IL-21-induced B{varepsilon} cell apoptosis mediated by natural killer T cells suppresses IgE responses

doi:10.1084/jem.20062206

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doi:10.1084/jem.20062206
The Journal of Experimental Medicine, Vol. 203, No. 13, 2929-2937
The Rockefeller University Press, 0022-1007 $30.00
© Harada et al.

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ARTICLE

IL-21–induced B ${varepsilon}$ cell apoptosis mediated by natural killer T cells suppresses IgE responses

Michishige Harada¹, Kumiko Magara-Koyanagi⁵, Hiroshi Watarai¹, Yuko Nagata¹, Yasuyuki Ishii², Satoshi Kojo¹, Shigetoshi Horiguchi⁶, Yoshitaka Okamoto⁶, Toshinori Nakayama⁵, Nobutaka Suzuki³, Wen-Chen Yeh⁷, Shizuo Akira⁸, Hiroshi Kitamura⁴, Osamu Ohara⁴, Ken-ichiro Seino¹, and Masaru Taniguchi¹

¹ Laboratory for Immune Regulation, ² Laboratory for Vaccine Design, ³ Laboratory for Cell Signaling, and ⁴ Laboratory for Immunogenomics, RIKEN Research Center for Allergy and Immunology, Yokohama, Kanagawa 230-0045, Japan
⁵ Department of Molecular Immunology and ⁶ Otorhinolaryngology/Head and Neck Surgery, Chiba University School of Medicine, Chiba-City, Chiba 260-8670, Japan
⁷ Amgen Institute, Ontario Cancer Institute and Department of Medical Biophysics, University of Toronto, Toronto, Ontario M5G 2C1, Canada
⁸ Department of Host Defense, Research Institute for Microbial Diseases, Osaka University, Suita Osaka 565-0871, Japan

CORRESPONDENCE Masaru Taniguchi: taniguti{at}rcai.riken.jp

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ABSTRACT
RESULTS
DISCUSSION
MATERIALS AND METHODS
REFERENCES

Epidemiological studies have suggested that the recent increasein the incidence and severity of immunoglobulin (Ig)E-mediatedallergic disorders is inversely correlated with Mycobacteriumbovis bacillus Calmette Guerin (BCG) vaccination; however, theunderlying mechanisms remain uncertain. Here, we demonstratethat natural killer T (NKT) cells in mice and humans play acrucial role in the BCG-induced suppression of IgE responses.BCG-activated murine V ${alpha}$ 14 NKT cells, but not conventional CD4T cells, selectively express high levels of interleukin (IL)-21,which preferentially induces apoptosis in B ${varepsilon}$ cells. Signalingfrom the IL-21 receptor increases the formation of a complexbetween Bcl-2 and the proapoptotic molecule Bcl-2–modifyingfactor, resulting in B ${varepsilon}$ cell apoptosis. Similarly, BCG vaccinationinduces IL-21 expression by human peripheral blood mononuclearcells (PBMCs) in a partially NKT cell–dependent fashion.BCG-activated PBMCs significantly reduce IgE production by humanB cells. These findings provide new insight into the therapeuticeffect of BCG in allergic diseases.

Abbreviations used: ${alpha}$ -GalCer, ${alpha}$ -galactosylceramide; BCG, Mycobacteriumbovis bacillus Calmette Guerin; BM-DC, BM-derived DC; Bmf, Bcl-2–modifyingfactor; ${gamma}$ c, common ${gamma}$ -chain; IRAK, IL-1R– associated kinase;MNC, mononuclear cell; MyD88, myeloid differentiation factor88; PGN, peptidoglycan; TLR, Toll-like receptor.

