Brain type I but not type II IL-1 receptors mediate the effects of IL-1beta  on behavior in mice

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Brain type I but not type II IL-1 receptors mediate the effects of IL-1 $beta$ on behavior in mice

Sandrine Cremona¹, Emmanuelle Goujon¹, Keith W. Kelley², Robert Dantzer¹, and Patricia Parnet¹

¹ Institut National de la Santé et de la Recherche Médicale U394, Neurobiologie Intégrative, 33077 Bordeaux Cedex, France; and ² Department of Animal Sciences, University of Illinois, Urbana, Illinois 61801

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

In the immune system, interleukin (IL)-1 $beta$ effects are mediated by the type I IL-1 receptors (IL-1RI), whereas the type IIIL-1 receptors (IL-1RII) act as inhibitory receptors. IL-1RI andIL-1RII are also present in the brain. To study their functionalityin the brain, mice were centrally treated with neutralizing monoclonalantibody (MAb) directed against IL-1RI (35F5, 1 µg) or againstIL-1RII (4E2, 2 µg) and were centrally injected with recombinantrat IL-1 $beta$ at a dose (2 ng) that decreased social exploration.Only 35F5 was effective in abrogating the behavioral effect ofIL-1 $beta$ . Moreover, 4E2 (1 µg icv) did not potentiate the behavioralresponse to a subthreshold dose of IL-1 $beta$ (1 ng icv). To examinethe ability of brain IL-1RI to mediate the effects of endogenousIL-1 $beta$ , mice were centrally treated with 35F5 (4 µg) and peripherallyinjected with IL-1 $beta$ (1 µg). Like IL-1 receptor antagonist (4 µgicv), 35F5 abrogated the effects of IL-1 $beta$ . These results suggestthat brain IL-1RI mediates the behavioral effects of IL-1 $beta$ inmice.

antibodies; social exploration; mouse

	INTRODUCTION

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INTERLEUKIN-1 $beta$ (IL-1 $beta$ ) is a proinflammatory cytokine synthesized and released by activated macrophages and monocytes duringthe host response to infection. Together with other proinflammatorycytokines, it coordinates the immune response to pathogens (9).IL-1 $beta$ also acts in the brain, where it is synthesized and releasedby glial cells (2, 14). In the brain, IL-1 $beta$ is responsiblefor fever, activation of the hypothalamic-pituitary-adrenal axis,anorexia, sleepiness, and decreased exploration (10). IL-1 $beta$ binds to two types of receptors belonging to the immunoglobulinsuperfamily (19) and representing two separate gene products(5). In the immune system, the type I IL-1 receptor (IL-1RI)is predominantly present on T cells and fibroblasts, whereas thetype II IL-1 receptor (IL-1RII) is found on B cells and macrophages(19). These two receptors are also expressed in the mouse brain(8, 23, 30), predominantly in the choroid plexus and inthe dentate gyrus of the hippocampus. Their cellular localizationwas demonstrated on neuronal cells of the hippocampus of mice(23, 30) and on human and mouse primary cultured astrocytes(27, 29). IL-1RIs transduce the signal to the nucleus, whereasIL-1RIIs, certainly due to their short intracytoplasmic domain(19), cannot transduce the signal (6). IL-1RIs function thenas effectors of IL-1 action, whereas IL-1RIIs have been describedto function as inhibitory receptors downregulating IL-1 action(4, 6, 7, 25). This inhibitory function has been demonstratedwith in vitro experiments using transfected cells with IL-1RIIand showing impaired responses of these cells to an IL-1 stimulation(4, 25). In contrast with these findings, the results ofexperiments using a monoclonal antibody (MAb) against human IL-1RII(ALVA42) show that IL-1RII mediates some of the effects of IL-1 $beta$ ,including the in vivo inhibition of gastric secretion (21) andstimulation of fever response (16) and the prostaglandin E₂release by hypothalamus explants (20). However, the specificityof binding of ALVA42 has been questioned (11). Moreover, thecontribution of IL-1RII to the fever response is doubtful, becausethere is a positive linear correlation between the affinity ofIL-1RI subtype selective ligands and their pyrogenic activity(17).

