the LG neuron
The effect of superfused serotonin on the responses of the LG neuron was tested over a range of concentrations from 10¹⁰ to 10³ M in isolate and dominant juvenile crayfish (Fig. 5). A smallincrease in LG responsiveness (+10%) during the experiment wasrevealed by a second exposure to saline alone ( $-$ $infinity$ on the abscissain Fig. 5). The LG response of the isolate animal increased ina log/linear manner from between 10¹⁰ and 10⁹ M. This apparent concentration threshold for isolates was belowthe range of hemolymph concentrations of monoamines found in thelobster (Livingstone et al., 1981). The effect of serotonin onthe response of the LG in dominant crayfish remained at controllevels for concentrations below 10⁷ M, above which it also increased linearly with the log of theapplied 5-HT concentration. An analysis of covariance indicatedthat the the dominant and isolate regression curves were differentat the p = 0.012 level (F_(1,60) = 6.70).
Fig. 5. Concentration dependence of 5-HT effect on LG EPSPs in social isolate and dominant crayfish. Mean ± SEM percent changes inthe $beta$ EPSPs in dominant (filled circles) and isolate (open circles)crayfish were calculated from the difference between EPSPs recordedbefore (control) and after superfusion with either saline (0 M5-HT, $-$ $infinity$ on the abscissa) or a known concentration of 5-HT (from10¹⁰ to 10⁴ M). Solid and dashed lines are linear regressions of the $beta$ EPSPsfrom dominant and isolate crayfish, respectively, against thelog₁₀[5-HT] concentration from 10⁸ to 10⁴ M (dominant) and 10¹⁰ to 10⁴ M (isolate).
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Time course and reversibility of the change in the neuromodulatory effect of 5-HT after a change in social status
To determine how the effect of serotonin on the LG neuron's response changes after a change in social status, we repeatedthe experiments described above at intervals from 1 to 12 d afterthe agonistic interaction that determined the animal's new socialstatus. As in the isolates, serotonin increased the response ofthe LG in the new subordinates in the first few days after pairing.The enhancing effect of serotonin on both the $alpha$ and the $beta$ EPSPsdecreased in new subordinates over the first week after the animalswere paired, and it became increasingly inhibitory in the secondweek (Fig. 6).
Fig. 6. Change in the effect of 5-HT on LG EPSP amplitude in isolate, new subordinate, and new dominant crayfish with the durationof subordinate/dominant pairing, and in reisolated crayfish. Left,Percent change in $alpha$ EPSPs (top) and $beta$ EPSPs (bottom) from controllevels produced by bath application of 50 µM 5-HT in new subordinates.Change in EPSPs in isolates is shown on the left of each panel(Isolated); change in EPSPs in animals that have been paired for12 d or longer and then reisolated for 8 d is shown on the rightof each panel (Reisolated). Right, Similar plots of data fromnew dominant crayfish. Each triangle represents data from oneanimal.
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The excitatory effect of serotonin was restored in new subordinates that were reisolated. When animals were paired for 12d and the subordinates were then reisolated for 8 d, serotoninincreased the responses of the LG neuron in these reisolated animalsto the same degree as occurred in the isolates. This result indicatesthat the development of serotonergic inhibition in new subordinatesis reversible after reisolation of the animal.

The enhancing effect of serotonin on both $alpha$ and $beta$ LG responses in social isolates was maintained in new dominant crayfish,but became "washable" after 12 d of pairing. Development of the"washability" of the serotonin effect was not traced over the12 d period of pairing. The responses of dominant animals thatwere reisolated for 8 d after 12 d of pairing were also increasedby serotonin.

