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Involvement of Dectin-2 in Ultraviolet Radiation-Induced Tolerance ¹

Yoshinori Aragane^2,*, Akira Maeda^*,, Agatha Schwarz, Tadashi Tezuka^*, Kiyoshi Ariizumi and Thomas Schwarz

^* Department of Dermatology, Kinki University School of Medicine, Osaka, Japan; Department of Dermatology, Southwestern Medical Center, University of Texas, Dallas, TX 75390; and Department of Dermatology, University of Münster, Münster, Germany

	Abstract

Top Abstract Introduction Materials and Methods Results and Discussion References

 
Hapten sensitization through UV-exposed skin induces hapten-specific tolerance which can be adoptively transferred by injecting T cells into naive recipients. The exact phenotype of the regulatory T cells responsible for inhibiting the immune response and their mode of action remain largely unclear. Dectin-2 is a C-type lectin receptor expressed on APCs. It was postulated that dectin-2 interacts with its putative ligands on T cells and that the interaction may deliver costimulatory signals in naive T cells. Using a soluble fusion protein of dectin-2 (sDec2) which should inhibit this interaction, we studied the effect on contact hypersensitivity (CHS) and its modulation by UV radiation. Injection of sDec2 affected neither the induction nor the elicitation phase of CHS. In contrast, UV-induced inhibition of the CHS induction was prevented upon injection of sDec2. In addition, hapten-specific tolerance did not develop. Even more importantly, injection of sDec2 into tolerized mice rendered the recipients susceptible to the specific hapten, indicating that sDec2 can break established tolerance. FACS analysis of spleen and lymph node cells revealed a significantly increased portion of sDec2-binding T cells in UV-tolerized mice. Furthermore, transfer of UV-mediated suppression was lost upon depletion of the sDec2-positive T cells. Taken together, these data indicate that dectin-2 and its yet unidentified ligand may play a crucial role in the mediation of UV-induced immunosuppression. Moreover, sDec2-reactive T cells appear to represent the regulatory T cells responsible for mediating UV-induced tolerance.

	Introduction

Top Abstract Introduction Materials and Methods Results and Discussion References

 
Ultraviolet radiation is one of the, if not the most, significant environmental factors affecting humans. Besides its well-known beneficial and indispensable effects for human life, UV, in particular the middle wave length range (290–320 nm, UVB), can be a hazard to human health by inducing skin cancer, premature skin aging, inflammation, and cell death (1, 2, 3, 4). In addition, UV exhibits immunosuppressive properties which may be relevant for photocarcinogenesis and the exacerbation of infectious diseases following UV exposure (5, 6). The immunosuppressive properties of UV are best illustrated by the inhibition of cellular immune reactions, such as contact hypersensitivity (CHS)³ (7, 8). Epicutaneous sensitization in mice is impaired when the hapten is applied onto skin which has been exposed to UV immediately before (7). In addition to the failure to generate hapten sensitization, tolerance develops because mice treated in this way cannot be resensitized against the same hapten at a later time point (7). UV-induced tolerance appears to be hapten-specific because the sensitization against other nonrelated haptens is not affected (7). Hapten-specific unresponsiveness can be adoptively transferred; injection of lymph node cells and splenocytes from UV-tolerized mice into syngeneic naive mice inhibits sensitization against the relevant hapten in the recipients (9). Consequently, it has been suggested that UV-induced tolerance is mediated via the induction of hapten-specific T suppressor cells, now renamed regulatory T cells (reviewed in Ref. 10). Although the cellular transfer of suppression and the hapten specificity were convincingly demonstrated almost two decades ago, the cells transferring hapten-specific unresponsiveness are still poorly characterized and their mode of action is unclear in major parts.

Using a subtractive cDNA cloning strategy, we previously isolated genes encoding for C-type lectin receptors (termed dectin-1 and dectin-2); dectin-1 is expressed by dendritic cells and macrophages (11). Preliminary in vitro data showed that a soluble receptor of dectin-1 binds to the cell surface of T cells, thereby delivering T cell costimulatory signals (11). Recently, dectin-1 was reported to bind to -glucan, a polysaccharide synthesized in yeasts in an opsonin-independent fashion, indicating that dectin-1 is a pattern recognition receptor (12, 13). This ligand does not block binding of dectin-1 to T cells (12). Thus, dectin-1 has been well-characterized.

