Ambiguous Role of Interleukin-12 in Yersinia enterocolitica Infection in Susceptible and Resistant Mouse Strains

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Infect Immun, May 1998, p. 2213-2220, Vol. 66, No. 5
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Ambiguous Role of Interleukin-12 in Yersinia enterocolitica Infection in Susceptible and Resistant Mouse Strains

Erwin Bohn,¹ Edgar Schmitt,² Claudia Bielfeldt,¹ Annette Noll,¹ Ralf Schulte,¹ and Ingo B. Autenrieth¹^,^*

Max-von-Pettenkofer-Institut, Ludwig-Maximilians-University, Munich,¹ and Institut für Immunologie, University of Mainz, Mainz,² Germany

Received 15 September 1997/Returned for modification 2 December 1997/Accepted 25 February 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Endogenous interleukin-12 (IL-12) mediates protection against Yersinia enterocolitica in C57BL/6 mice by triggering gammainterferon (IFN- $gamma$ ) production in NK and CD4⁺ T cells. Administration of exogenous IL-12 confers protectionagainst yersiniae in Yersinia-susceptible BALB/c mice but exacerbatesyersiniosis in resistant C57BL/6 mice. Therefore, we wanted todissect the different mechanisms exerted by IL-12 during Yersiniainfections by using different models of Yersinia-resistant and-susceptible mice, including resistant C57BL/6 mice, susceptibleBALB/c mice, intermediate-susceptible wild-type 129/Sv mice, 129/SvIFN- $gamma$ -receptor-deficient (IFN- $gamma$ R^/) mice and C57BL/6 tumor necrosis factor (TNF) receptor p55 chain-deficient(TNFR p55^/) mice. IFN- $gamma$ R^/ mice turned out to be highly susceptible to infection by Y. enterocoliticacompared with IFN- $gamma$ R^+/+ mice. Administration of IL-12 was protective in IFN- $gamma$ R^+/+ mice but not in IFN- $gamma$ R^/ mice, suggesting that IFN- $gamma$ R-induced mechanisms are essentialfor IL-12-induced resistance against yersiniae. BALB/c mice couldbe rendered Yersinia resistant by administration of anti-CD4 antibodiesor by administration of IL-12. In contrast, C57BL/6 mice couldbe rendered more resistant by administration of transforming growthfactor $beta$ (TGF- $beta$ ). Furthermore, IL-12-triggered toxic effects inC57BL/6 mice were abrogated by coadministration of TGF- $beta$ . Whileadministration of IL-12 alone increased TNF- $alpha$ levels, administrationof TGF- $beta$ or TGF- $beta$ plus IL-12 decreased both TNF- $alpha$ and IFN- $gamma$ levelsin Yersinia-infected C57BL/6 mice. Moreover, IL-12 did not inducetoxicity in Yersinia-infected TNFR p55^/ mice, suggesting that TNF- $alpha$ accounts for IL-12-induced toxicity.Taken together, IL-12 may induce different effector mechanismsin BALB/c and C57BL/6 mice resulting either in protection or exacerbation.These results are important for understanding the critical balanceof proinflammatory and regulatory cytokines in bacterial infectionswhich is decisive for beneficial effects of cytokine therapy.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Yersinia enterocolitica is a gram-negative, predominantly extracellularly located pathogen which causes enteritis and enterocolitisin humans and rodents (17, 24, 40). Moreover, systemic infectionincluding abscesses and granulomatous lesions in the spleen andliver occur, particularly in immunocompromised individuals (9,36). As in infections with intracellular pathogens, T cells,particularly CD4⁺ Th1 cells, in cooperation with activated macrophages are requiredfor clearance of primary Yersinia infection (1, 2, 5).The protective host response to yersiniosis is mediated by variousproinflammatory cytokines. Thus, neutralization of tumor necrosisfactor alpha (TNF- $alpha$ ), gamma interferon (IFN- $gamma$ ), or interleukin-12(IL-12) abrogates resistance against this pathogen, suggestingthat T-cell-activated macrophages are important effector cellsin the protective host response to yersiniae (1, 4, 8).

Previous studies showed that C57BL/6 mice are resistant against Y. enterocolitica while BALB/c mice are susceptible (16).Administration of IFN- $gamma$ , IL-12, or anti-IL-4 antibodies (Abs)rendered BALB/c mice resistant to yersiniae. In contrast, in Yersinia-resistantC57BL/6 mice, administration of IFN- $gamma$ and anti-IL-4 Abs did notsignificantly affect yersiniosis. However, IL-12 treatment ofYersinia-infected C57BL/6 mice increased bacterial numbers inthe spleen and caused toxic effects in the liver (1, 8).Experimental viral infection revealed that TNF- $alpha$ is involved inIL-12-triggered toxicity (31). Furthermore, it was shown thatthe higher and predominantly IL-12-dependent IFN- $gamma$ levels producedby CD4⁺ T and NK cells of C57BL/6 mice correlate with resistance againstyersiniae compared to BALB/c mice. In line with these results,IL-12-mediated protection of BALB/c mice was partially abrogatedby administration of anti-IFN- $gamma$ Abs (8).