In view of these contradictory results, the aim of our work was to assess the receptor mechanisms by which IL-1 acts in thebrain to induce behavioral alterations, such as decreased socialexploration. For this purpose, we used neutralizing MAb raisedagainst IL-1RI and IL-1RII to evaluate the respective role ofthese receptors in the decrease of social exploration inducedby IL-1 $beta$ . On the basis of previous experiments showing that IL-1receptor antagonist (IL-1ra), which has a greater affinity forIL-1RI than for IL-1RII in vitro (1), blocks this behavioraleffect of IL-1 $beta$ (3), and despite the fact that this antagonistis usually dosed in excess, our first hypothesis was that IL-1RIis the IL-1 receptor subtype mediating decreased social exploration.Our second hypothesis, based on Colotta and colleagues' reports(6, 7), was that IL-1RII might play a negative regulatoryrole in the brain. Used as dependent variable, the decrease ofsocial exploration is induced by intracerebroventricular injectionof IL-1 $beta$ (13). We predicted that a MAb raised against IL-1RIshould block, whereas a MAb raised against IL-1RII should potentiate,this IL-1 $beta$ action. The first but not the second hypothesis wassupported by the results of the present study.

	MATERIAL AND METHODS

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Animals

Adult male mice of the CD-1 (ICR) BR strain were obtained from Charles River at 3 wk of age. They were housed in polypropylenecages (42 × 22 × 17 cm) in groups of 10 until surgery, with foodand water freely available, at controlled ambient temperature(22 ± 2°C) and under a 12:12-h light-dark cycle (lights off at9:00 AM). Experiments were conducted when mice were 8-10 wk oldand weighed 25-35 g. A total of 95 mice was used for all the experiments.Juvenile male mice (21-28 days) from the same strain and raisedunder the same conditions served as stimulus animals for behavioralobservations. The protocol was approved by the Animal Care andUse Committee of the French Minister of Agriculture.

Surgery

Mice were anesthetized with a mixture of ketamine (12.2 mg/kg) and xylazine (1.8 mg/kg) intraperitoneally injected (10 ml/kgbody wt). Implantation of a guide cannula for intracerebroventricularinjections was carried out when mice were 6 wk old. A 23-gauge,7-mm long, stainless steel guide cannula was stereotaxically insertedover the lateral ventricle at the following coordinates from bregma: $-$ 0.6 mm anterioposterior, ±1.5 mm lateral, $-$ 2 mm vertical accordingto Lehman's stereotaxical atlas (14a). After surgery, animalswere allowed a 2-wk recovery period and individually housed inpolypropylene cages (24 × 14 × 13 cm).

Behavioral Observations

All animals were tested (3 observations/animal) the day before the first injection to ensure stability of the behavioral baselineand to familiarize them with the experimental procedure. Behaviorallyunstable and aggressive mice were discarded at this stage. Thebehavioral test took place in the home cage of experimental mice(24 × 14 × 13 cm) during the dark phase of the cycle. The cagewas placed in a separate room with a red light, and behavior wasmonitored via a video camera. A juvenile conspecific was introducedinto the cage of the experimental mouse for a period of 4 min,and the observer recorded the amount of time (in s) spent by theadult mouse following, grooming, and sniffing its juvenile conspecific.Social exploration was defined as the total time spent in thesebehaviors. The first behavioral observation, serving as the baselinevalue, took place 1 h after lights off. Immediately after, eachmouse received its treatments (randomly allocated) and was tested1.5, 3, and 6 h later (experiments 1 and 2) and 1.5, 3, 6, and9 h later (experiment 3).

Reagents

The IL-1 receptor antagonist (recombinant human IL-1ra; Synergen, Boulder, CO), which binds both IL-1RI and IL-1RII, was dilutedin apyrogenic physiological saline (NaCl 0.9%). The dose of IL-1rawas chosen according to previous experiments run in our laboratory(3). The rat anti-mouse IL-1RI MAb (35F5) and the rat anti-mouseIL-1RII MAb (4E2) (Hoffman Laroche, Nutley, NJ) were diluted inPBS (20 mM sodium phosphate, pH7.4; 0.25 M NaCl). Doses of 35F5(1 and 4 µg/mouse, experiments 1 and 3) to block brain IL-1RIwere selected on the basis of the results of pilot experiments.Because affinity of 4E2 to IL-1RII is twofold higher than 35F5to IL-1RI (22) and because pilot experiments did not revealany effect of this MAb at 0.5 µg/mouse, the doses selected weretwo- to fourfold (experiments 2 and 1, respectively) the doseof 35F5 based on the affinity. Rat immunoglobulin G (IgG) (Sigma)diluted in PBS served as control treatment for the antibodies.IL-1 $beta$ (recombinant rat IL-1 $beta$ , NIBSC, Potters Bar, UK) was dilutedin a 0.1% bovine serum albumin (BSA) solution (Sigma; A-8806).IL-1 $beta$ doses were selected from results of pilot experiments. Freshsolutions were made on every day of test.