Dectin-2 is also a C-type lectin receptor with a type II configuration, consisting of, from the N terminus, a short cytoplasmic domain, a transmembrane domain, and an extracellular domain that contains a neck domain and a single carbohydrate recognition domain in the C terminus (14). Unlike dectin-1, dectin-2 expression appears more restricted to dendritic cells including epidermal dendritic cells (Langerhans cells); using a transgenic mouse bearing a dectin-2 promoter-driven luciferase gene, Bonkobara et al. (15) found the highest luciferase activity in the skin, lower levels in spleen, lymph node, and thymus and only background levels in nonlymphoid organs. Despite having a perfect C-type lectin motif, responsible for recognition of carbohydrates, the ligand for dectin-2 has not yet been identified and even its carbohydrate recognition has not been proven. Accordingly, the function of dectin-2 still remains to be determined.

To study the function of dectin-2, we have prepared a soluble dectin-2 receptor in the format of histidine-fusion proteins, consisting of the extracellular domains (aa 43–209) of dectin-2. This soluble dectin-2 (sDec2) should bind to the putative ligand and thus presumably inhibit dectin-2-triggered stimulation. We used this soluble receptor protein to examine whether dectin-2 is involved in the mediation of CHS. Surprisingly, injection of sDec2 affected neither the induction nor the elicitation of CHS, but blocked UV-induced suppression of CHS. Even more importantly, injection of sDec2 was able to break established tolerance. T cells transferring suppression were found to bind sDec2. Depletion of the sDec2-binding fraction of T cells was associated with a loss of transfer of suppression. Taken together, these data indicate that dectin-2 and its yet unidentified ligand may play a crucial role in the mediation of UV-induced immunosuppression. In addition, sDec2 may be a useful tool to further characterize the regulatory T cells mediating UV-induced tolerance.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results and Discussion References

 
Reagents

Recombinant soluble protein of dectin-2 (sDec2) was generated from an expression vector encoding for 6xHis-tagged extracellular domain of dectin-2 (aa 43–209) as described previously (14). Recombinant soluble protein of dihydrofolate reductatse (DHFR) was derived from 6xHis-tagged DHFR and used as a control protein. Both proteins were expressed in Escherichia coli M15 and purified by using a Ni-NTA resin (Life Technologies, Grand Island, NY) followed by refolding.

Contact hypersensitivity

C3H/HeN mice (8- to 10-wk-old) were obtained from Japan Clea (Hamamatsu, Japan). Mice were sensitized on day 0 by painting 25 µl of 0.5% 2,4-dinitrofluorobenzene (DNFB; solved in acetone-olive oil, 4:1) onto the shaved back. After 5 days, mice were challenged by painting 20 µl of 0.3% DNFB onto the left ear. The right ear was painted with the acetone-olive oil solution without DNFB. Ear swelling was quantified 24 h later using a spring-loaded micrometer. CHS was determined as the amount of swelling of the hapten-challenged ear compared with the thickness of the vehicle-treated ear in sensitized animals and expressed in millimeters x 10^-2 (mean ± SD). After 2 wk, mice were resensitized through nonirradiated abdominal skin and challenged on the right ear after 5 days. Each group consisted of at least seven mice. Data were analyzed by Student’s t test, and differences were considered as significant at p < 0.05.

UV irradiation

Mice were exposed to 1000 J/m² UV on the shaved back daily for 4 consecutive days. FS-20 fluorescent lamps (Westinghouse Electric, Pittsburgh, PA) which emit most of their energy within the UVB range (290–320 nm) with an emission peak at 311 nm were used. DNFB was applied onto the surface of the irradiated skin area 24 h after the last UV exposure.