In various infection models, it was shown that transforming growth factor $beta$ (TGF- $beta$ ) counteracts IL-12-mediated resistance.TGF- $beta$ is an immunoregulatory molecule which inhibits the activationof macrophages (30, 45) and the generation and cytolytic activitiesof cytotoxic T cells, natural killer cells, and lymphokine-activatedkiller cells (23, 37, 38). The immunosuppressive effectof TGF- $beta$ appears to be mainly caused by inhibition of IFN- $gamma$ , TNF- $alpha$ ,IL-1, IL-2, and IL-12 production (12, 21, 37). TGF- $beta$ playsan important role in the progression of infections including infectionswith Mycobacterium avium (11), Leishmania amazonensis (7),Leishmania braziliensis (6, 7), Trypanosoma cruzi (39),and Toxoplasma gondii (21). In contrast to these investigations,TGF- $beta$ plays a beneficial role in acquired resistance against Candidaalbicans (41) and Listeria monocytogenes (29) infection.

The aim of this study was to analyze the mechanisms of IL-12 exerted in Y. enterocolitica infections in different strainsof mice. For this purpose, we have used various mouse models includingYersinia-resistant C57BL/6 mice, Yersinia-susceptible BALB/c mice,Yersinia-intermediate-susceptible 129/Sv mice, and 129/Sv IFN- $gamma$ -receptor-deficient(IFN- $gamma$ R^/) mice, and C57BL/6 TNF receptor p55 chain-deficient (TNFR p55^/) mice to dissect the differential and ambiguous IL-12-mediatedmechanisms which cause either protection or exacerbation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Mice. Female, 6- to 8-week-old C57BL/6 and BALB/c mice were purchased from Charles River Wiga (Sulzfeld, Germany) and kept underspecific-pathogen-free conditions (positive-pressure cabinet).Female, 6- to 8-week-old 129/Sv/Ev IFN- $gamma$ receptor type II^+/+, 129/Sv/Ev IFN- $gamma$ receptor type II^/ mice (20), and C57BL/6 TNFR p55^/ (34) were bred under specific-pathogen-free conditions.

Infection of animals. Freshly thawed, plasmid-harboring Y. enterocolitica WA-314 serotype O:8 organisms suspended in 0.1 ml of sterile phosphate-bufferedsaline (PBS), pH 7.4, were used for intravenous and oral infectionas described previously (1). The actual number of bacteriaadministered was determined by plating serial dilutions of theinoculum on Mueller-Hinton agar and counting CFU after an incubationperiod of 36 h at 26°C. In kinetic studies, five mice per groupwere killed by carbon dioxide asphyxiation on days 1, 3, and 7postinfection (p.i.) with 5 × 10³ bacteria for both mouse strains if not otherwise stated. Thespleens were aseptically removed, and single-cell suspensionswere prepared by using 5 ml of PBS containing 0.1% bovine serumalbumin. Duplicates of 0.1 ml of serial dilutions of these preparationswere plated on Mueller-Hinton agar. The limit of detectable CFUwas 25 (log₁₀25 = 1.4). All animal experiments were repeated atleast three times and gave comparable results.

Abs. The Abs used in this study were anti-CD4 (GK1.5 [Dianova, Hamburg, Germany)] and YTS 191), anti-CD8 (53-6.7 [Dianova] andYTS 169), anti-CD3 (145 2C11), anti-IFN- $gamma$ (R4-6A2 and AN 18.17.24),anti-IL-4 (BVD6 24G2 [Pharmingen, San Diego, Calif.] and 11B11),anti-TNF- $alpha$ (MP6-XT22 [Pharmingen] and polyclonal anti-TNF- $alpha$ [Pharmingen]),polyclonal anti-asialo GM1 (Wako, Neuss, Germany), and EE5 (controlAb; kindly provided by W. Bohne, Würzburg, Germany). Abs werepurified from hybridoma supernatants by protein G-Sepharose 4Fast Flow (Pharmacia-LKB, Uppsala, Sweden) and fast-performanceliquid chromatography (Pharmacia-LKB), and then coupled to normalhuman serum-biotin (Sigma, Deisenhofen, Germany) or fluoresceinisothiocyanate (FITC) (Sigma) by standard methods (15).

Lymphocyte preparation. A part of the splenic single-cell suspensions described above was used for in vitro cultures. Erythrocytes were lysed by ashort incubation in 0.15 M NH₄Cl, washed three times with Hanksbalanced salt solution and resuspended in Click/RPMI 1640 cellculture medium (Biochrom, Berlin, Germany) supplemented with 2mM L-glutamine (Biochrom), 10 mM HEPES (Biochrom), 5 × 10⁵ M 2-mercaptoethanol (Biochrom), 10 µg of streptomycin (Biochrom)per ml, 100 U of penicillin (Biochrom) per ml, and 10% heat-inactivatedfetal calf serum (FCS) (Roth, Karlsruhe, Germany) at a final cellconcentration of 2 × 10⁶ per ml of Click/RPMI 1640 medium containing 10% FCS.