Treatments

Experiment 1. On the test session, mice received a double intracerebroventricular injection (1 µl each) with a 1-min timeinterval between the two injections. Mice were first treated withfour different treatments and their respective controls, whichwere IL-1ra (2 µg/mouse) vs. NaCl 0.9%, 35F5 (1 µg/mouse) vs.rat IgG (1 µg/mouse), 4E2 (2 µg/mouse) vs. rat IgG (2 µg/mouse),or 35F5 + 4E2 (1 µg + 2 µg/mouse) vs. rat IgG (3 µg/mouse). Micewere then treated with IL-1 $beta$ (2 ng/mouse) vs. BSA 0.1%. Each mousewas used for two test sessions, receiving the double treatmentsin a randomized order, with a 3-day interval between two testsessions.

Experiment 2. On the test session, mice received a double intracerebroventricular injection (1 µl each) with a 1-min timeinterval between the two injections. Mice were first treated with4E2 (1 µg/mouse) vs. rat IgG (1 µg/mouse) and then treated withIL-1 $beta$ (1 ng/mouse) vs. BSA 0.1%. Each mouse was used for two testsessions, receiving the double treatments in a randomized orderwith a 3-day interval between two test sessions.

Experiment 3. On one test session, mice received the first treatment intracerebroventricularly (1 µl/mouse) and the secondtreatment intraperitoneally (200 µl/mouse) with a 1-min time intervalbetween the two injections. Three different first treatments [ratIgG (1 µg/mouse), IL-1ra (2 µg/mouse), or 35F5 (1 µg/mouse)] combinedwith two second treatments [IL-1 $beta$ (1 µg/mouse) or BSA 0.1%] weretested. Each mouse was used for two test sessions with a 3-dayinterval between two test sessions, receiving two double treatmentsin such a manner that no mouse received the following first treatmentcombinations: IL-1ra and IL-1ra, IL-1ra and 35F5, 35F5 and 35F5.

Statistical Analysis

Durations of social exploration, expressed as percent of the baseline values, were analyzed according to a three-way analysisof variance (ANOVA) (first treatment × second treatment × time),with repeated measures on time factor in the three experiments.When IL-1ra effects were studied (experiment 1), repeated measureswere on second treatment factor. When antibody effects were studied(experiments 1 and 2), repeated measures were on first treatmentfactor. In experiment 3, first treatment and second treatmentfactors were independent. If the three-way ANOVA showed a significantinteraction between the three factors, data were analyzed accordingto a one-way ANOVA followed by the post hoc Newman-Keuls test.

	RESULTS

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Experiment 1: Effects of Intracerebroventricular IL-1ra (2 µg/Mouse), 35F5 (1 µg/Mouse), 4E2 (2 µg/Mouse), or 35F5 + 4E2 (1 µg + 2 µg/Mouse) on the Decrease of Social Exploration Induced by Intracerebroventricular IL-1 $beta$ (2 ng/Mouse)

To determine which receptor subtype mediates the behavioral effects of IL-1 $beta$ , mice were first treated with neutralizing antibodiesagainst IL-1RI (35F5) or IL-1RII (4E2), IL-1ra serving as positivecontrol, before receiving the IL-1 $beta$ injection. IL-1 $beta$ (2 ng icv)induced a significant decrease of social exploration 1.5 and 3h after injection (Fig. 1) [second treatment × time interactionin the 4 groups: IL-1ra, F(2,36) = 8.29, P $<=$ 0.001; 35F5, F(2,26)= 17.6, P $<=$ 0.001; 4E2, F(2,26) = 12.1, P $<=$ 0.001; 35F5 + 4E2,F(2,24) = 10.1, P $<=$ 0.001]. First treatment with IL-1ra (2 µgicv) (Fig. 1A), 35F5 (1 µg icv) (Fig. 1B), or 35F5 + 4E2 (1 +2 µg icv) (Fig. 1D) abrogated this effect [first treatment × secondtreatment interaction: IL-1ra, F(1,18) = 14.1, P $<=$ 0.001; 35F5,F(1,13) = 5.35, P $<=$ 0.05; 35F5 + 4E2, F(1,12) = 14.1, P $<=$ 0.05].In contrast, first treatment with 4E2 (2 µg icv) (Fig. 1C) hadno effect on decrease of social exploration [first treatment ×second treatment interaction: F(1,13) = 0.53, P = NS].