Casualty rates among paired animals depend on their social status
The reversal of serotonin's effect on the response of LG after reisolation of subordinate crayfish suggested that the modulatoryeffects of serotonin might change with subordinate-to-dominanttransitions and vice versa. To test this, we took subordinateanimals from existing pairs and paired them to form new dominant/subordinatepairs, and we took dominant animals from other existing pairsand formed new dominant/subordinate pairs. These animals sufferedhigher casualty rates than the pairs of former isolates, in whichonly 35% of the new subordinates were killed. New subordinatesin pairs of former subordinates experienced a casualty rate near50%, and new subordinates in pairs of former dominants suffereda 72% casualty rate. In those new pairs of either type in whichboth animals survived, the new dominant and subordinate crayfishdisplayed behavior patterns that were indistinguishable from thoseof dominants and subordinates created by pairing former isolates.

The modulatory effect of serotonin follows a change in social status from subordinate to dominant
After two former subordinates were paired and the new dominant had been identified, that animal was tested for the effectof serotonin on the response of the LG neuron. We found that theinhibitory effect of serotonin that is typical of subordinatesgradually changed to the enhancing effect typical of dominantsover a 2 week period (Fig. 7).
Fig. 7. Effect of 5-HT on $alpha$ (top) and $beta$ (bottom) LG EPSPs in new dominants produced by pairing subordinate crayfish (Dom from S-S)for periods of time between 2 and 15 d (filled inverted triangles).The change in EPSPs in the 12 d subordinates is replotted at left(0 d of pairing) from Figure 6. The effect of 5-HT on LG EPSPsin dominants derived from pairing isolate crayfish (Dom from I-I)is replotted from Figure 6 for comparison (open triangles). Thedotted and dashed lines are linear regressions of the filled invertedtriangles and open triangles, respectively.
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Effect of 5-HT depends on social history and on social status
When we tested new subordinates made from pairing dominant crayfish, we found that the effect of serotonin on the responseof the LG neuron depended on the social history of the animalas well as on its current social status. Instead of becoming inhibitoryafter 2 weeks of pairing, serotonin continued to increase theresponses of the LG neuron in the new (formerly dominant) subordinateseven after 38 d pairing (Fig. 8). Despite this "dominant-like"effect of serotonin on their LG responses, the social behaviorof these subordinates was similar to that of new subordinatesmade from isolate pairs: throughout the 38 d period, the subordinateavoided the dominant during interactions and retreated or tailflippedat its approach.
Fig. 8. Effect of 5-HT on $alpha$ (top) and $beta$ (bottom) LG EPSPs in new subordinates produced by pairing dominant crayfish (Sub from D-D)for periods of time between 2 and 38 d (filled inverted triangles).The change in EPSPs in the 12 d dominants is replotted at left(0 d of pairing) from Figure 6. The effect of 5-HT on LG EPSPsin subordinates derived from pairing isolate crayfish (Sub fromI-I) is replotted from Figure 6 for comparison (open triangles).The dotted and dashed lines are linear regressions of the filledinverted triangles and open triangles, respectively.
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Effects of vertebrate 5-HT₁ and 5-HT₂ agonists in animals of different social status
The different effects of serotonin on the LG neuron responses of animals of different social status suggested to us that changesin social status may cause changes in serotonin receptors or intheir transduction mechanisms. To test for different serotoninreceptors, we repeated the experiments described above with oneof two vertebrate serotonin agonists substituted for serotonin.When we substituted 50 µM mCPP Cl₂, a vertebrate 5-HT₁ agonist,for serotonin, we found that it had no effect on the responsesof the LG neuron in isolate animals but that it inhibited LG neuronresponses in both dominant and subordinates (Fig. 9). These effectsoccurred at all LG stimulus levels and were reversible with asaline wash.
