Cytokines mediate protective stimulation of glucocorticoid output during autoimmunity: involvement of IL-1

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Cytokines mediate protective stimulation of glucocorticoid output during autoimmunity: involvement of IL-1

Adriana Del Rey¹, Isabel Klusman², and Hugo O. Besedovsky¹

¹ Division of Immunophysiology, Institute of Physiology, Medical Faculty, D-35037 Marburg, Germany; and ² Division of Neurobiology, Department of Research, Kantonsspital, CH-4031 Basel, Switzerland

ABSTRACT

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Abstract
Introduction
Methods
Results
Discussion
References

Endogenous glucocorticoid levels are increased during experimental autoimmune encephalomyelitis (EAE) in Lewis rats. Althoughthis endocrine response is essential for survival, the mechanismthat triggers the stimulation of glucocorticoid output duringthe disease remains unknown. We report here that 1) after immunizationwith the encephalitogenic antigen myelin basic protein (MBP),increased blood glucocorticoid levels are not only observed inLewis rats, but also in PVG rats, which do not develop EAE; 2)immune cells obtained from animals with EAE and stimulated invitro with MBP produced mediators that increased glucocorticoidlevels when administered to naive recipients; and 3) acute invivo blockade of interleukin-1 (IL-1) receptors inhibited, toa large extent, the increase in corticosterone levels during EAE.These results show that the increase in corticosterone levelsafter immunization with MBP can be dissociated from the stressof the paralytic attack that characterizes EAE. Furthermore, theyindicate that an endocrine response, which is decisive for theprevention or moderation of EAE, is mainly the result of the stimulationof the hypothalamic-pituitary-adrenal axis by cytokines producedduring the immune response that induces the autoimmune disease.

corticosterone; neuroimmunology; interleukin-1 receptor antagonist; experimental autoimmune encephalomyelitis

	INTRODUCTION

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EXPERIMENTAL AUTOIMMUNE encephalomyelitis (EAE) has been widely used as a model of human multiple sclerosis (MS). The diseasecan be induced in different species of laboratory animals by injectionof central nervous tissue antigens emulsified in adjuvants. InLewis rats, a susceptible strain, EAE is manifested by a paralyticattack that affects the tail and hind limbs 11-14 days after injectionof guinea pig myelin basic protein (MBP) as encephalitogenic antigen.T helper 1 lymphocytes mediate the autoimmune component of thedisease, and cytokines such as interleukin-1 $beta$ (IL-1 $beta$ ) and tumornecrosis factor- $alpha$ (TNF- $alpha$ ) are implicated in the pathogenesis ofEAE (for review see Ref. 22). During the experimentally induceddisease in Lewis rats, the endogenous levels of glucocorticoidsare elevated (13, 14). Recovery from the disease, which occursspontaneously 4-5 days after the onset of the paralytic signs,is clearly dependent on this endocrine change because adrenalectomyresults in death of the animals (14). Remission can be obtainedin adrenalectomized animals only when glucocorticoids are administeredin doses that result in an elevation of the plasma level of thishormone comparable to that observed in intact rats with EAE (14).

Despite the crucial role played by the increased glucocorticoid output in the recovery from EAE, the mechanism that triggersthis endocrine response is not known. It is reasonable to assumethat the hypothalamic-pituitary-adrenal (HPA) axis is stimulatedby the stress caused by the paralytic attack that characterizesthis disease (13, 18). Alternatively, such an increase inblood glucocorticoid levels could be, at least in part, immunologicallymediated. This is hypothesized on the basis of previouswork showing that the immune response to innocuous antigens resultsin stimulation of the HPA axis (7, 26, 27). Furthermore,products derived from activated immune cells, including IL-1 $beta$ ,IL-6, and TNF- $alpha$ , can increase glucocorticoid output when theyare administered to normal animals (Refs. 3-5; for review seeRef. 2). On this basis, we have investigated the possibilitythat an immunoregulatory circuit, involving immune-derived productsand glucocorticoid hormones, operates during the course of EAE.For this purpose, we have first studied whether injection of MBPalso results in an increased glucocorticoid output in PVG rats,which develop an immune response to this encephalitogenic antigenbut are resistant to the induction of EAE (1). We have alsostudied whether in vitro stimulation of immune cells with MBPresults in the production of factor(s) capable of inducing anincrease in glucocorticoid levels on injection into normal animals.Finally, because IL-1 $beta$ is probably the most potent cytokine thatcan stimulate the HPA axis (3), we have explored whether endogenousIL-1 contributes to the increase in glucocorticoid levels observedduring EAE.