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Fig. 1. Effects of the blockade of brain interleukin (IL)-1 receptors on the behavioral effect of centrally injected IL-1 $beta$ . Effects of IL-1 receptor antagonist (IL-1ra; A; 2 µg/mouse icv), monoclonal antibody 35F5 (B; 1 µg/mouse icv), 4E2 (C; 2 µg/mouse icv), or 35F5 + 4E2 (D; 1 + 2 µg/mouse icv) were assessed by the decrease of social exploration induced by IL-1 $beta$ (2 ng/mouse icv). Mice were injected with NaCl (A, n = 10) or immunoglobulin G (IgG; B and C, n = 8; D, n = 6) and bovine serum albumin (BSA; $open circle$ ), with NaCl (A, n = 10) or IgG (B and C, n = 7; D, n = 8) and IL-1 $beta$ ( $bullet$ ), with IL-1ra (A, n = 10) or 35F5 (B, n = 8) or 4E2 (C, n = 8) or 35F5 + 4E2 (D, n = 6) and BSA ( $triangle$ ), and with IL-1ra (A, n = 10) or 35F5 (B, n = 7) or 4E2 (C, n = 7) or 35F5 + 4E2 (D, n = 8) and IL-1 $beta$ ( $black-triangle$ ). Duration of social exploration (%baseline value) is presented as means ± SE.

Experiment 2: Effects of Intracerebroventricular 4E2 (1 µg/Mouse) on a Subthreshold Dose of Intracerebroventricular IL-1 $beta$ (1 ng/Mouse) on Social Exploration

To detect a possible negative regulatory role of IL-1RII, mice first treated with 4E2 (1 µg/mouse) were injected with a subthresholddose of IL-1 $beta$ (1 ng/mouse). As illustrated in Fig. 2, IL-1 $beta$ induceda small nonsignificant decrease in social exploration [secondtreatment × time interaction: F(2,20) = 3.05, P $<=$ 0.10] and thiseffect was not potentiated by first treatment with 4E2 [firsttreatment × second treatment interaction: F(1,10) = 0.14, P =NS].

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Fig. 2. Effects of the blockade of brain IL-1 receptor type II on the behavioral effect of centrally injected IL-1 $beta$ . Effects of 4E2 (1 µg/mouse icv) injected with a subthreshold dose of IL-1 $beta$ (1 ng/mouse icv) were assessed on social exploration. Mice were injected with IgG and BSA ( $open circle$ , n = 6), with IgG and IL-1 $beta$ ( $bullet$ , n = 6), with 4E2 and BSA ( $triangle$ , n = 6), or with 4E2 and IL-1 $beta$ ( $black-triangle$ , n = 6). Duration of social exploration (%baseline value) is presented as means ± SE.

Experiment 3: Effects of Intracerebroventricular IL-1ra (4 µg/Mouse) or 35F5 (4 µg/Mouse) on the Decrease of Social Exploration Induced by Intraperitoneal IL-1 $beta$ (1 µg/Mouse)