Adoptive transfer

Donor mice were exposed to UV and sensitized with DNFB through UV-exposed skin as described above. Five days after sensitization, spleens and regional lymph nodes were removed, and single cell suspensions were prepared. T cells were prepared by passing the cell suspension through a nylon wool column twice, which yields 95% pure T cells as measured by FACS analysis using Abs directed against T cell markers (Thy 1.2, CD3). The cell number was adjusted to 1 x 10⁸ cells/ml, and 200 µl were injected i.v. into naive recipient mice. Recipients were sensitized 24 h later by epicutaneous application of DNFB on the shaved abdomen. After 5 days, mice were challenged on the left ear and ear swelling was evaluated 24 h later. For control purposes, identical numbers of cells obtained from untreated or DNFB-sensitized mice were injected.

Depletion and enrichment of T cell subpopulations

Lymphocytes obtained from regional lymph nodes and spleens were incubated in nylon wool columns. T cells were first reacted with biotinylated-sDec2, -DHFR, or -sDec2 which was boiled. Biotinylation was conducted by use of the ECL Protein Biotinylation Module (Amersham Biosciences, Buckinghamshire, U.K.). One hour after the incubation of the cells with the biotinylated proteins, cells were incubated with streptavidin-coupled magnetic beads for 30 min. Magnetoseparation was performed by placing the tubes into a magnetic field (Dynal, Oslo, Norway) for 4 min. The supernatants containing the cells not binding to sDec2 were removed. Cells were washed and used for i.v. injection. Cells bound to the magnetobeads were detached by incubating cells overnight in cell culture medium at 37°C in a humidified atmosphere containing 5% CO₂. Magnetobeads which had spontaneously detached from the cells after overnight incubation were removed with a magnet. The remaining (dectin-2 binding) cells were harvested, washed, and adjusted to 2.5 x 10⁷ cells/ml for i.v. injection (200 µl/mouse). The efficacy of separation was determined by flow cytometry (FACSCalibur; BD Biosciences, Mountain View, CA).

Flow cytometry

T cells prepared from superficial regional lymph nodes and spleens were first incubated in PBS supplemented with 1% BSA on ice for 30 min. After extensive washing in PBS/BSA, T cells were incubated with biotinylated sDec2 on ice for 1 h. To perform competition of the binding, boiled sDec2, DHFR, and sDec2 were added to the reaction as a nonspecific and a specific competitor, respectively. After extensive washing in PBS/BSA, the samples were reacted with streptavidin-coupled with FITC on ice for 15 min. After washing, the samples were analyzed by flow cytometry (FACSCalibur). In some experiments, three-color staining was conducted with an allophycocyanin-conjugated Ab directed against CD4 (clone RM4-5; BD Biosciences, San Diego, CA), with a PE-conjugated Ab directed against CD25 (clone 7D4; BD Biosciences), and with biotinylated sDec2, which was finally reacted with FITC-coupled streptavidin (BD Biosciences).

Cytokine induction in vitro

T lymphocytes were prepared from mice which were tolerized by applying DNFB onto UV-irradiated skin and separated into sDec2⁺ and sDec2^- fractions by magnetobead separation. T cells (5 x 10⁶/ml) were incubated with dendritic cells (1 x 10⁶/ml) which were isolated from bone marrow of syngeneic naive mice as described previously (16). Coincubations were performed in the absence or presence of the water soluble DNFB analog 2,4-dinitrobenzene-sulfonic sodium salt (DNBS, 0.1 mM). Supernatants were collected 48 h after stimulation and tested for the amounts of IL-4, IL-10, IFN-, and TGF- using ELISAs (Bender Medsystems, Vienna, Austria).

	Results and Discussion

Top Abstract Introduction Materials and Methods Results and Discussion References

 
Injection of sDec-2 does not affect CHS but inhibits UV-induced suppression of CHS

To elucidate whether interaction of dectin-2 with its putative ligand is of relevance in the generation of CHS, sDec2 was used. The soluble form of dectin-2 should bind to the putative though yet unknown ligand, inhibit the interaction of dectin-2 and therefore act as an antagonist of dectin-2. To test whether dectin-2 is involved in the mediation of CHS, mice received an i.v. injection of 50 µg of sDec2 or of DHFR. Three hours later, the animals were sensitized against DNFB. The ear swelling response caused by the ear challenge performed 5 days later was not affected by the injection of sDec-2 (data not shown). Likewise, ear challenge was not altered when sDec2 was injected i.v. into sensitized mice 3 h before challenge (data not shown). These data suggest that dectin-2 does not play an important role either in the induction or in the elicitation of CHS.