Fig. 9. Effect of vertebrate 5-HT₁ agonist mCPP-Cl₂ on LG responses to sensory nerve shock in isolate, subordinate, and dominant juvenilecrayfish. The experiments and the figure are organized as in Figure2, with 50 µM 5-HT₁ agonist substituted for 5-HT.
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Like the effect of serotonin, the full inhibitory effect of the 5-HT₁ agonist developed over a 12 d period after the isolateswere paired (Fig. 10). As stated above, the 5-HT₁ agonist had noeffect on the responses of the LG neuron in isolates. In the newsubordinate crayfish, the 5-HT₁ agonist became inhibitory after4 d, and the inhibition became stronger over the next week. $alpha$ and $beta$ EPSPs were similarly affected. The inhibitory effect ofthe 5-HT₁ agonist developed in the new dominants in a similarmanner. Reisolation of the new dominants and subordinates removedthe inhibition so that the 5-HT₁ agonist once again had no effecton the response of the LG neuron.
Fig. 10. Change in the effect of the 5-HT₁ agonist mCPP-Cl₂ on the amplitudes of $alpha$ (top) and $beta$ (bottom) LG EPSPs in isolate crayfishand in newly paired subordinate (left) and dominant (right) crayfish.Responses of animals that were reisolated for 8 d after 12 d ofdominant or subordinate status are shown to the right of eachpanel. The experiments and the figure are organized as in Figure6, with 50 µM 5-HT₁ agonist substituted for 5-HT.
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Substitution of 50 µM $alpha$ -CH₃ 5-HT, a vertebrate 5-HT₂ agonist, for serotonin had completely different effects (Fig. 11). Insocially isolate crayfish, $alpha$ -CH₃ 5-HT increased the responsesof the LG neuron and continued to do so after 1 hr saline wash,much as serotonin had done (see Fig. 2). In both subordinate anddominant crayfish, the 5-HT₂ agonist also increased the responseof the LG neuron, but it did so reversibly: the increase was removedafter a 1 hr saline wash (Fig. 11). Response increases occurredat all stimulus levels.
Fig. 11. Effect of 5-HT₂ agonist $alpha$ -methyl-5-HT on LG responses to sensory nerve shock in isolate, subordinate, and dominant juvenilecrayfish. The experiments and the figure are organized as in Figure2, with 50 µM 5-HT₂ agonist substituted for 5-HT.
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The opposing effects of the vertebrate 5-HT₁ and 5-HT₂ agonists were seen in all of the animals examined (Fig. 12). The 5-HT₁agonist reduced the $beta$ EPSPs of the LG neuron by an average ofnearly 50% in dominant and subordinate animals, whereas the 5-HT₂agonist increased $beta$ EPSPs by an average of between 32 and 35%in isolate, dominant, and subordinate crayfish. The effects on $alpha$ EPSPs were similar but usually smaller.
Fig. 12. Effect of 5-HT₁ and 5-HT₂ agonists on LG neuron responses. A, Percent change in $alpha$ and $beta$ LG EPSPs in isolate, subordinate,and dominant crayfish before and during superfusion of 50 µM 5-HT₁agonist mCPP-Cl₂ and after saline wash for 1 hr. B, Percent changein $alpha$ and $beta$ LG EPSPs in isolate, subordinate, and dominant crayfishbefore and during superfusion of 50 µM 5-HT₂ agonist $alpha$ -CH₃ 5-HTand after saline wash for 1 hr. The number of animals used inboth sets of experiments is given in parentheses in the top frameof each panel.
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5-HT-like-immunoreactive terminals and the LG axon
Approximately 100 neurons in the crayfish CNS display 5-HT-like immunoreactivity (Real and Czternasty, 1990). Many of thesecrayfish neurons appear homologous to the 5-HT-immunoreactiveneurons in the CNS of lobster (Beltz and Kravitz, 1983). Stimulationof one of these lobster neurons (the large cells in the firstabdominal ganglion) has been shown to mimic the modulatory effectof superfused serotonin on command-activated abdominal posturalflexion (Ma et al., 1992). We wished to determine whether anyof these or other 5-HT-like-immunoreactive processes appear toinnervate the LG neuron.