Cytokine assays. For determination of cytokine production, 2 × 10⁶ splenocytes were cultured in 2 ml of cell culture medium in 12-well macrocultureplates (Nunc, Roskilde, Denmark) in the presence of 10 µg of heat-killedyersiniae (HKY) per ml or 3 µg of concanavalin A (ConA) per ml.Cytokines were modulated by incubation with recombinant IL-12(kindly provided by M. Gately; 0.1 ng per ml of medium), and recombinantTGF- $beta$ 2 (kindly provided by G. Zenke, Sandoz Pharma-Ag, Basel,Switzerland, 1 to 4 ng per ml of medium). After 48 h, supernatantswere harvested and used in the cytokine assays.

(i) IFN- $gamma$ . IFN- $gamma$ levels were determined by using a capture enzyme-linked immunosorbent assay (ELISA) (3). Briefly, microtiter plates(Greiner, Solingen, Germany) were coated with anti-IFN- $gamma$ monoclonalantibody (MAb) (AN-18.17.24). After blocking of nonspecific bindingsites, supernatants were added to the wells and incubated overnight.After several wash steps, biotin-labeled anti-IFN- $gamma$ MAb (R4-6A2)was added. Finally, an avidin-biotin-alkaline phosphatase complex(Strept ABC-AP kit; DAKO, Glostrup, Denmark) was added. For signaldevelopment, the wells were incubated with p-nitrophenyl phosphatedisodium (Sigma), and the optical density was determined at wavelengthsof 405 and 490 nm with an ELISA reader. The levels of IFN- $gamma$ fromspleen cell cultures were calculated from the straight-line portionof the standard curve by using recombinant IFN- $gamma$ (1).

(ii) TNF- $alpha$ . TNF- $alpha$ levels were determined by using a capture ELISA including polyclonal rabbit anti-murine TNF- $alpha$ antiserum (Genzyme, Boston,Mass.) and biotin-labeled anti-TNF- $alpha$ MAb (Dianova) as describedabove for IFN- $gamma$ ELISA.

(iii) IL-4. IL-4 levels were determined by using a capture ELISA including anti-IL-4 MAb (BVD6 24G2) and biotin-labeled anti-IL-4 MAb(11B11) as described above for IFN- $gamma$ ELISA.

In vivo administration of Abs and cytokines. In various experiments, the course of infection was modulated by intraperitoneal (i.p.) administration of (i) human TGF- $beta$ 2(1 to 4 µg), (ii) recombinant murine IL-12 (20 to 100 ng) on days $-$ 1, 0, 1, 2, and 3 p.i., (iii) anti-CD4 (YTS 191), (iv) anti-CD8(YTS 169), and (v) anti-asialo GM1 on day $-$ 1 and day 3 p.i. Controlanimals were i.p. injected with the appropriate volume of PBScontaining control MAb or serum.

Flow cytometry. Success of T-cell depletion was confirmed by flow cytometry. Splenocytes were suspended in PBS containing 2% FCS and stainedwith one of the following MAbs: an FITC-conjugated anti-CD3 MAband phycoerythrin-conjugated anti-CD4 (GK1.5) and anti-CD8 (53-6.7)MAbs. Labeling procedures were conducted at 4°C. From each sample,10,000 cells were analyzed in a FACScan (Becton Dickinson, Heidelberg,Germany). Depletion efficiency was >95% after CD4 or CD8 T-celldepletion measured in the spleen after 3 and 7 days.

Cytotoxicity assays. Success of NK cell depletion was confirmed by cytotoxicity assays (8). YAC-1 cells (5 × 10⁶; American Type Culture Collection, Rockville, Md.) as targetcells were labeled with 200 µCi of Na[⁵¹Cr]O₄ by incubation for 1 h at 37°C, and then washed three timesin Click/RPMI-5% FCS. One hundred microliters of YAC-1 cells wasadded to each well in 96-well microtiter plates (Nunc) and incubatedfor 6 h at 37°C. Then, 25 µl of supernatant was harvested fromeach well and counted with a beta plate scintillation counter(Pharmacia-LKB). The percentage of specific ⁵¹Cr release was calculated by the following formula: [(experimentalrelease $-$ spontaneous release)/(maximum release $-$ spontaneousrelease)] × 100. Experimental release was obtained from wellsthat contained target and effector cells, and maximum releasewas obtained by resuspending target cells before harvesting. Valuesare the means of six wells. After NK cell depletion, no specificlysis was detectable when the effector/target ratio was 100:1.