UV radiation is well known to inhibit the induction of CHS and to induce hapten-specific tolerance, although the detailed underlying mechanisms still remain to be determined. Therefore, we were interested in whether interaction of dectin-2 is involved in UV-induced immunosuppression. For that purpose, mice were sensitized against DNFB by epicutaneous application of the hapten on UV-exposed or unirradiated back skin. Ear challenge was performed 5 days later. In accordance with previous observations, ear swelling response was significantly suppressed in mice which were sensitized through UV-exposed skin (Fig. 1). To test whether dectin-2 is involved in UV-induced immunosuppression, mice were injected i.v. with various amounts of sDec2 3 h before application of DNFB onto UV-exposed skin. Mice which received 50 µg of sDec2 mounted an ear swelling response upon challenge comparable to that of positive control mice, despite the fact that sensitization was performed in UV-exposed skin (Fig. 1). sDec2 prevented UV-induced immunosuppression in a dose-dependent manner. Injection of 50 µg of the control protein DHFR did not affect inhibition of the induction of CHS by UV. Together, these data demonstrate that i.v. injection of sDec2 prevents UV-induced suppression of CHS, suggesting that interaction of dectin-2 with its putative ligand may play an important role in UV-induced immunosuppression.

View larger version (21K): [in this window] [in a new window]   FIGURE 1. sDec2 prevents UV-induced immunosuppression. C3H/HeN mice were sensitized on day 0 by painting 25 µl of 0.5% DNFB onto the shaved back which was exposed to UV or sham-treated. Five days later, mice were challenged by painting 20 µl of 0.3% DNFB onto the left ear. Ear swelling was quantified 24 h later. To evaluate the involvement of dectin-2 in this process, various amounts of sDec2 or DHFR were injected 3 h before sensitization. CHS was determined as the amount of swelling of the hapten-challenged ear compared with the thickness of the vehicle-treated ear in sensitized animals and expressed in millimeters x 10-2 (mean ± SD). *, p < 0.05; **, p < 0.01.

Application of haptens onto UV-exposed skin does not only result in the failure to induce a CHS response, but also induces long-term immunosuppression because the respective mice cannot be sensitized at a later time against the specific hapten. This tolerance is hapten-specific because the animals can be sensitized at later time points against other unrelated haptens (7). Because both impairment of CHS and induction of hapten-specific tolerance are caused by the identical procedure, i.e., sensitization through UV-exposed skin, it was postulated for quite a long time that the same mechanisms are involved and that induction of tolerance is the direct consequence of the inhibition of CHS induction. However, there is accumulating evidence that the molecular basis of UV-induced tolerance is different from the mechanism responsible for UV-impaired induction of CHS (17). Whereas a key event in the suppression of CHS by UV appears to be the depletion of Langerhans cells from the epidermis (7, 18), hapten-specific tolerance seems to be due to the generation of T suppressor cells (reviewed in Refs. 10 and 19).

Therefore, we next checked whether injection of sDec2 also prevents UV-mediated tolerance. For this purpose, the mice which were sensitized through UV-exposed skin after injection of sDec2 were resensitized with DNFB on the abdomen 2 wk after the first sensitization. Five days after resensitization, the second challenge was performed on the right ear. There was no difference in the ear swelling response between sensitized mice and UV-exposed mice which had initially received sDec2 i.v. (Fig. 2). In contrast, mice which were sensitized through UV-exposed skin but had not received sDec2 were unresponsive to resensitization, indicating that tolerance had developed. Taken together, these data demonstrate that injection of sDec2 prevents the UV-induced inhibition of sensitization and the development of UV-induced tolerance.