To determine if the IL-1 receptors mediating the effects of exogenous IL-1 $beta$ are the same as these mediating the effects ofendogenous IL-1 $beta$ , mice first treated with an intracerebroventricularinjection of IL-1ra or 35F5 were injected with IL-1 $beta$ in the abdominalcavity. The effect of IL-1 $beta$ was differentially modulated by thefirst treatments according to time [first treatment × second treatment× time interaction: F(6,90) = 2.26, P $<=$ 0.05]. When mice werefirst treated with rat IgG (1 µg/mouse) (Fig. 3A), IL-1 $beta$ (1 µg/mouse)induced a significant decrease of social exploration at all observationtimes [second treatment effect: 1.5 h, F(1,9) = 18.1, P $<=$ 0.01;3 h, F(1,9) = 8.51, P $<=$ 0.05; 6 h, F(1,9) = 17.2, P $<=$ 0.01; 9h, F(1,9) = 6.30, P $<=$ 0.05]. When IL-1 $beta$ injection was precededby IL-1ra (4 µg/mouse) (Fig. 3B) or by 35F5 (4 µg/mouse) (Fig.3C), its effects were totally abrogated 3, 6, and 9 h postinjection.At 1.5 h, IL-1 $beta$ still produced a significant decrease of socialexploration [second treatment effect: IL-1ra, F(1,10) = 10.7,P $<=$ 0.01; 35F5, F(1,11) = 13.8, P $<=$ 0.01], which was significantlyattenuated by the first treatment [first treatment effect: F(2,16)= 6.78, P $<=$ 0.01; Newman-Keuls: IgG-IL-1 $beta$ vs. IL-1ra-IL-1 $beta$ , P $<=$ 0.01, and vs. 35F5-IL-1 $beta$ , P $<=$ 0.05].

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Fig. 3. Effects of the blockade of brain IL-1 receptors on the behavioral effect of peritoneally injected IL-1 $beta$ . Effects of IL-1ra (4 µg/mouse icv) or 35F5 (4 µg/mouse icv) were assessed on the decrease of social exploration induced by IL-1 $beta$ (1 µg/mouse ip). Mice were first treated with IgG (A), IL-1ra (B), or 35F5 (C) and treated with BSA 0.1% ( $open circle$ ; A, n = 5; B and C, n = 6) or IL-1 $beta$ ( $bullet$ ; A and B, n = 6; C: n = 7). Duration of social exploration (%baseline value) is presented as means ± SE.

	DISCUSSION

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The present results demonstrate that blockade of IL-1RI abrogated the behavioral effects of centrally and peripherally injectedIL-1 $beta$ in mice, whereas blockade of IL-1RII had no effect on centrallyinjected IL-1 $beta$ .

Previous in vivo experiments on the role of IL-1 receptor subtypes have mainly been carried out in relationship to the immuneeffects of IL-1 $beta$ . Accordingly, blockade of IL-1RI with a neutralizingMAb has been shown to decrease the acute inflammatory responsein mice (12, 18, 22), confirming the results from in vitrostudies demonstrating the predominant role of IL-1RI in the signaltransduction of IL-1. Moreover, peripheral IL-1RI has been shownto be involved in centrally mediated physiological responses toinfection: intraperitoneal administration of 35F5 (IL-1RI-neutralizingMAb) abrogated the LPS-induced adrenocorticotropic hormone releasein mice (26); there was a positive correlation between the affinityof selective ligands to IL-1RI intraperitoneally administeredand the fever response of rats (17); IL-1RI-knockout mice werefound to be resistant to fever, lethargy, and anorexia inducedby an intraperitoneal administration of IL-1 $beta$ (15). Becausebinding sites to IL-1 are expressed in the brain of mice (8,23, 30), the aim of this study was to investigate the contributionof the brain type I and type II IL-1 receptors to the centraleffects of IL-1 $beta$ on behavior. Our results show that blockade ofthe brain IL-1RI with a neutralizing MAb (35F5) fully abrogatesthe decrease of social exploration induced by intracerebroventricularlyinjected IL-1 $beta$ , whereas the blockade of brain IL-1RII with a neutralizingMAb (4E2) has no effect. Moreover, the simultaneous blockade ofthe two IL-1 receptor subtypes produces an identical curve responseas blockade of IL-1RI alone, confirming that IL-1RI plays a predominantrole in the IL-1 $beta$ -induced decrease of social exploration. Thiswork is the first to demonstrate the functionality of IL-1RI subtypein the brain of mice.

The significance of these results is critically dependent on the effectiveness and specificity of the MAb. 35F5 and 4E2 havebeen shown to bind specifically to IL-1RI and IL-1RII, respectively,without any interference (22). The affinity of 4E2 to IL-1RII,twofold greater than 35F5 to IL-1RI (22), ensures the full blockadeof brain IL-1RII by the doses used in this study. The lack ofeffect of nonspecific rat IgG injected in control animals confirmsthe specificity of both MAb effects.