Statistics. Differences between mean values were analyzed with Student's t test. A P value of <0.05 was considered statistically significant.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

What are the effector cells for IL-12-mediated protection against Y. enterocolitica? To evaluate which cell populations are the effectors for IL-12-mediated protection against Y. enterocolitica in BALB/c mice,CD4⁺ T cells, CD8⁺ T cells, or NK cells were depleted by administration of anti-CD4,anti-CD8, or anti-asialo GM1 Abs before and after infection withY. enterocolitica. Parallel groups of mice were additionally treatedwith 20 ng of IL-12. Bacterial numbers in spleens were determined7 days p.i. As depicted in Table 1, CD4⁺ T-cell depletion rendered BALB/c mice resistant against Y. enterocolitica(P < 0.001), whereas CD8⁺ T cell or NK cell depletion had no impact on the numbers of bacteriain spleens.

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TABLE 1. Modulation of Y. enterocolitica infection in BALB/c mice by administration of anti-CD4, anti-CD8, or anti-asialo GM1 Abs and IL-12^a

CD4⁺ T-cell depletion in IL-12-treated mice did not influence bacterial numbers in spleens compared to IL-12-treated controlmice (Table 1). In contrast, NK cell depletion partially abrogatedIL-12-mediated protection in Yersinia-infected BALB/c mice (P< 0.01). After CD8⁺ T-cell depletion of IL-12-treated BALB/c mice, there was alsoa slight increase in bacterial numbers in spleens (P < 0.05).Therefore, we conclude that NK cells and possibly CD8⁺ T cells are involved in IL-12-mediated protection in BALB/c mice.

In parallel experiments, spleen cells were stimulated with HKY, and production of IFN- $gamma$ and IL-4 was determined in cell culturesupernatants (Table 1). After stimulation with HKY, a slightdecrease in the IFN- $gamma$ level after NK or CD4⁺ T-cell depletion was observed. Administration of IL-12 in vivocaused only a marginal increase of IFN- $gamma$ in NK cell-depleted mice.Comparison of IFN- $gamma$ levels after ConA stimulation showed no significantdecrease after NK, CD8⁺, or CD4⁺ T-cell depletion. Likewise, after ConA stimulation, IFN- $gamma$ levelswere only slightly increased in IL-12-treated Yersinia-infectedcontrols and in IL-12-treated CD4⁺ T-cell- or NK-cell-depleted mice (Table 1). IL-4 productionwas detectable only after ConA stimulation and was reduced inIL-12-treated or CD4⁺ T-cell-depleted mice (P < 0.01), suggesting that IL-4 productioncould be involved in the inhibitory effect of CD4⁺ T cells on elimination of yersiniae (Table 1).

IL-12-activated CD8 T cells and NK cells are essential to protect against yersiniae in CD4 T-cell-depleted mice. To identify the effector cells for protection against yersiniae in CD4⁺ T-cell-depleted BALB/c mice, animals were treated with anti-CD4Abs prior to Yersinia infection and on day 3 p.i. with anti-CD4Abs in the presence or absence of anti-CD8 or anti-asialo GM1Abs. In addition, some groups of mice were treated with 20 ngof IL-12 each day. The results in Fig. 1 show that additionalCD8⁺ T-cell or NK cell depletion abrogated resistance mediated byCD4⁺ T-cell depletion (P < 0.001). These results indicate that bothCD8⁺ T and NK cells are essential for protection against yersiniaein CD4⁺ T-cell-depleted BALB/c mice. Abrogation of resistance in IL-12-treated,CD4⁺ T-cell-depleted mice was detected only in mice additionally depletedof both CD8⁺ T cells and NK cells, indicating that either of these two cellpopulations upon administration of IL-12 is sufficient to mediateprotection against yersiniosis.

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FIG. 1. Bacterial numbers in spleens of BALB/c mice 7 days p.i. with 2 × 10³ Y. enterocolitica and administration of PBS containing control Abs or anti-CD4 Abs 1 day prior to infection. On day +3 p.i., mice were treated with PBS containing control or anti-CD4 Abs without or in combination with anti-CD8, anti-asialo GM1 (NK), or anti-CD8 plus anti-asialo GM1 Abs. Results are the means and standard deviations for four mice. The asterisks indicate statistically significant differences (P < 0.01) compared with the values obtained with the control group (* for group of mice treated with anti-CD4 MAb alone; ** for group of mice treated with anti-CD4 MAb plus IL-12). w/o IL-12, without IL-12.

IL-12 has no protective effect against yersiniae in IFN- $gamma$ receptor knockout mice. Administration of anti-IFN- $gamma$ Abs in BALB/c mice abrogates IL-12-mediated protection against yersiniosis only partially (8).Therefore, we studied whether IL-12 can protect mice against yersiniaein an IFN- $gamma$ -independent manner. 129/Sv IFN- $gamma$ R^+/+ and 129/Sv IFN- $gamma$ R^/ mice were infected with Y. enterocolitica, and bacterial countsin the spleen were determined 5 days p.i. As shown in Table 2,yersinia-infected IFN- $gamma$ R^/ mice had significant higher bacterial counts in the spleen 5days p.i. than the wild-type mice did, indicating that IFN- $gamma$ R^/ mice are much more susceptible to Yersinia infection than wild-typemice are. The results of these experiments confirmed previousdata that IFN- $gamma$ is essential for clearance of Yersinia infection(8).