	MATERIAL AND METHODS

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Animals. Lewis male rats (6-8 wk old, 200 g body wt) were purchased from Iffa Credo and PVG male rats (6-8 wk old, 150 g body wt) fromHarlan Olac. Rats were caged individually for 7 days before startingthe experiments and kept isolated throughout. Animals were housedin temperature- and light (12:12-h light-dark cycles)-controlledrooms and were fed ad libitum.

Inoculation of MBP, clinical signs, and blood sampling. For minimization of the stress of bleeding, a silicone cannula was chronically implanted into one of the jugular veins ofLewis and PVG rats according to standard procedures (3). Fiveto seven days after the operation, 100 µl of an emulsion containing25 µg guinea pig MBP in complete Freund's adjuvant (CFA)-incompleteFreund's adjuvant (IFA) containing 4 mg/ml killed Mycobacteriumtuberculosis, H37 RA (Difco) were inoculated subcutaneously ineach hind foot pad. Groups of rats receiving CFA, IFA, or physiologicalsaline (0.9% NaCl) were included, simultaneously, as controlsto exclude any effects of the CFA alone. All animals were weighedand scored daily for clinical signs of disease, based on a conventionalscale from 0 to 5 depending on severity: 0, normal; 1, limp tail;2, hind limb paresis; 3, unilateral hind limb paralysis; 4, bilateralhind limb paralysis; 5, bilateral hind limb paralysis and incontinence.Blood samples were withdrawn via the cannula between 9:30 and10:30 AM 1 day before inoculation and once a day at the same timefrom day 6 to day 20 postinoculation. Blood samples were collectedin chilled EDTA-coated tubes, immediately centrifuged, and aliquotedfor hormone determinations.

Spleen cell supernatants. Spleen cells were obtained from Lewis rats that received MBP in CFA 11 days earlier. Then, 1 × 10⁷ cells/ml were cultured in RPMI 1640 medium supplemented with10% fetal calf serum, 5 × 10⁵ M 2-ME, 1% penicillin-streptomycin, 1% glutamine, and 1% HEPES,with or without addition of 10 µg/ml MBP. Supernatants were collectedafter 22 h of incubation at 37°C. The culture medium containing10 µg/ml MBP and incubated for the same time was used as control.Between 9:30 and 10:30 AM, a basal blood sample was obtained fromchronically cannulated normal Lewis rats. Immediately after this,1 ml of each supernatant or of the control medium was injectedvia the implanted cannula. Additional blood samples were obtainedat the time points indicated in the figures and processed as previouslydescribed.

Administration of IL-1ra. EAE was induced in chronically cannulated Lewis rats as previously described, and animals were scored daily for clinical signsof disease. Other groups of cannulated rats received only PBSinoculated subcutaneously in each hind foot pad. One day beforeinoculation and every day from day 5 postinoculation, blood sampleswere withdrawn via the cannula between 9:30 and 10:30 AM. Immediatelyafter the sample corresponding to day 13 postinoculation was obtained,IL-1 receptor antagonist (IL-1ra; 100 mg/kg body wt; kindly providedby Dr. J. Relton, Synergen, Boulder, Colorado) was administeredsubcutaneously as a single bolus injection to a group of ratsthat were inoculated with MBP. The other group of MBP-injectedrats and the PBS-injected animals received PBS also injected subcutaneously.Additional blood samples were collected on this day after 2, 4,and 6 h. Thereafter, a blood sample was obtained between 9:30and 10:30 AM every 24 h until day 20.