The fact that IL-1RI blockade abrogates the behavioral effect of IL-1 $beta$ does not allow the exclusion of a possible contributionof IL-1RII to the regulation of IL-1 action in the brain. In theimmune system, IL-1RII is described as an active regulative targetthat is able to downregulate IL-1 action (4, 6, 7, 25).Because IL-1 $beta$ has a higher affinity for IL-1RII than for IL-1RI(28), this property should be of physiological importance. Inaccordance with this hypothesis, blockade of IL-1RII with a MAbwas found to potentiate the activity of a suboptimal concentrationof IL-1 $beta$ on cytokine production by cultured monocytes (6),and transfection of cells with IL-1RII impaired their responsivenessto IL-1 (4, 25). In contrast with these results, blockadeof IL-1RII in the brain with a neutralizing MAb (ALVA42) abrogatedthe in vivo fever response of rats to IL-1 $beta$ (16) and the exvivo IL-1 $beta$ -induced prostagladin E₂ release from hypothalamus explants(20). However, the significance of these results is doubtfulbecause ALVA42 was subsequently found to bind the human leukocyteantigen DR $alpha$ - and $beta$ -chains rather than IL-1RII (11). Therefore,we tested the possible negative regulatory role of IL-1RII inthe brain by looking for a possible potentiation of the effectof a subthreshold dose of intracerebroventricular IL-1 $beta$ on socialexploration in mice treated with a neutralizing MAb against IL-1RII(4E2). We were unable to observe any effect of this MAb on thebehavioral effects of a subthreshold dose of IL-1 $beta$ . It is difficultto decide whether this negative result is due to the lack of sensitivityof the behavioral response under study or to the lack of a functionalrole of IL-1RII in the brain.

Because all these results were observed with exogenous IL-1 $beta$ , it was important to study the physiological role of brain IL-1RIon the action of endogenous IL-1 $beta$ . A convenient way to inducethe expression of brain IL-1 $beta$ is to inject IL-1 $beta$ at the periphery(24). We therefore chose this model to induce endogenous brainIL-1 $beta$ . Our results show that blockade of the brain IL-1RI witha neutralizing MAb (35F5) abrogated the decrease of social explorationinduced by intraperitoneally injected IL-1 $beta$ . The fact that thisabrogation was only partial 1.5 h after the injection suggeststhat a minor part of the decrease of social exploration was dueto the IL-1 $beta$ action at the periphery or to other proinflammatorycytokines (e.g., tumor necrosis factor- $alpha$ and IL-6) that couldbe induced in the brain in response to peripheral IL-1 $beta$ . Thiscannot be explained by interaction of IL-1 $beta$ with brain IL-1RII,because the blockade of central IL-1 receptors with IL-1ra alsopartially abrogated the IL-1 $beta$ effects on behavior 1.5 h postinjection.These results confirm that IL-1 $beta$ acts in the brain to decreasesocial exploration in mice (3) and clearly demonstrate thatthese effects are mediated by brain IL-1RI.

Perspectives

The existence of multiple cytokine receptor subtypes in the brain raises questions about the functional significance of thisdiversity. The present results clearly show the importance ofselecting appropriate tools to address these questions.

	ACKNOWLEDGEMENTS

We thank V. Tridon for skillful assistance with surgery, Dr. R. Chizzonite for the generous gift of rat anti-mouse IL-1 receptorMAb 35F5 and 4E2, and Dr. R. J. Vannice for the generous giftof recombinant human IL-1ra. Recombinant rat IL-1 $beta$ was obtainedthrough the BIOMED I Concerted Action "Cytokines in the Brain."

	FOOTNOTES

This work was partially supported by National Institutes of Health Grant MH-51569-01A2 to K. W. Kelley. S. Cremona is financiallysupported by the Conseil Régional d'Aquitaine (France).

Address for reprint requests: S. Cremona, Inserm U394 Neurobiologie Intégrative, 1 rue Camille Saint-Saëns, 33077 Bordeaux Cedex, France.

Received 20 June 1997; accepted in final form 17 November 1997.

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Brain type I but not type II IL-1 receptors mediate the effects of IL-1 on behavior in mice

Brain type I but not type II IL-1 receptors mediate the effects of IL-1 $beta$ on behavior in mice