View larger version (24K): [in this window] [in a new window]   FIGURE 2. sDec2 prevents UV-induced tolerance. The UV-exposed mice which were untreated or had received 50 µg of sDec2 or DHFR before sensitization (shown in Fig. 1) were resensitized with DNFB applied on non-UV-exposed abdominal skin 2 wk after first challenge. Challenge on the right ear was performed 5 days after resensitization. *, p < 0.01.

We next were interested in whether injection of sDec2 is not only able to prevent the development of UV-induced tolerance but can also break tolerance once developed. To address this issue, mice were tolerized against DNFB by painting the hapten onto UV-exposed back skin. As demonstrated above, this procedure induces tolerance because these animals cannot be resensitized against DNFB 2 wk later. In one group of mice, sDec2 was injected i.v. before resensitization, while the other group received DHFR. Mice which were injected with DHFR did not show an ear swelling response after resensitization, indicating development of tolerance against DNFB (Fig. 3). In contrast, mice which received an i.v. injection of 50 µg of sDec2 revealed a specific ear swelling response after resensitization. Because tolerance had already developed at the time of injection of sDec2, one can conclude that injection of sDec2 is able to break established tolerance.

View larger version (21K): [in this window] [in a new window]   FIGURE 3. sDec2 breaks UV-induced tolerance. Mice were tolerized by application of DNFB onto UV-exposed skin. Two weeks after tolerization, mice were resensitized with DNFB applied on non-UV-exposed abdominal skin. Mice were left untreated or received an i.v. injection of 50 µg of sDec2 or DFHR 3 h before resensitization. Five days later challenge was performed on the right ear. Mice which were sensitized without UV exposure served as positive controls, mice which received only challenge without sensitization served as negative controls. *, p < 0.05.

UV-induced tolerance is mediated via T cells with suppressor activity because adoptive transfer of T cells obtained from lymph nodes and spleens of mice which had been UV-tolerized against DNFB renders the recipient mice unresponsive against DNFB (9). The mechanism and the phenotype of these T cells with regulatory/suppressor function still remain to be determined. To address whether injection of sDec2 prevents the development of these regulatory T cells, donor mice were tolerized against DNFB by painting the hapten onto UV-exposed skin. Five days later, lymph nodes and spleens were removed and single cell suspensions were prepared. T cells (2 x 10⁷) were injected i.v. into naive syngeneic mice. Recipients were sensitized against DNFB 24 h later. Mice which received cells from UV-tolerized donors could not be sensitized against DNFB (Fig. 4). Mice which received cells from untreated donors were not impaired in their CHS response (data not shown). Transfer of cells from mice which received an injection of sDec2 before tolerization against DNFB did not suppress the CHS response against DNFB in the recipients. In contrast, transfer of suppression was observed upon injection of cells from DHFR-treated and UV-tolerized mice (Fig. 4). These data indicate that injection of sDec2 before tolerization either inhibits the development of UV-induced regulatory T cells or alternatively inhibits their suppressive activity.

View larger version (25K): [in this window] [in a new window]   FIGURE 4. Injection of sDec2 inhibits transfer of suppression. Donor mice were sensitized through UV-exposed skin. Three hours before sensitization through UV-exposed skin, 50 µg of sDec2 or DFHR was injected. Five days later spleens and regional lymph nodes were removed and T cells were prepared. Cells (2 x 107) were injected i.v. into naive recipient mice which were sensitized against DNFB 24 h later. After 5 days, mice were challenged on the left ear and ear swelling was evaluated 24 h later. *, p < 0.01.

The data so far suggested that interaction of dectin-2 with its putative ligand is crucial in the development and mediation of UV-induced tolerance. Because dectin-2 is expressed on dendritic cells, we postulated that the putative ligand may be expressed on T cells. To test this hypothesis, T cells were incubated with biotinylated sDec2 followed by incubation with streptavidin-coupled FITC. After washing, FACS analysis was performed. Although in naive and DNFB-sensitized animals 0.3 and 2.48% T cells, respectively, bound sDec2, the number of sDec2-positive T cells was increased (5.95%) in UV-tolerized animals (Fig. 5). The specificity of the binding was confirmed by competition with excess amounts of unlabeled sDec2, while the control protein DHFR did not compete (Fig. 5).