In socially isolate juvenile crayfish, we first injected the axon of the LG neuron with LuY and then processed the entireCNS for 5-HT-like immunoreactivity, using a secondary antibodyconjugated with Texas Red (see Materials and Methods). We founda pattern of 5-HT-like immunostaining that was very similar tothat reported previously for crayfish (Real and Czternasty, 1990).We also found a pair of stained fibers, each of which projectedalong the lateral and dorsal margins of one side of the ventralnerve cord and gave rise to a set of terminal varicosities ineach abdominal ganglion that were in close proximity to ventralsurface of the LG axon (Fig. 13). In abdominal ganglia 1-5 (A1-A5),the terminal varicosities were adjacent to the distal end of theaxon of the next caudal LG (Fig. 13A), where it makes output connectionswith both the segmental giant interneuron and the fast flexormotor neurons, and where it makes a septate junction with theaxon of the ganglionic LG (Watanabe and Grundfest, 1961). A few5-HT varicosities appear on the anterior side of the septate junction,adjacent to the initial axon segment of the ganglionic LG (Fig.13A). Curiously, the LG dendrites appear to have no 5-HT-like-immunoreactivefibers or terminals near them (Fig. 13B). In the terminal abdominalganglion, A6, there are two LG neurons, a local LG (lLG) and aprojecting LG (pLG) (Kondoh and Hisada, 1983). Immunostained varicositiesare largely confined to the axon and proximal dendrite of thelocal LG neuron, although a few span the septate junction betweenthe lLG and the pLG and appear to make contact with the pLG atits initial axon segment (Fig. 13C). There are no immunostainedvaricosities or fibers near the distal dendrites of the lLG oranywhere on the dendrites of projecting LG, where it receivesinputs from primary afferents and interneurons (Fig. 13D). We havetraced the lateral/dorsal 5-HT-immunostained fiber rostrally throughthe thoracic ganglia, but we have not yet identified its cellbody.
Fig. 13. 5-HT-like-immunoreactive terminals and the LG neurons. A, The LG neuron in ganglion A5 stained with LuY (false red) and photographedwith a confocal attachment (Newport Instruments) laterally inthe focal plane of the LG axon, and 5-HT-like-immunoreactive axonalterminals labeled with Texas Red (false green) photographed inthe same focal plane as the LG image. The 5-HT-like terminalsare restricted to the vicinity of the initial axon segment ofthe ganglionic LG and to the anterior end of the axon of the nextcaudal LG (from A6). The septate junction between the two is indicated(S). Similar immunoreactivity is seen in all five anterior abdominalganglia. B, The same preparation as in A, photographed in thefocal plane of LG's major dendrites in A4. No 5-HT immunoreactivityabove background is seen in this plane. C, The local and projectingLG neurons in A6 (red), with the 5-HT-like-immunoreactive terminals(green) on the proximal segment of the both neurons. No labelappears near the dendrites of the projecting LG, which receiveinputs from mechanosensory interneurons and primary afferents(D). D, Diagram showing the relationship of the LG neurons tothe 5-HT neuron in A₅ and A₆.
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DISCUSSION

The effects of 5-HT vary with social status and social history
We have found that the effect of serotonin on a central synapse depends on the social status and the social history of theanimal. Like other neuromodulators in many animals, serotoninsets the gain of synapses and circuits in crayfish and, in thisway, appears to modify or select those circuits for a greateror lesser role in controlling the behavior of the animal (Kravitz,1988; Katz, 1995). In the present instance, the modulatory effectof serotonin is itself modulated by the social status and socialhistory of the crayfish, so that in dominant crayfish the LG responseis transiently increased, in subordinates it is transiently inhibited,and in isolates it is persistently increased.

Although crayfish adopt dominant or subordinate patterns of behavior immediately after their first fight, the changes in theeffect of serotonin take much longer to develop. The changes onlyfollow persistent changes in social status and develop more orless linearly over an ~2 week period after the change in socialstatus. The slow change in the effect of serotonin may reflectthe time it takes to turn the population of serotonin receptorsover, but it may also reflect the undesirability of changing thereceptor population merely because the animal had a bad day. Afterthe changes in the effects of serotonin are established, theycan be reversed if the change in social status is reversed ina persistent manner, such as when a subordinate animal becomesdominant. However, we also found that some changes in the modulatoryeffect of serotonin occur more easily than changes in the reversedirection: changes in the effect of serotonin that follow a subordinate-to-dominantsocial promotion follow much more quickly than changes that followa dominant-to-subordinate social demotion.