Corticosterone determinations. Plasma corticosterone levels were determined by RIA as described previously (3).

Statistical analysis. Results are expressed as means ± SE. Data were analyzed using one-way ANOVA followed by Fisher's test for multiple comparisons.Differences were considered significant at P < 0.05.

	RESULTS

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Clinical signs and blood corticosterone levels in Lewis rats during EAE. The levels of corticosterone in blood of rats from the three control groups (CFA, IFA, and saline) remained within the rangeof basal values from day 6 to day 20 postinoculation (Fig. 1A).The only exception was observed on days 17 and 18 postinoculation,when blood glucocorticoid levels of rats that received CFA tendedto increase. In contrast, the levels of corticosterone in thegroup of rats that received MBP started to increase on day 11,peaked on day 13, and remained elevated until day 19 postinoculation.By day 20 postinoculation, the levels of corticosterone in bloodof MBP-injected rats returned to the normal range. Only thoseanimals that received MBP lost weight, and this started on day12 after immunization (data not shown). Mild signs of disease(limp tail) became apparent in some animals on this day (Fig.1B). The disease was maximally expressed in all MBP-injected ratson days 15-16, and thereafter the clinical signs decreased progressively.It is noteworthy that the levels of glucocorticoids remained elevateduntil day 19 postinoculation, when the clinical signs had alreadydisappeared in most of the animals.

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Fig. 1. Blood corticosterone levels and clinical signs after myelin basic protein (MBP) administration to Lewis rats. Lewis rats received either MBP in complete Freund's adjuvant (CFA) (n = 14), CFA (n = 13), incomplete Freund's adjuvant (IFA) (n = 6), or saline (n = 9). A: blood corticosterone levels were determined at times indicated. Statistical differences between groups at each given time point were determined by using one-way ANOVA followed by Fisher's test for multiple comparisons. Blood corticosterone levels in group of MBP-injected rats are statistically significantly different from 3 control groups from day 12 to day 19 postinoculation (P < 0.05), with the exception of days 17 and 18, when they do not statistically differ from levels of animals that received CFA. B: clinical signs of group of rats that received MBP. Each point in curves represents mean ± SE.

Changes in blood glucocorticoid levels in PVG rats after immunization with MBP. As in the case of Lewis rats, different groups of chronically cannulated PVG rats received either MBP emulsified in CFA, CFAalone, IFA, or physiological saline. Animals of the four experimentalgroups gained weight during the 20 days after immunization (datanot shown). None of the MBP-injected rats developed symptoms ofEAE. However, as in the case of Lewis rats, changes in corticosteroneblood levels were noticed in these animals (Fig. 2). With theexception of a transient increase on day 7 in blood corticosteronelevels of CFA-injected rats, only the MBP-injected animals showeda sustained elevation in the levels of the hormone. The increasein blood corticosterone levels in this group of animals becameevident on day 9 after immunization with MBP and fluctuated athigh levels until day 17 postinoculation. Thereafter, corticosteroneconcentrations in blood returned to basal levels.

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Fig. 2. Blood corticosterone levels after MBP administration to PVG rats. PVG rats received either MBP in CFA (n = 10), CFA (n = 8), IFA (n = 7), or saline (n = 6). Same procedures and statistical analysis as described in Fig. 1 were used. The following statistically significant differences (P < 0.05) were detected: CFA vs. IFA and vs. saline on day 7; MBP vs. IFA and vs. saline on day 8; MBP vs. all other groups on days 9, 11, 12, 14, and 15. None of the MBP-injected PVG rats showed any clinical sign of experimental autoimmune encephalomyelitis (EAE). Each point in curves represents mean ± SE.

Products of MBP-stimulated immune cells, obtained from rats with EAE, increase blood corticosterone levels. Supernatants of spleen cells from MBP-primed rats further stimulated in vitro with the antigen, induced a clear increase inblood corticosterone levels 8 h after injection into naive Lewisrats (Fig. 3). No comparable changes were observed in animalsthat received supernatants from non-restimulated spleen cellsor the culture medium incubated with MBP.