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TABLE 2. Bacterial numbers in the spleens of IFN- $gamma$ R^/ and IFN- $gamma$ R^+/+ mice^a

To study the effect of IL-12 on the course of Yersinia infection in IFN- $gamma$ R^/ and IFN- $gamma$ R^+/+ mice, these mice were treated with PBS or IL-12 prior to andafter Yersinia infection, and bacterial counts in spleens weredetermined on day 5 p.i. Administration of IL-12 rendered IFN- $gamma$ R^+/+ mice resistant to infection, while IL-12 treatment had no impacton yersiniosis in IFN- $gamma$ R^/ mice (Fig. 2). These results suggest that IL-12 is not able toprotect against yersiniae in the absence of IFN- $gamma$ -induced mechanisms.In parallel experiments, spleen cells of infected mice were isolatedand exposed to HKY in vitro, and IFN- $gamma$ and IL-4 levels were determinedin cell culture supernatants. The results show that both IFN- $gamma$ R^+/+ and IFN- $gamma$ R^/ mice produced comparable IFN- $gamma$ levels (Fig. 2). In vivo administrationof IL-12 slightly increased IFN- $gamma$ production in both mouse strains,suggesting that IL-12 may be partially involved in the amplificationcascade leading to IFN- $gamma$ production. However, we found no evidencethat IL-4 is upregulated in IFN- $gamma$ R^/ mice, because IL-4 levels were not detectable in HKY- or ConA-stimulatedspleen cells of either in vivo untreated or IL-12-treated IFN- $gamma$ R^+/+ or IFN- $gamma$ R^/ mice (data not shown).

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FIG. 2. Bacterial numbers (A) and IFN- $gamma$ production (B) in the spleen cells from Yersinia-infected (day 5 p.i.) 129/Sv IFN- $gamma$ R^+/+ (2 × 10⁴ Y. enterocolitica) or 129/Sv IFN- $gamma$ R^/ mice (2 × 10² Y. enterocolitica) treated with PBS or 20 ng of IL-12 each day. Spleen cells were stimulated with HKY (10 µg per ml). Results are the means and standard deviations for four mice. The asterisk indicates a statistically significant difference (P < 0.01) compared with the values obtained with the control group.

Modulation of Yersinia infection by TGF- $beta$ . C57BL/6 mice produce high levels of IFN- $gamma$ dependent on endogenous IL-12 production, which in this particular case correlateswith higher resistance against Yersinia compared to BALB/c mice.Treatment with exogenous IL-12, however, is toxic in C57BL/6 mice.We therefore tested whether TGF- $beta$ might influence IL-12-triggeredexacerbation of yersiniosis.

To determine whether TGF- $beta$ alters production of cytokines in Yersinia infection, spleen cells from Yersinia-infected C57BL/6mice were stimulated with HKY in the presence of TGF- $beta$ and productionof IFN- $gamma$ and TNF- $alpha$ was determined in culture supernatants. TGF- $beta$ reduced IFN- $gamma$ and TNF- $alpha$ levels in a dose-dependent manner (Fig.3). Therefore, we hypothesized that administration of TGF- $beta$ mightexacerbate yersiniosis. Both C57BL/6 and BALB/c mice were treatedwith various amounts of TGF- $beta$ prior to and after Y. enterocoliticainfection. Administration of 1 µg of TGF- $beta$ each day decreasedbacterial numbers (P < 0.01) in Yersinia-infected C57BL/6 mice,while administration of 4 µg of TGF- $beta$ (data not shown) had noeffect on clearance of yersinae (Fig. 4). TGF- $beta$ treatment hadno impact on the numbers of bacteria in BALB/c mice.

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FIG. 3. TGF- $beta$ -modulated IFN- $gamma$ and TNF- $alpha$ production by HKY-stimulated spleen cells from C57BL/6 mice prepared 3 and 7 days p.i. with 5 × 10³ Y. enterocolitica. Results are the means and standard deviations for three mice.

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FIG. 4. Bacterial numbers in the spleen from C57BL/6 and BALB/c mice 5 days after infection with 2 × 10⁴ or 2 × 10³ Y. enterocolitica, respectively, and i.p. administration of PBS or 1 µg of TGF- $beta$ 2 on days $-$ 1, 0, +1, +2, and +3 p.i. The results are the means and standard deviations for four mice. The asterisk indicates a statistically significant difference (P < 0.01) compared with the values obtained with the control group.