The prevalence of IgE-mediated allergic diseases such as asthma,hay fever, and atopic dermatitis has increased dramaticallyover the past two decades, especially in industrialized countries(1). For example, the incidence of asthma has nearly doubledsince 1980 in the United States as well as in Japan (1, 2).However, the precise mechanisms underlying the increased incidenceof allergic diseases are not fully understood. One possibleexplanation has been termed "the hygiene hypothesis," whichproposes that improved hygiene combined with the excessive useof antibiotics in industrial countries has markedly reducedthe incidence of infections, particularly in children. Thislack of early exposure to infectious agents is associated withaccelerated IgE production and an increased incidence of allergicdisorders (1–3). Epidemiological studies support thishypothesis (4–6), and bacterial and viral products havebeen proposed as therapeutic strategies to suppress the developmentof allergic responses. For example, vaccination with Mycobacteriumbovis bacillus Calmette Guerin (BCG) has been reported to suppressIgE production and inhibit the development of allergic diseasesin mouse models (7–9) and in humans (10). Furthermore,injection of CpG oligodeoxynucleotides, bacterial DNA surrogatesrecognized by Toll-like receptor (TLR)9, reduces serum IgE levelsin mice (11).

It has been widely accepted that IgE production is totally dependenton Th2 cells, whose functions are reciprocally inhibited byTh1 cells. Mechanistically, therefore, the hygiene hypothesisis based on an imbalance in the Th1/Th2 ratio because bacterialcomponents stimulate Th1 responses that in turn inhibit Th2responses and IgE production (12). On the other hand, recentfindings have indicated that a spectrum of T cells with immunoregulatoryproperties is involved in the regulation of IgE production andthe pathophysiology of allergic diseases (13). For example,CD4⁺CD25⁺ regulatory T cells inhibit Th2 responses by producingimmunosuppressive cytokines that can directly inhibit B cellactivation (14, 15). Furthermore, NKT cells expressing an invariantantigen receptor (V ${alpha}$ 14-J ${alpha}$ 281 for mice and V ${alpha}$ 24-J ${alpha}$ Q for humans; reference16) suppress Th2 and IgE responses via their production of IFN- ${gamma}$ (17).

In addition to these cellular mechanisms, it has also been reportedthat IL-21 is involved in the suppression of IgE productionin both mice and humans (18, 19). IL-21 is a type I cytokineproduced by activated CD4⁺ T cells and has a broad capacityto regulate lymphoid cell functions (20–22). Among thesefunctions, IL-21 directly inhibits antibody production by IgE-bearingB (B ${varepsilon}$ ) cells induced by CD40L and IL-4 (18). Conversely, IL-21R–deficientmice exhibit enhanced IgE production (23). IL-21 has been shownto specifically inhibit germ line transcription of the IgE constantregion (C ${varepsilon}$ ) gene but not of other isotype genes (18). However,there is no direct evidence that this inhibition of germ linetranscription is responsible for the suppression of IgE production,as class switch recombination of Ig genes and subsequent antibodysecretion are differentially regulated events (24). IL-21 alsoinduces apoptosis in B cells (25, 26), which could partiallyexplain the reduction of IgE production; however, this effectwas not shown to be specific for IgE. Hence, the mechanism bywhich IL-21 specifically inhibits IgE production is not yetfully understood.

Here, we have investigated BCG-mediated IgE suppression andfound that NKT cells specifically induced apoptosis in B ${varepsilon}$ cellsthrough the production of IL-21, resulting in a dramatic decreasein IgE production. IL-21 increased the formation of a complexbetween Bcl-2 and the proapoptotic molecule Bcl-2–modifyingfactor (Bmf), which is selectively expressed in B ${varepsilon}$ cells andcounteracts the antiapoptotic activity of Bcl-2. We have foundthat similar mechanisms are operative in humans. This is thefirst report demonstrating that IL-21 produced by V ${alpha}$ 14 NKT cellsplays an important role in the regulation of IgE responses inboth mouse and human immune systems.