It is unclear what signals the abdominal nervous system to begin to change the effect of serotonin on the response of LG aftera change in social status. Presumably, social status is recognizedin the brain or anterior nervous system, and a persistent signalalerts LG and perhaps other parts of the nervous system to thenature of the change.

Changes in social status have also been found to influence cell size and the level of expression of gonadotropin-releasinghormone (GnRH) in a population of hypothalamic neurons in an Africancichlid fish. The cells are larger and the expression levels aregreater in territorial (dominant) males, and both are smallerin nonterritorial (subordinate) males (Francis et al., 1993; Whiteand Fernald, 1993). Like the modulatory effects of serotonin describedabove, the effects of social promotion (size increases) on theGnRH neurons occur more readily than the do the effects of socialdemotion (size decreases).

5-HT receptors
The changes in the effects of serotonin that we report in crayfish appear to result from changes in the effects of differentserotonin receptor subtypes that have opposing effects on theresponse of the LG neuron. The inhibition of the response of theLG neuron by a 5-HT₁ agonist appears to result from a crayfishserotonin receptor subtype that is distinct from the receptorsubtype that was preferentially excited by a 5-HT₂ agonist andfacilitated the responses of LG to its inputs. Each of these effectslasted only as long as the agonist was present. The persistentexcitatory effect of both serotonin and the 5-HT₂ agonist on theresponse of the LG neuron in isolated crayfish may result fromactivation of a third receptor subtype or from what might be amodified version of the second receptor subtype. At present, however,both the nature of the different 5-HT receptor subtypes and themechanisms of their effects, including their second messengers,are unknown.

The changes in the effects of serotonin with social pairing may reflect differential changes in the receptor subtypes or intheir downstream mechanisms. The lack of an inhibitory effectof 5-HT or the 5-HT₁ agonist in social isolate crayfish and thesubsequent appearance of the effect in new dominant and subordinatecrayfish suggest that the inhibitory receptor mechanism is absentor disabled in isolate crayfish and is increasingly activatedor restored in new dominant and subordinate animals. As this happens,the persistently excitatory effect of 5-HT in isolates may beeither replaced by or transformed into the transiently excitatory5-HT effect in the same new dominant and subordinate crayfish.Under this hypothesis, the transient excitatory effect of onereceptor becomes preeminent in new dominant crayfish, whereasthe inhibitory receptor becomes preeminent in new subordinateanimals. At present, these hypotheses await testing by detailedanalysis of the different 5-HT receptor subtypes, their secondmessengers, and their physiological mechanisms.

The crayfish serotonin receptors may differ from vertebrate serotonin receptors. The 5-HT₁ agonist that we used, mCPP Cl₂,has its greatest effects on vertebrate 5-HT_1B and 5-HT_1C receptors,but also has some agonistic effect on 5-HT_1A receptors (Julius,1991; Leonard, 1992; Humphrey and Hartig, 1993). It is unclearwhether the crayfish receptors that respond to this agonist, orthe receptors that respond to the vertebrate 5-HT₂ agonist, arehomologous to their counterparts in vertebrates. Recent work incrab has shown that crustacean serotonin receptors may be distinctfrom those of vertebrates (Zhang and Harris-War- rick, 1994) .

The reason for the difference in threshold concentration for the effects of serotonin in isolate and dominant animals (Fig.5) is also unknown. It may reflect either a difference in thesensitivity of serotonin receptors in the two types of animalsor the coactivation of excitatory and inhibitory effects in thedominant animal that would increase its threshold concentration.