View larger version (40K): [in this window] [in a new window]   FIGURE 5. Increase of sDec2+ T cells in UV-tolerized mice. T cells were prepared from the lymph nodes and spleens of untreated, DNFB-sensitized, and UV-tolerized mice. Cells were incubated with biotinylated sDec2. For competition of the binding, excess amounts of unlabeled sDec2, boiled sDec2, or DHFR were added. Samples were further incubated with streptavidin-coupled FITC and FACS analysis was performed.

Due to the increased binding of sDec2 on T cells from UV-tolerized mice, we surmised that sDec2 binds to the regulatory T cells which are responsible for transferring suppression. Therefore, T cells obtained from UV-tolerized mice were incubated with biotinylated sDec2. Subsequently, cells were incubated with streptavidin-coupled beads. Finally, UV-tolerized T cells were depleted of the sDec2-bound fraction. The sDec2-depleted fraction of cells was injected into naive recipients, which were sensitized against DNFB 24 h later. Although transfer of bulk T cells from UV-tolerized donors inhibited sensitization in the recipients, animals which received the depleted fraction could be successfully sensitized against DNFB (Fig. 6A). Depletion of sDec2-bound cells from T cells obtained from DNFB-sensitized donors did not affect induction of CHS in the recipients.

View larger version (20K): [in this window] [in a new window]   FIGURE 6. sDec2-binding T cells transfer suppression. A, T cells were prepared from naive, DNFB-sensitized, or UV-tolerized donors. T cells were left untreated or depleted of sDec2-binding cells by magnetobead separation. Subsequently, 200 µl of each T cell fraction (1 x 108 cells/ml) were injected i.v. into naive recipients. Recipients were sensitized with DNFB 24 h after injection. Five days later, ear challenge was performed and ear swelling was evaluated 24 h later. B, sDec2-bound T cells from UV-tolerized mice cells were obtained by magnetobead separation. Magnetobeads which had spontaneously detached from the cells after overnight incubation were removed with a magnet and the remaining cells were harvested, 5 x 106 cells (sDec2-bound T cells) were injected i.v. into naive recipients, which were then DNFB-sensitized and challenged. In parallel, "bulk T cells" obtained from UV-tolerized animals were injected. Positive control mice were sensitized and challenged, negative control mice were challenged only. *, p < 0.05.

Phenotypic characterization of sDec2-binding T cells

To further characterize the phenotype of sDec2-bound T cells, FACS analysis was performed. T cells obtained from lymph nodes and spleens of either naive, DNFB-sensitized, or UV-tolerized mice were triple-stained with the Abs directed against CD4 and CD25, respectively, and with biotinylated sDec2. FACS analysis (Fig. 7) revealed an increase in the number of CD4⁺CD25⁺ T cells in UV-tolerized animals as compared with naive and sensitized mice. sDec2-binding cells were detected by incubating the cells with FITC-coupled streptavidin. sDec2-bound CD25⁺ T cells were almost exclusively observed in UV-tolerized animals, the same was observed for CD4. Together, these findings indicate that sDec2-bound T cells also express CD4 and CD25 and thus may belong to the group of CD4⁺CD25⁺ regulatory T cells. We are currently investigating whether these cells also express CTLA-4 which has been suggested to be involved in mediating UV-induced tolerance (25).

View larger version (47K): [in this window] [in a new window]   FIGURE 7. sDec2-binding T cells express CD4 and CD25. T cells were prepared from the lymph nodes and spleens of untreated, DNFB-sensitized, and UV-tolerized mice. Cells were incubated with an allophycocyanin-conjugated Ab directed against CD4, with a PE-conjugated Ab directed against CD25 and with biotinylated sDec2, which was finally reacted with FITC-coupled streptavidin. After washing, the samples were analyzed by flow cytometry.