RESULTS

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ABSTRACT
RESULTS
DISCUSSION
MATERIALS AND METHODS
REFERENCES

V ${alpha}$ 14 NKT cell–dependent IgE suppression by BCG treatment
We used an OVA-patched sensitization protocol (27) to determineif BCG activates V ${alpha}$ 14 NKT cells. V ${alpha}$ 14 NKT cells were detectedby ${alpha}$ -galactosylceramide ( ${alpha}$ -GalCer)–loaded CD1d tetramerstaining. In control mice treated with PBS or OVA without BCG, $~$ 15% of the liver mononuclear cells (MNCs) were V ${alpha}$ 14 NKT cells(Fig. 1 A, left and middle). However, BCG treatment significantlyincreased the frequency of V ${alpha}$ 14 NKT cells to >25% (Fig. 1 A,right). BCG treatment also increased the absolute number ofV ${alpha}$ 14 NKT cells because the total number of liver MNCs was alsoincreased by 50–80% (not depicted). Sera were collectedfrom these mice 1 wk after the last sensitization, and IgE levelswere evaluated. In WT mice, both total and OVA-specific IgElevels were suppressed by BCG treatment (Fig. 1 B). In micelacking the J ${alpha}$ 18 gene (V ${alpha}$ 14 NKT KO), there was no significantBCG-induced suppression of IgE responses, suggesting that suppressionrequires V ${alpha}$ 14 NKT cells.

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Figure 1. Requirement of V ${alpha}$ 14 NKT cells in BCG-mediated IgE suppression. (A) FACS profiles of liver MNCs. The liver MNCs obtained 1 wk after the last immunization were stained with ${alpha}$ -GalCer/CD1d tetramer and anti-TCRß mAb. Three mice per each group were analyzed and representative data are shown. (B and C) Effects of BCG on antibody responses in WT and V ${alpha}$ 14 NKT KO mice. Total and OVA-specific serum IgE (B), IgG1, and IgG2a (C) were assayed by ELISA. Five mice were used in each group. Values are expressed as mean ± SD. The asterisks (*) indicate that the amount of IgE was below the detection level for anti-OVA IgE (<31.2 U/ml), anti-OVA IgG1 (<0.002 U/ml), or anti-OVA IgG2a (<1.25 U/ml). N.S., not significant. All experiments were repeated three times with similar results.

The effect of BCG administration on Th1/Th2 responses
It is well known that the isotype commitment of B cells duringIg class switching is tightly regulated by Th1/Th2 cell cytokines(28) and that V ${alpha}$ 14 NKT cells play a regulatory role in T celldifferentiation (17, 29, 30). Therefore, we measured serum IgG2a(Th1) and IgG1 (Th2) levels to assess any changes in the Th1/Th2balance. BCG administration did not significantly alter thelevels of OVA-specific IgG1 or IgG2a, although total levelsof both isotypes were significantly enhanced (Fig. 1 C).

Innate signaling pathway for BCG-mediated IL-12 production
During microbial infection, both CD1d- and IL-12–mediatedsignals are required for the rapid activation of V ${alpha}$ 14 NKT cells(31). Thus, we assessed IL-12 production after BCG treatment.BM-derived DCs (BM-DCs) were stimulated in vitro with 50 µg/mlBCG and examined for IL-12 production by intracellular cytokinestaining using an IL-12p40/p70 mAb. Upon BCG stimulation, alarge fraction of CD11c^high cells produced IL-12 (Fig. 2 A). NF- ${kappa}$ B activation is crucial for IL-12 production, and BCG treatmentactivated NF- ${kappa}$ B to the same extent as treatment with the positivecontrol CpG, as demonstrated by electrophoretic mobility shiftassay (Fig. 2 B). These results indicate that BCG directly inducesIL-12 production in DCs by activating NF- ${kappa}$ B.