To test whether TGF- $beta$ can modulate toxicity of IL-12, C57BL/6 mice were treated with TGF- $beta$ plus IL-12 prior to and after Yersiniainfection. As shown in Fig. 5A, the combination of IL-12 and TGF- $beta$ decreased bacterial numbers (P < 0.001) compared to PBS and IL-12treatments in mice. In parallel experiments, spleen cells wereisolated and exposed to HKY and production of TNF- $alpha$ and IFN- $gamma$ was determined (Fig. 5B and C). HKY-stimulated spleen cells ofIL-12-treated Yersinia-resistant mice produced significant higherTNF- $alpha$ levels (Fig. 5B) than those of control mice (P < 0.001),while IL-12 treatment had no significant impact on IFN- $gamma$ production(Fig. 5C). TGF- $beta$ treatment in the presence or absence of IL-12in vivo led to decreased TNF- $alpha$ and IFN- $gamma$ levels compared to thoseof control mice (P < 0.001). These results suggest that IL-12-mediatedtoxic effects could be due to increased TNF- $alpha$ levels and thatthe protective effects of IL-12 can be restored in C57BL/6 miceby TGF- $beta$ , possibly via a moderate downregulation of TNF- $alpha$ production.

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FIG. 5. Bacterial numbers in the spleen (A) and TNF- $alpha$ (B) and IFN- $gamma$ production (C) by spleen cells from C57BL/6 mice 5 days after infection with 2 × 10⁴ Y. enterocolitica and i.p. administration of PBS or 1 µg of TGF- $beta$ 2 on days $-$ 1, 0, +1, +2, and +3 p.i. with (+) or without (w/o) the addition of 100 ng of IL-12 on days $-$ 1, 0, +1, +2, and +3 p.i. (A). Spleen cells were stimulated with HKY (10 µg per ml), and the presence of IFN- $gamma$ (B) and TNF- $alpha$ (C) in cell culture supernatants was determined. The results are the means and standard deviations for four mice. The asterisks indicate statistically significant differences (P < 0.01) compared with the values obtained with the control group.

TNF- $alpha$ accounts for IL-12-mediated toxicity in yersiniosis. To investigate whether TNF- $alpha$ is involved in IL-12-mediated exacerbation of Yersinia infection in C57BL/6 mice, TNFR p55^/ mice were used. C57BL/6 TNFR p55^/ and TNFR p55^+/+ mice were treated with PBS or IL-12 before and after infectionwith yersiniae. As indicated in Fig. 6, bacterial numbers in thespleens of Yersinia-infected TNFR p55^/ mice were more than 1,000-fold higher than in the spleens ofTNFR p55^+/+ mice, even when hundredfold-less yersiniae were used to infectTNFR p55^/ mice. These data show that TNFR-mediated mechanisms are essentialfor clearance of Yersinia infection. Consequently, both TNFR p55^+/+ and TNFR p55^/ mice were treated with IL-12 before and after Yersinia infection.IL-12 increased bacterial numbers in the spleens of Yersinia-infectedTNFR p55^+/+ mice. In contrast, IL-12 treatment slightly decreased (P < 0.01)bacterial numbers in the spleen of Yersinia-infected TNFR p55^/ mice (Fig. 6A), suggesting that TNFR-mediated mechanisms areinvolved in the toxic effects of IL-12 in Yersinia-infected C57BL/6mice.

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FIG. 6. Bacterial numbers in the spleen (A), and IFN- $gamma$ production by spleen cells (B) from C57BL/6 TNFR p55^+/+ and C57BL/6 TNFR p55^/ mice 5 days after infection with 2 × 10⁴ or 2 × 10² Y. enterocolitica, respectively, and i.p. administration of PBS or 1 µg of IL-12 on days $-$ 1, 0, +1, +2, and +3 p.i. The asterisks indicate statistically significant differences (P < 0.01) compared with the values obtained with the control group.

In parallel experiments, spleen cells were isolated and exposed to HKY, and production of IFN- $gamma$ was determined (Fig. 6B).HKY-stimulated spleen cells derived from PBS-treated Yersinia-infectedTNFR p55^/ mice produced only low levels of IFN- $gamma$ compared to wild-typemice. IFN- $gamma$ production of HKY stimulated spleen cells derivedfrom TNFR p55^/ mice was partially restored by IL-12 treatment in vivo.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

TNF- $alpha$ , IL-12, and IFN- $gamma$ are essential for clearance of Yersinia infection (1, 8, 35). Comparison of Yersinia-resistantC57BL/6 and Yersinia-susceptible BALB/c mice revealed that thetwo mouse strains differ in their ability to produce IFN- $gamma$ (8,35). BALB/c mice are IFN- $gamma$ low producers, while C57BL/6 miceare IFN- $gamma$ high producers. Furthermore, BALB/c and C57BL/6 micehave different responses to the administration of IL-12 (8).Thus, IL-12 confers protection against yersiniae in susceptibleBALB/c mice but exacerbates yersiniosis and toxicity in resistantC57BL/6 mice. Extending these studies, we wanted to dissect themechanisms of the ambiguous IL-12 effects in different mouse strains.