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Fig. 3. Products released by MBP-stimulated immune cells from rats with EAE increase blood corticosterone levels. Lewis rats received either supernatants of spleen cells obtained from Lewis rats with EAE and restimulated in vitro with MBP (MBP + MBP), or from nonrestimulated cells (MBP + med) or culture medium containing MBP (med + MBP). Blood corticosterone levels were determined at times indicated in figure. Each point in curves represents mean ± SE of corticosterone values from 5 animals per group. Statistical analysis was performed as described in Fig. 1. * P < 0.05 vs. MBP + med and vs. med + MBP.

Blockade of IL-1 receptors interferes with increase in corticosterone levels during EAE. A single injection of the specific IL-1ra was injected into Lewis rats 13 days after inoculation of MBP, when the diseasewas already manifested and glucocorticoid levels were clearlyelevated. This treatment did not significantly affect the clinicalsigns of EAE (data not shown). Two hours after administrationof IL-1ra, a 60% decrease in corticosterone levels was observedcompared with those of rats with EAE that received PBS (Fig. 4).The levels attained at 4 h were comparable to those of normalrats. When corticosterone blood levels increased in normal rats,in accord with the circadian variation (see controls Fig. 4),the difference between control rats and those rats given MBP,with or without IL-1ra treatment, was no longer apparent. Surprisingly,given the short half-life of IL-1ra (17), decreased corticosteronelevels in blood of rats with EAE that received IL-1ra were stillobserved in the morning of the next day (24 h after IL-1ra injection),and were even more markedly decreased on the following day (15days after injection of MBP, 48 h after injection of IL-1ra, Fig.5). This was followed by an increase in glucocorticoid levelson day 16, which did not significantly differ from those of MBP-injectedrats that received PBS.

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Fig. 4. Blockade of interleukin-1 (IL-1) receptors interferes with increase in corticosterone levels during EAE. Lewis rats received MBP or PBS. Blood samples were obtained 1 day before inoculation and once daily from day 5 to day 20 postinoculation. Levels of corticosterone determined on day 13 postinoculation are shown, when all MBP-injected rats already showed clinical signs of EAE. Immediately after obtaining blood sample corresponding to this day (time 0), we administered IL-1 receptor antagonist (IL-1ra) to a group of MBP-injected rats (MBP + IL-1ra, n = 8). Another group of MBP-injected rats (n = 12) and PBS-injected animals (n = 8) received the vehicle alone (MBP + PBS and PBS + PBS, respectively). Additional blood samples were collected on this day after 2, 4, and 6 h. Each bar represents mean ± SE of corticosterone values. Statistical analysis was performed as described in Fig. 1. * P < 0.05 vs. MBP + PBS.

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Fig. 5. Decreased glucocorticoid levels after injection of IL-1ra into rats with EAE. See legend for Fig. 4. A: results obtained from day $-$ 1 to day 20 after MBP or PBS injection. Statistical analysis was performed as described in Fig. 1. On days 12 and 13 before IL-1ra administration, corticosterone levels of animals that received MBP differ from those of rats that received PBS (P < 0.05). After IL-1ra or PBS injection, the following statistical significant differences (P < 0.05) in corticosterone levels were detected: MBP + PBS vs. PBS + PBS (days 14, 15, 17, and 18); MBP + IL-1ra vs. PBS + PBS (days 16, 17, and 18); MBP + IL-1ra vs. MBP + PBS (day 15). B: results obtained on day 15, when maximal decrease in glucocorticoid levels after injection of IL-1ra into rats with EAE was observed. * P < 0.05 vs. MBP + IL-1ra and vs. PBS + PBS.

	DISCUSSION

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The studies reported here tested the possibility that an immune regulatory pathway, involving endogenous cytokines and glucocorticoids,operates during EAE in Lewis rats. We first demonstrate that theelevation of glucocorticoid levels observed in this strain inparallel to the clinical signs was induced by the encephalitogenicantigen and not by the adjuvant. MBP inoculation also triggeredan increase in corticosterone levels in PVG rats, which respondimmunologically to this antigen but do not develop the disease.These results indicate that the endocrine change observed duringEAE can be induced by the immune response to MBP and it is notnecessarily a consequence of the stress of the paralytic attackthat characterizes the disease.