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Figure 2. Activation of DCs by BCG. IL-12 production (A) and NF- ${kappa}$ B activation (B). (A) Intracellular staining of BM-DCs with anti–IL-12p40/p70 and anti-CD11c mAbs with or without in vitro BCG (50 µg/ml) treatment for 12 h. BCG-treated BM-DCs (10,000 cells) were analyzed by FACS, and the number in each panel indicates the percentage of total cells. (B) NF- ${kappa}$ B activation. 2 x 10⁵ BM-DCs were stimulated with or without 50 µg/ml BCG or 1 µM CpG in vitro. NF- ${kappa}$ B activity was determined by EMSA. (C and D) No requirement of TLR2 and TLR4 in BCG-mediated IL-12 production. 2 x 10⁵ BM-DCs derived from WT (C) or TLR2/4 double KO (D) mice were stimulated in vitro with or without 10 µg/ml LPS, 10 µg/ml PGN, or 150 µg/ml BCG for 48 h, and IL-12p70 levels were measured by ELISA. (E and F) Requirement of IRAK-4 for IL-12 production. 2 x 10⁵ BM-DCs were assayed for IL-12p70 by ELISA after stimulation with 0, 50, or 150 µg/ml BCG or 1 µM CpG (E), and for IL-6 with 10 ng/ml TNF- ${alpha}$ stimulation for 48 h (F). In C–F, values are expressed as mean ± SD of triplicate cultures. The asterisks (*) indicate that the levels were below the detection limits for IL-12p70 (<62.5 pg/ml) and IL-6 (<15.6 pg/ml). N.S., not significant. All experiments were repeated twice with similar results.

It has been reported that mycobacterial cell wall antigens suchas peptidoglycan (PGN) or lipoarabinomannan induce proinflammatorygene transcription through TLR2 and TLR4 (32). However, whenwe compared IL-12p70 production by BCG-stimulated WT and TLR2/TLR4double KO BM-DCs, there was no difference (Fig. 2 C). As expected,however, the TLR2/4-deficient cells failed to respond to LPSor PGN (Fig. 2 D). These results indicate that receptor(s) otherthan TLR2 and TLR4 are responsible for the recognition of wholeBCG organisms.

To analyze intracellular signaling pathways activated by BCG,we measured IL-12p70 production by BM-DCs from WT and IL-1R–associatedkinase (IRAK)-4 KO mice. BM-DCs from IRAK-4 KO mice producedless IL-12p70 than those from WT mice in response to both BCGand CpG (Fig. 2 E), whereas they produced comparable levelsof IL-6 in response to TNF- ${alpha}$ stimulation (Fig. 2 F). Similarly,BM-DCs from myeloid differentiation factor 88 (MyD88) KO miceproduced nearly undetectable IL-12p70 upon BCG stimulation,whereas IL-6 production remained unchanged (Fig. S1, availableat http://www.jem.org/cgi/content/full/jem.20062206/DC1). Therefore,the recognition of BCG organisms is mediated by innate receptorsother than TLR2 and TLR4 that signal through both IRAK-4 andMyD88.

BCG-induced IL-21 expression in V ${alpha}$ 14 NKT cells
The recently identified IL-21 and its receptor (IL-21R), membersof the common ${gamma}$ -chain ( ${gamma}$ c)-dependent cytokine family, have beenshown to regulate IgE production without influencing Th2 celldifferentiation (18, 20, 23). Thus, we examined the possibilitythat IL-21 might be induced by BCG stimulation and might suppressIgE responses in a V ${alpha}$ 14 NKT cell–dependent manner. We firstmeasured IL-21 mRNA expression in TCRß⁺ liver MNCsby a RT-PCR. IL-21 mRNA was detected in liver TCRß⁺liver MNCs of WT mice within 6 h after BCG injection (Fig. 3 A). In contrast, no IL-21 mRNA was detected in the V ${alpha}$ 14 NKT KO mice(Fig. 3 A), suggesting that V ${alpha}$ 14 NKT cells are the source ofIL-21 in response to BCG. To test this hypothesis, we separatedconventional T cells and V ${alpha}$ 14 NKT cells and found that IL-21mRNA was more abundant in the V ${alpha}$ 14 NKT cells after BCG injection(Fig. 3 B). Similarly, after stimulation with anti-CD3, IL-21mRNA levels in V ${alpha}$ 14 NKT cells were more than seven times higherthan in CD4 T cells, confirming that these cells are the majorsource of IL-21 in this model (Fig. S2 A, available at http://www.jem.org/cgi/content/full/jem.20062206/DC1).