CD4⁺ T cells play a crucial but ambiguous role for clearance of Yersinia infection. Thus, CD4⁺ T cells promote clearance of Y. enterocolitica in C57BL/6 mice(8) but promote exacerbation of Yersinia infection in BALB/cmice. In line with these data, previous studies showed that depletionof CD4⁺ T cells improved resistance of BALB/c mice against Leishmania(26, 27). Depletion of NK cells or CD8⁺ T cells had no impact on clearance of Yersinia infection in BALB/cmice. However, we showed that both CD8⁺ T and NK cells are crucial for clearance of Yersinia infectionin CD4⁺ T-cell-depleted BALB/c mice, suggesting that CD4⁺ T cells may inhibit both CD8⁺ T and NK cells in their potential ability to eliminate yersinae.

To identify the effector cells for IL-12-mediated protection against yersinae, BALB/c mice were simultaneously treated withIL-12 and antibodies against different cell populations. Theseexperiments showed that CD8⁺ T-cell and NK cell depletion increased bacterial numbers in Yersinia-infectedIL-12-treated BALB/c mice, indicating that in these mice, CD8⁺ T or NK cells may be sufficient to control Yersinia infection,probably in concert with remaining cell populations like macrophages.

In C57BL/6 mice, there is a clear-cut correlation of IL-12-dependent IFN- $gamma$ production of NK cells (early phase of infection)or CD4 T cells (late phase) and clearance of Yersinia. In contrast,CD4 T-cell depletion or IL-12 mediates protection but does notincrease IFN- $gamma$ production in BALB/c mice. In experimental leishmaniasis,CD4 T-cell depletion caused a decrease in the frequency of IL-4-secretingT-cell clones without a concomitant increase of IFN- $gamma$ -secretingT-cell clones (26). Likewise, HKY-stimulated spleen cells ofCD4 T-cell-depleted Yersinia-infected BALB/c mice showed no significantincrease of IFN- $gamma$ production compared to control mice. In contrastto leishmaniasis, no significant levels of IL-4 were found inyersiniosis. However, after ConA stimulation, no significant differencesin IFN- $gamma$ levels after depletion of CD4 T cells, CD8 T cells, orNK cells were observed, whereas IL-4 production was significantlydecreased after CD4 T-cell depletion or IL-12 administration.These results suggest that IL-4 produced by CD4 T cells mightbe involved in promoting Yersinia susceptibility of BALB/c mice.In keeping with this assumption, in both Yersinia and Leishmaniainfections, administration of anti-IL-4 Abs rendered BALB/c miceresistant (1, 18). These data suggest that although IFN- $gamma$ is crucial for IL-12-mediated protection, alternative mechanismsseem to be involved in clearance of Yersinia infection.

Previous work showed that the protective effect of IL-12 in BALB/c mice can be only partially abrogated by the addition ofanti-IFN- $gamma$ Abs, suggesting that IL-12 might cause protective effectsin an IFN- $gamma$ -independent manner (8). Herein we show that IFN- $gamma$ R-deficientmice are more susceptible to Yersinia infection than wild-typemice. Similar results were demonstrated in other infection models(10, 20, 22). Administration of IL-12 increased resistanceagainst yersinae in IFN- $gamma$ -R^+/+ but not in IFN- $gamma$ R^/ mice. These data confirm that IFN- $gamma$ is essential for clearanceof Yersinia infection and suggest that IL-12 has no protectiveeffect in the absence of IFN- $gamma$ R-mediated mechanisms. On the otherhand, we cannot yet exclude the possibility that the lack of IFN- $gamma$ Rin knockout mice might have affected the development of the immunesystem per se.

Yersinia-triggered IFN- $gamma$ production was only slightly affected in IFN- $gamma$ R^/ mice compared to wild-type mice, indicating that initial upregulationof IFN- $gamma$ is not affected by IFN- $gamma$ R-mediated mechanisms. This resultis in keeping with reports demonstrating that IFN- $gamma$ ^/ mice produce IL-12 during murine endotoxemia and show highersusceptibility to Mycobacterium bovis (10). Since IFN- $gamma$ seemsto be essential for upregulation of IL-12R $beta$ ₂ expression, IFN- $gamma$ Rdeficiency may also cause a low IL-12R $beta$ ₂ expression on T cells,leading to IL-12 unresponsiveness (44) and thereby inhibitingeffector mechanisms mediated directly by IL-12. However, it isnot yet clear whether IFN- $gamma$ is required for both initial mechanismsinducing anti-Yersinia host responses and for the resulting effectormechanisms leading to resolution of Y. enterocolitica infection.