View this table: [in this window] [in a new window]   Table I. sDec2+ T cells release IL-4, IL-10, and TGF- upon hapten-specific stimulation

Finally, we tested whether injection of sDec2 into recipients of UV-tolerized T cells prevents transfer of suppression. Therefore, T cells isolated from UV-tolerized animals were transferred into naive recipients, which had been injected with sDec2 3 h before transfer. Mice which received T cells from tolerized mice could not be sensitized, while recipients of the same fraction of cells which in addition were treated with sDec2 revealed a normal CHS responses against DNFB (Fig. 8). This indicates that injection of sDec2 into recipients enables sensitization in the presence of regulatory T cells. When T cells from DNFB-sensitized animals were transferred, injection of sDec2 did not affect the onset of CHS in the recipients (data not shown).

View larger version (24K): [in this window] [in a new window]   FIGURE 8. Injection of sDec2 into recipients inhibits transfer of suppression. Three hours before i.v. transfer of UV-tolerized T cells (2 x 107 cells/mouse) into naive recipients, 50 µg of sDec2 or DHFR was injected. Recipients were subsequently DNFB-sensitized and challenged 5 days later. Ear swelling was evaluated 24 h later. *, p < 0.01.

In summary, the present data indicate that dectin-2 and its yet unidentified ligand may play a crucial role in the mediation of UV-induced immunosuppression. Interaction between these two molecules appears to be involved both in the inhibition of the induction of CHS by UV and in the mediation of UV-induced tolerance. Because sDec2 binds to the fraction of T cells which are crucial for transferring suppression, the putative ligand may serve as a future marker for UV-induced regulatory T cells. Hence, identification of the ligand for dectin-2 on the T cells is urgently required and ongoing in our laboratory.

However, the binding of sDec2 must not be regarded as a specific feature of the cells transferring UV-induced suppression because it cannot be excluded that only a minority of cells transferred are responsible for mediating hapten-specific unresponsiveness in the recipients. In contrast, interaction of dectin-2 with its ligand appears to be functionally relevant for mediating UV-induced immunosuppression because injection of sDec2 in vivo prevented the suppression of CHS by UV and even broke UV-mediated tolerance. It has been previously reported that established tolerance can be broken by the injection of IL-12 (27, 28). We do not know whether these two phenomena are related or independent, but we are currently investigating whether the binding sites for sDec2 on T cells are regulated by IL-12. In addition, injection of neutralizing Abs against CTLA-4 is also able to break UV-induced tolerance (29). In this context, it was proposed that triggering of CTLA-4 by B7 molecules expressed on the APCs induces release of IL-10 which subsequently inhibits resensitization, thereby rendering the respective animal tolerant to the hapten. Accordingly, T cells obtained from UV-tolerized mice were found to release high amounts of IL-10 upon in vitro stimulation with hapten-coupled APCs (29). It remains to be determined whether the release of IL-10 by T cells is suppressed in the presence of sDec2.

UV-induced regulatory T cells are still poorly characterized. A major obstacle in this context may be the poor proliferative capacity which makes cloning extremely difficult probably even impossible. Therefore, the detection of any further surface marker expressed on UV-induced regulatory T cells will help to better characterize these cells and to better understand their mode of action. The detection of the binding sites for dectin-2 as demonstrated in this study may add to this.

	Footnotes

 
¹ This work was supported by grants from the Grants-in-Aid for Scientific Research (Category B, No. 14370263) and for Exploratory Research (No. 14657205) from the Japanese Ministry of Education, Culture, Sports, Science, and Technology (to Y.A.), and from the German Research Foundation (SFB 293, B9; to T.S.).

² Address correspondence and reprint requests to Dr. Yoshinori Aragane, Department of Dermatology, Kinki University, 377-2 Ohnohogashi, Osakasayama City, 589-8511 Osaka, Japan. E-mail address: nori{at}med.kindai.ac.jp

³ Abbreviations used in this paper: CHS, contact hypersensitivity; sDec2, soluble dectin-2; DHFR, dihydrofolate reductase; DNFB, 2,4-dinitrofluorobenzene; DNBS, 2,4-dinitrobenzene-sulfonic sodium salt.

Received for publication March 14, 2003. Accepted for publication July 22, 2003.

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