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Figure 3. IL-21 expression. (A) V ${alpha}$ 14 NKT cell–dependent IL-21 production. Liver MNCs were obtained after BCG injection (500 µg/mouse) and examined for IL-21 mRNA expression. (B) Identification of the source of IL-21. V ${alpha}$ 14 NKT and conventional T cells were sorted from liver MNCs and examined for IL-21 mRNA expression. (C) Requirement of DCs for BCG-induced IL-21 expression by V ${alpha}$ 14 NKT cells. Liver TCRß⁺ cells were cultivated in the presence of 50 µg/ml BCG with (top) or without (bottom) BM-DCs for 24 h and analyzed for IL-21 mRNA expression. Liver TCRß⁺ cells stimulated with 10 µg/ml anti-CD3 mAb were used as a positive (Pos.) control. (D) Requirement of IL-12– and CD1d-mediated signals for IL-21 mRNA expression upon BCG stimulation. An isotype control, anti–IL-12p40/p70, or anti-CD1d mAb (20 µg/ml) was added to the cultures of liver TCRß⁺ cells and BM-DCs as described in C. All experiments were repeated twice with similar results.

Requirement for IL-12 and CD1d in IL-21 expression by V ${alpha}$ 14 NKT cells
We next analyzed the role of DCs in BCG-induced IL-21 mRNA expression.Co-culture of V ${alpha}$ 14 NKT cells with DCs plus IL-12 strongly inducedIL-21 mRNA expression, whereas no IL-21 mRNA was induced inthe absence of DCs (Fig. 3 C). Furthermore, IL-21 mRNA expressionwas inhibited by the addition of anti–IL-12, anti-CD1d,or both into the cultures (Fig. 3 D), indicating that both IL-12and CD1d are required for IL-21 expression by V ${alpha}$ 14 NKT cells.

IL-21–mediated IgE suppression
To examine whether BCG-activated V ${alpha}$ 14 NKT cells actually suppressIgE production, B ${varepsilon}$ cells were generated from naive CD19⁺ splenicB cells using the 3-d culture system described by Snapper etal. (33). The starting population of naive B cells expressednegligible IL-21R and contained no B ${varepsilon}$ cells as defined by C ${varepsilon}$ transcripts(Fig. 4 A). However, after 3 d of the culture, the majorityof CD19⁺ B cells became B ${varepsilon}$ cells and expressed IL-21R (Fig. 4 A).We then investigated the effects of BCG treatment on B cells,before and after IgE class switching. The addition of BCG-treatedliver MNCs at the onset of the naive B cell cultures significantlysuppressed IgE production ( $~$ 50%; Fig. 4 B). However, when BCG-activatedV ${alpha}$ 14 NKT cells were added to the B ${varepsilon}$ cell culture on day 3 andthe cells were further cultivated for 5 d, IgE production waseven more strongly inhibited (>90% suppression; Fig. 4 C).These results indicate that, even after B cells have undergoneC ${varepsilon}$ class switching, BCG-activated V ${alpha}$ 14 NKT cells can potentlysuppress IgE production. The inhibition of IgE production wasIL-21 dependent, as an anti–IL-21 mAb completely abrogatedthe inhibitory effects (Fig. 4, B and C). When the B cells inthese cultures were assessed for apoptosis by annexin V staining,there was a significant increase in apoptotic B ${varepsilon}$ cells that wasnot observed in the B ${gamma}$ cells (Fig. 4 D, middle). Apoptosis ofB ${varepsilon}$ cells was abrogated by the addition of anti–IL-21, atreatment that had no significant effect on B ${gamma}$ cells (Fig. 4 D,right).