A virus infection model revealed that TNF- $alpha$ accounts for IL-12-induced toxicity (31). As IL-12 triggers toxicity and exacerbatesyersiniosis in C57BL/6 mice, the course of Yersinia infectionin C57BL/6 TNFR p55^/ mice was investigated and revealed that IL-12-triggered toxicitywas not observed in the absence of TNFR. Moreover, bacterial numberswere slightly decreased in IL-12-treated TNFR p55^/ mice, suggesting that TNF- $alpha$ is involved in IL-12-triggered toxicityin yersiniosis. Nevertheless, IL-12 had only a slight beneficialeffect on Yersinia infection in TNFR p55^/ mice, probably because TNF- $alpha$ is crucial for clearance of Yersiniainfection (4). Moreover, as mentioned above, it should be consideredthat the lymphoid organogenesis is altered in TNFR p55^/ mice (25) and that this fact might partially account for theresults obtained in this study.

In Leishmania infection, CD4 T-cell depletion elevated tissue expression of inducible nitric oxide synthetase (iNOS) in susceptibleBALB/c mice to a level comparable with resistant C57BL/6 mice(42). Furthermore, it was suggested that the relative lack ofiNOS in susceptible mice could be due to a higher expression ofTGF- $beta$ in tissues of susceptible mice than in resistant mice (42).In this study, we found that TGF- $beta$ improved resistance againstyersiniae in C57BL/6 mice but had no impact on the course of infectionin BALB/c mice. Administration of IL-12 plus TGF- $beta$ rendered C57BL/6mice more resistant to Yersinia infection and abrogated toxiceffects of IL-12.

It was recently shown that TNF- $alpha$ in synergism with IL-2 is essential for triggering IL-12-induced toxicity (14, 31-33). Likewise,administration of IL-12 led to increased TNF- $alpha$ levels in HKY-stimulatedspleen cells from Yersinia-infected C57BL/6 mice. TGF- $beta$ had anopposing effect to IL-12 by moderate downregulation of TNF- $alpha$ production,suggesting that in Yersinia-resistant C57BL/6 mice which inducea strong Th1 response, there might be a deficit of negative immunoregulatorymechanisms. Therefore, we speculate that both IL-12-induced toxicitymediated by TNF- $alpha$ and IL-12-induced protection mediated by IFN- $gamma$ may be balanced by TGF- $beta$ , which seems to be critical to obtainan optimal immune response against yersinae.

The immunoregulatory role of TGF- $beta$ , however, is not yet clear. Contradictory data on TGF- $beta$ -mediated Th1 responses have beenreported, indicating that TGF- $beta$ stimulates (13, 28, 43)or downregulates Th1 development (19, 46). TGF- $beta$ with or withoutcombination of IL-12 decreases IFN- $gamma$ production by CD4⁺ T cells from C57BL/6 or BALB/c mice but increases IFN- $gamma$ productionby CD4⁺ T cells from CBA/J and C3H/He mice (19).

There are also contradictory reports about the role of TGF- $beta$ in infections. TGF- $beta$ promotes infection in L. braziliensis (6)and T. gondii (21) in correlation with downregulation of IFN- $gamma$ (6, 21) and upregulation of IL-4 and IL-10 (6). Moreover,in T. gondii infection, TGF- $beta$ counteracts IL-12 protective effectin mice with severe combined immunodeficiency disorder (21).On the other hand, TGF- $beta$ plays a beneficial role in resistanceagainst C. albicans (41) and L. monocytogenes (29) by upregulatingIL-4 and IL-10 production (41) and downregulating IFN- $gamma$ , TNF- $alpha$ ,and IL-6 production (29). Thus, TGF- $beta$ -mediated downregulationof various cytokines correlates with either resolution or excerbationof infections, suggesting that balancing of certain cytokine productionlevels is decisive for the outcome in different infectious diseases.

Taken together, cytokine regulation of effector mechanisms leading either to CD4⁺ T cells promoting or suppressing immune responses against Yersiniaplay a central role in the different abilities of C57BL/6 andBALB/c mice to clear Yersinia infection. These data are importantfor understanding the critical balance of proinflammatory andregulatory cytokines during bacterial infections which is decisivefor beneficial effects of cytokine therapy.

	ACKNOWLEDGMENTS

We are grateful to K. Pfeffer (Technical University of Munich, Munich, Germany) for providing TNFR p55 knockout mice, M. Gately(Hoffmann-LaRoch Inc., Nutley, New Jersey) for generously providingus with IL-12, G. Zenke (NOVARTIS, Pharma-AG, Basel, Switzerland)for generously providing us with TGF- $beta$ 2, and S. Preger and N.Bücheler for expert technical assistance.

	FOOTNOTES

^* Corresponding author. Mailing address: Max-von-Pettenkofer-Institute, Ludwig-Maximilians-University, Pettenkoferstrasse 9a,D-80336, Munich, Germany. Phone: 49-89-5160-5280. Fax: 49-89-5380-584.E-mail: Autenrieth{at}m3401.mpk.med.uni-muenchen.de.

Editor: J. R. McGhee

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