After in vitro restimulation, spleen cells obtained from MBP-primed Lewis rats released products with glucocorticoid-stimulatoryactivity. These results support the possibility that cytokinesmediate the activation of the HPA axis during EAE. We and othershave previously used mitogens to prepare cytokine-containing supernatantsthat increase glucocorticoid output when administered to naiverecipients (4, 6, 8). These supernatants, as well aspurified or recombinant cytokines, induce an increase in glucocorticoidlevels within minutes after injection (3-6, 8). In the caseof the MBP supernatants, this effect was observed 8 h after administration,which is a delayed response compared with that obtained with supernatantsfrom mitogen-stimulated spleen cells. One main explanation forthis is that the supernatants derived from an antigen-specificimmune response would be expected to contain a mixture of cytokinesthat is either qualitatively or quantitatively different fromthat obtained after polyclonal stimulation of mononuclear cellsby mitogens. It seems that the MBP supernatant increased bloodglucocorticoid levels indirectly, via secondarily produced endogenousfactors. This is supported by the finding that a similar delayin the increase in glucocorticoid levels is observed after administrationof conditioned medium from a T cell lymphoma (21). This responserequires the presence of T cells in the host, indicating thatthe material injected triggers the production of the productsthat finally cause the endocrine effect.

Finally, we show here that endogenous IL-1 contributed to the increased glucocorticoid output during EAE. Administration ofIL-1ra close to the peak of EAE caused a reduction in corticosteronelevels within 2 h. This effect was most likely due to an acuteblockade of the action of IL-1 on the HPA axis. However, the levelsof corticosterone were still reduced 24 h later, and the decreasewas even more pronounced after 48 h. It is known that IL-1 canstimulate its own production (9, 16) and that of other cytokinesproduced during EAE (for review see Ref. 22), such as TNF- $alpha$ and IL-6 (9), which can also increase glucocorticoid levels(3). Thus the prolonged reduction in the levels of corticosteronecaused by the receptor antagonist could be the result of interferingtransiently with a cytokine cascade that stimulates glucocorticoidoutput. Administration of a single injection of IL-1ra did notsignificantly affect the clinical signs of EAE. This is expectedbecause it is known that IL-1ra needs to be injected repeatedlyover several days to moderate or prevent EAE (17).

The data reported here, together with previous publications, allow some speculation on how immune-HPA axis interactions maycontribute in determining susceptibility to EAE. In Lewis ratsthat are genetically predisposed to the induction of differentautoimmune diseases, the immune-mediated stimulation of the HPAaxis results in moderation of EAE. Such stimulation is, however,not sufficient to prevent the development of the disease in thisstrain. Although the concentration of corticosterone in the bloodof rats with EAE was increased in the morning, afternoon levelsdid not differ from those of the simultaneously injected controlrats (Fig. 4). These results suggest that the circadian patternof plasma corticosterone is abolished in MBP-immunized Lewis ratsand that corticosterone levels are stabilized at higher levelsof the circadian rhythm. It is also conceivable that the endocrineresponse that parallels the disease in Lewis rats is less intensethan what could be expected, especially because several proinflammatorycytokines produced in the brain during EAE (for review see Ref.2) can stimulate the HPA axis acting at central levels (forreview see Ref. 22). This is further supported by the observationsthat Lewis rats exhibit a decreased activation of the HPA axisin response to bacterial wall products (28), and hypothalamiccorticotrophin-releasing hormone-producing neurons in this strainshow a blunted response to the stimulatory action of IL-1 (29).Defects in the response of the HPA axis to immune-derived productshave also been reported in animal models of spontaneous autoimmunethyroiditis (26) and lupus (11). In PVG rats, endogenous glucocorticoidsseem to be effective enough to impede the occurrence of the disease,because animals of this strain develop EAE when they are adrenalectomized(19). The increase in corticosterone output triggered by theimmune response to MBP is a mechanism that may at least partlyunderlie the resistance of PVG rats to EAE induction. Ultradianvariations of plasma corticosterone may also play a protectiverole. In fact, we have observed that although at the nadir ofthe circadian cycle plasma corticosterone levels are comparablein normal Lewis and PVG rats, there are major differences in theamplitude of the circadian pattern, being several fold higherin PVG than in Lewis rats (del Rey, Klusman, and Besedovsky, unpublisheddata). Other authors have reported significant differences inthe circadian rhythm of plasma corticosterone between Lewis andFisher rats, a strain that is resistant to EAE induction (10).