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Figure 4. IL-21–mediated B ${varepsilon}$ cell apoptosis. (A) RT-PCR analysis. Expression of IgE (C ${varepsilon}$ ), IL-21R, and ${gamma}$ c was investigated in naive B (left) and B ${varepsilon}$ (right) cells. (B) Suppression of IgE production in naive B cell cultures. Naive B cells and V ${alpha}$ 14 NKT cells (10⁵ each) were cocultured in the presence of sCD40L and IL-4. (C) Suppression of IgE production in the B ${varepsilon}$ cell culture. 10⁵ V ${alpha}$ 14 NKT cells were added to the B ${varepsilon}$ cell (10⁵) cultures. In B and C, 20 µg/ml anti–IL-21 mAb or isotype control mAb was added at the same time as the V ${alpha}$ 14 NKT cells. The concentration of total IgE was measured by ELISA in triplicate. Values are expressed as mean ± SD. N.S., not significant. The experiments were repeated three times with similar results. (D) IL-21–mediated B ${varepsilon}$ cell apoptosis. 2 x 10⁵ B ${varepsilon}$ and B ${gamma}$ cells were generated and then further cultured with or without 30 ng/ml IL-21 for 30 h. Annexin V staining was then performed. The numbers represent percentage of the gated cells. Annexin V⁺ cells among B ${varepsilon}$ and B ${gamma}$ cells just before IL-21 treatment was 25.7 and 29.2%, respectively (not depicted). The experiments were repeated three times with similar results.

Bmf-induced B ${varepsilon}$ cell apoptosis
To understand the molecular mechanisms underlying IL-21–induced IgE suppression, we performed DNA microarray analysesto compare gene expression between B ${varepsilon}$ and B ${gamma}$ cells. The DNA microarraydata were deposited in the Center for Information Biology GeneExpression database (CIBEX; http://cibex.nig.ac.jp/) under accessionnumber CBX15. The proapoptotic Bmf gene (34) was dramaticallyup-regulated in B ${varepsilon}$ cells, a finding that was confirmed by RT-PCR(Fig. 5 A). No significant difference in the expression ofIL-21R, Bcl-2, or ${gamma}$ c was detected (Fig. 5 A), suggesting thatelevated Bmf gene expression in B ${varepsilon}$ , but not in B ${gamma}$ , cells may accountfor their differential sensitivity to IL-21–mediated apoptosis.

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Figure 5. Bmf-mediated B ${varepsilon}$ cell apoptosis. (A) RT-PCR. RNA from B ${varepsilon}$ and B ${gamma}$ cells was analyzed for its expression of the indicated genes by RT-PCR. Note that no significant differences in Bcl-2 and IL-21R expression between B ${varepsilon}$ and B ${gamma}$ cells were observed. (B) Western blotting. B ${varepsilon}$ cells were stimulated with IL-21 at 37°C for 30 min, and their cell lysates (6 x 10⁶) were subjected to immunoprecipitation with anti–Bcl-2 mAb and immunoblotting with anti-Bmf antibody (top) or anti–Bcl-2 mAb (bottom). All experiments were repeated three times with similar results.

To investigate whether the Bmf expressed in B ${varepsilon}$ cells is functionalin its proapoptotic activity, Bmf cDNA was isolated from B ${varepsilon}$ cellsand used to prepare several mutants of enhanced GFP–fusedBmf. These mutations included an A69P mutation in the dyneinlight chain 2 binding motif and an L138A mutation in the BH3domain. These Bmf mutants were transfected into Baf3 cells.Upon IL-3 deprivation, mock transfectants underwent apoptosis.Transfection with WT Bmf or Bmf-A69P to Baf3 cells also significantlyaugmented apoptosis (Fig. S3, available at http://www.jem.org/cgi/content/full/jem.20062206/DC1).However, reduced apoptosis was seen in Baf3 cells transfectedwith BH3 mutants, such as Bmf-L138A or Bmf-A69P/L138A (Fig.S3), indicating that Bmf in B ${varepsilon}$ cells is functional and the BH3domain of the protein is important for mediating its proapoptoticactivity.