Most of the serotonin receptors that affect the response of the LG neuron appear to act on the LG neuron itself, but somemay also be presynaptic to LG. Serotonin depolarized LG in isolate(Glanzman and Krasne, 1983) and dominant crayfish and hyperpolarizedit in subordinate crayfish. Serotonin had similar effects on $alpha$ and $beta$ EPSPs in LG but had no significant effect on the responsesof mechanosensory interneurons that contribute to the $beta$ EPSP,which suggests that serotonin acts directly on LG. The lack ofserotonergic neurons near LG dendrites (Fig. 13) is consistentwith this. However, serotonin can act neurohumorally in lobsters,and crayfish possess homologous serotonergic neurosecretory neuronsin the abdominal nervous system (Beltz and Kravitz, 1983; Realand Czternasty, 1990). Because serotonin has been well establishedas a presynaptic modulator in both Aplysia (Brunelli et al., 1976;Bernier et al., 1982; Klein, 1993; Zhu et al., 1995) and at thecrayfish neuromuscular junction (Dixon and Atwood, 1989), it ispossible that the humoral effects are mediated presynaptically.

Serotonin immunoreactivity and the LG neuron
The LG neurons appear to be contacted in each abdominal hemiganglion by a serotonergic neuron that projects caudally alongthe nerve cord from the thorax. The location of the serotonergicvaricosities on the LG axon is where LG makes connections to fastflexor (FF) motorneurons (Krasne, 1969; Kennedy et al., 1971;Zucker, 1972a,b; Roberts et al., 1982; Fraser and Heitler, 1989;Edwards et al., 1991; Heitler et al., 1991). Some of the axonalterminals of the serotonin fiber are just rostral to the septatejunction between LG axons, on the initial axon segment of theganglionic LG, where they could affect EPSPs and the thresholdfor spike initiation in the ganglionic LG neuron (Vu and Krasne,1993).

Serotonin, aggression, social status, and the escape circuit
Serotonergic systems have been implicated in the release of aggressive behavior in humans, mice, fish, and crayfish and lobsters(Winberg et al., 1991; Brunner et al., 1995; Cases et al., 1995;Huber, 1995; Huber and Kravitz, 1995). Injection of serotonininto freely behaving subordinate crayfish evokes a sudden increasein fighting behavior affecting both the duration and the intensityof fighting (Huber, 1995; Huber and Kravitz, 1995). These resultssuggest that the onset of aggression is accompanied by the releaseof endogenous serotonin. If this occurs, then the threshold forLG-mediated tailflip escape should go up in subordinate crayfishand down in dominants and isolates. Experiments on pairs of freelybehaving dominant and subordinate crayfish have shown that theLG stimulus threshold increased greatly in the subordinate memberof the pair during a fight and slightly or not at all in the dominantmember (Krasne et al., 1997). Although the relative differencein the change of LG threshold in the two crayfish is consistentwith the effect of serotonin reported here, it is not yet knownwhether endogenous serotonin is released during a fight.

Adaptive significance of status-related changes in LG excitability
LG is part of a reflexive escape circuit and is known to be activated only by sharp, sudden taps on the tail, not voluntarilyby the animal. The tailflip pitches the animal upside down andforward, away from the source of the tap. During a fight, sucha tailflip would pitch a subordinate animal upside down and towardits opponent. Suppression of the response of LG during a fightmight help a retreating subordinate that bumps its abdomen preventan unwanted tailflip. An attacking dominant crayfish would bemost likely to experience an LG tailflip triggered by the suddenattack of a third party so that, under these conditions, it maybe advantageous for the threshold of LG to be reduced.

FOOTNOTES

Received June 13, 1996; revised Sept. 10, 1996; accepted Sept. 12, 1996.

This work was supported by National Institutes of Health Research Grant RO1-NS26457 and National Science Foundation ResearchGrant IBN-9423846. We thank C. D. Derby, M. Hörner, F. B. Krasne,and E. A. Kravitz for many helpful discussions of this work.

Correspondence should be addressed to Dr. Donald H. Edwards, Department of Biology, Georgia State University, Atlanta, GA30302-4010.

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Neuronal Adaptations to Changes in the Social Dominance Status of Crayfish

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