As already mentioned, EAE is considered a model of MS. Some indirect evidence indicates that in humans interactions betweenimmune-derived cytokines and endogenous glucocorticoids may alsooperate during the course of MS. After allogeneic and mitogenstimulation, human peripheral blood mononuclear cells can producefactors capable of stimulating the HPA axis (4, 6). Alsothe administration to human volunteers of a low dose of endotoxin,which induces the production of IL-1 $beta$ , IL-6, and TNF- $alpha$ , resultsin activation of the HPA axis (20, 25). More specificallyit has been shown that peripheral blood monocytes from MS patientsin the acute phase produce more IL-1, IL-6, and TNF than thosefrom healthy subjects (12) and that there is an excessive productionof IL-1 $beta$ when monocytes from patients with chronic progressiveMS are stimulated with T cell-derived lymphokines (15). Takentogether, these data indicate that cytokines that can stimulatethe HPA axis are produced during the acute phase of MS. On theother hand, it has been shown that the activity of the HPA axisis enhanced in a considerably large proportion of MS patients(23). Also, an increase in the size of the adrenal gland hasbeen found at autopsy, indicating that these glands are beinghyperstimulated in the course of MS (24). Although fragmentary,the evidence suggests that interactions between endogenous glucocorticoidsand cytokines also exist during the course of MS.

In conclusion, the results shown here, together with the reported protective effect of endogenous glucocorticoids during EAE(13, 14), illustrate the relevant immunoregulatory role ofa feedback mechanism integrated by immune cell products and theHPA axis. These data provide the first example of a specific immuneresponse that triggers an autoimmune process and simultaneouslyactivates an endocrine mechanism that either prevents or moderatesthis process. In the particular case of EAE, our results indicatethe existence of a subtle balance between opposing effects ofIL-1 that on one hand contributes to the inflammatory componentof the disease (for review see Ref. 22), while on the otherinduces the release of glucocorticoids, which are powerful anti-inflammatoryhormones (for review see Ref. 2).

Perspectives

The knowledge that endogenous cytokines induce the stimulation of corticosterone output during EAE requires a more detaileddefinition of the cytokine cascade involved in this process. Thistype of study needs to be extended to other models of autoimmunediseases. The data presented here also provide the rationale toexplore the cytokine-HPA axis circuit in patients with MS andits potential relevance for the course of the disease in humans.Furthermore, these studies emphasize the need of simultaneousevaluations of cytokine production and the function of the HPAaxis in patients with MS, particularly when cytokine antagonistsare used as a therapeutic approach. The possibility exists thatinappropriate doses of an antagonist could interfere with theprotective glucocorticoid response more effectively than withthe autoimmune response, causing paradoxical and undesirable effects.

	ACKNOWLEDGEMENTS

We thank Drs. H. Wekerle and J. Relton for kindly providing the MBP and IL-1ra, respectively, and Dr. G. McGregor for criticallyreviewing the manuscript.

	FOOTNOTES

This work was supported by the Volkswagen Stiftung, the Deutsche Forschungsgemeinschaft (SFB 297), and the Swiss Nationalfonds.

I. Klusman was supported by a grant from the Schweizerische Multiple Sklerose Gesellschaft.

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate this fact.

Address for reprint requests: A. del Rey, Institute of Physiology, Div. of Immunophysiology, Deutschhaustrasse 2, D-35037 Marburg, Germany.

Received 30 January 1998; accepted in final form 30 June 1998.

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