Based on the understanding of proapoptotic activity of Bmf expressedin B ${varepsilon}$ cells, we investigated the formation of Bmf–Bcl-2complexes in B ${varepsilon}$ cells after activation with IL-21. Bmf in B ${varepsilon}$ cellsfaintly binds to Bcl-2 in unstimulated cells (Fig. 5 B, left).However, when B ${varepsilon}$ cells were stimulated with IL-21, the formationof Bmf–Bcl-2 complexes was significantly augmented (Fig. 5 B,right).

BCG-mediated IL-21 induction in human V ${alpha}$ 24 NKT cells
To determine how widespread our findings are, we investigatedwhether IL-21 and V ${alpha}$ 24 NKT cells are required for the BCG-mediatedsuppression of human IgE responses. When human PBMCs were stimulatedwith ${alpha}$ -GalCer or BCG, a significant up-regulation of IL-21 mRNAwas detected by quantitative PCR (Fig. 6 A). The BCG-inducedup-regulation of IL-21 mRNA was effectively suppressed by blockingwith antibodies against CD1d, IL-12p40/p70, or both (Fig. 6 B),indicating that the CD1d-restricted NKT cell–dependentsuppression of IgE responses observed in mice also operatesin the human immune system. IL-21 mRNA expression by anti-CD1dand anti–IL-12 treatment was significantly reduced butwas not as effective as in the mouse V ${alpha}$ 14 NKT cell system (Fig. 3 D),perhaps suggesting a significant contribution of human conventionalCD4⁺ T cells (Fig. S2 B).

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Figure 6. IL-21 mRNA expression and IL-21–induced IgE suppression in humans. (A) IL-21 mRNA expression in PBMCs. 10⁶ human PBMCs were stimulated with 100 ng/ml ${alpha}$ -GalCer or 50 µg/ml BCG and examined for IL-21 expression by quantitative real-time PCR with Taqman probes. The data are representative of five donors. (B) IL-12 and CD1d are required for IL-21 expression. 10⁶ PBMCs were stimulated in vitro with 50 µg/ml BCG in the presence of 10 µg/ml anti-CD1d and/or anti–IL-12p40/p70 mAb. Representative data from five donors are shown. (C) IL-21 mRNA expression in PBMCs. Healthy volunteers were inoculated intradermally with BCG (two drops of 26.7 mg/ml of BCG emulsion per person). In A–C, the data for IL-21 expression were normalized to 18S ribosomal RNA expression, and relative expression levels are shown. Statistical analysis was performed using a matched pairs t test in C. (D) Suppression of IgE production. Left, suppression of IgE production by IL-21. 2 x 10⁵ human B cells were cultured with sCD40L and IL-4 in the presence of human IL-21 for 14 d. Right, suppression of IgE production by BCG-activated human PBMCs. 10⁵ B ${varepsilon}$ cells were cocultured with 10⁵ PBMCs, sCD40L, and IL-4 in the presence of 50 µg/ml BCG for 14 d. Total IgE was measured by ELISA. Values are expressed as mean ± SD of triplicate cultures. The asterisks (*) indicate that the IgE levels are below the detection limit for total IgE (<0.014 IU/ml). Data shown are representative of three donors. Results were expressed as a fold difference in human IL-21 gene expression relative to a control sample (vehicle) after being normalized with 18S ribosomal RNA expressions in each sample.

To evaluate in vivo responses, we inoculated BCG into healthyvolunteers and examined IL-21 mRNA levels in PBMCs 1 wk later.There was a significant up-regulation of IL-21 mRNA levels infive out of six individuals (Fig. 6 C), and, furthermore, IL-21suppressed IgE production by human B ${varepsilon}$ cells (Fig. 6 D, left).As expected, the addition of BCG-stimulated, but not control,PBMCs significantly inhibited IgE production (Fig. 6 D, right).

DISCUSSION

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ABSTRACT
RESULTS
DISCUSSION
MATERIALS AND METHODS
REFERENCES

It is widely accepted that the mechanistic basis of the hygienehypothesis for suppression of IgE responses is an increase inthe Th1/Th2 ratio (12). However, in reality, the Th1 responseexacerbates allergic reactions, as human asthma is associatedwith the production of IFN- ${gamma}$ , a cytokine that appears to contributeto the pathogenesis of the disease (35). Furthermore, the adoptivetransfer of allergen-specific Th1 cells causes severe airwayinflammation (36). Thus, a shift in the Th1/Th2 ratio alonecannot explain all of the immunological findings observed inallergic diseases (1). Furthermore, there are several studiessuggesting that BCG vaccination has little or no effect on thedevelopment and prevalence of allergic diseases (37, 38). Therefore,it is necessary to better understand the precise mechanism ofIgE suppression in BCG-treated animals or humans.

In this study, neither a Th1/Th2 imbalance nor an involvementof regulatory T cells was observed in response to BCG treatment(Fig. 1). Instead, we demonstrated that IL-21–inducedB ${varepsilon}$ cell apoptosis is the mechanism responsible for BCG-mediatedsuppression of IgE production (Figs. 1, 3, and 5). Because thehuman IL-21 responses to BCG vaccination were heterogeneous(Fig. 6 C), it seems likely that the magnitude of the responsein each individual could cause different degrees of BCG-inducedIgE suppression and might be prognostic.

Previous studies have indicated that IL-21 is preferentiallyexpressed by activated CD4⁺ T cells (20), the results that arepartially in agreement with the present data, as half of peripheralV ${alpha}$ 14 NKT cells are CD4⁺ (39, 40). Interestingly, upon anti-CD3mAb stimulation, V ${alpha}$ 14 NKT cells, but not conventional T cells,preferentially expressed IL-21 (Fig. S2 A), similar to the resultswith BCG (Fig. 3 B). Therefore, the major IL-21 producers inresponse to BCG in mice are V ${alpha}$ 14 NKT cells.

It has been proposed that, for full activation of V ${alpha}$ 14 NKT cellsto produce IFN- ${gamma}$ , two signals are required: one CD1d-dependentand the other TLR-mediated IL-12–dependent signals (31).In agreement with this, IL-21 expression by BCG-activated V ${alpha}$ 14NKT cells was significantly inhibited by blocking with antibodiesto IL-12 and/or CD1d (Fig. 3 D). Therefore, it is likely thatV ${alpha}$ 14 NKT cells recognize endogenous antigens presented by CD1dmolecules but require IL-12 signals to produce IL-21. Nevertheless,it is still possible that glycolipid BCG components such asphosphatidylinositol mannoside may directly stimulate V ${alpha}$ 14 NKTcells to produce IL-21 in a CD1d-dependent manner (41, 42).

In terms of the receptors on DCs that are required for BCG recognitionand signal transduction, we showed in this study that BCG-inducedIL-12 production is IRAK-4 and MyD88 dependent (Fig. 2 E andFig. S1). These results in mice are consistent with a recentreport indicating that BCG cannot induce IL-12 or IFN- ${gamma}$ productionby PBMCs from IRAK-4–deficient patients (43). In addition,it has been reported that BCG enhances NF- ${kappa}$ B–dependentgene transcription through the activation of phosphatidylinositol3 kinase and c-Jun N-terminal kinase cascades (44). The activatedNF- ${kappa}$ B is then liberated for nuclear translocation and transactivatesa variety of immune response genes, including IL-12.

In contrast to a previous report that implicated TLR2 and TLR4in the recognition of mycobacterial antigens (32), we couldnot identify any involvement of these receptors in IL-12 productionby BCG-stimulated BM-DCs (Fig. 2, C and D). In agreement withour findings, it has recently been reported that TLR2/4 doubleKO mice infected with live BCG have normal adaptive immune responsesand survived as long as WT mice (45). As whole BCG containsmultiple components including mycobacterial glycolipids, proteins,and DNA, several receptors that use IRAK-4 and MyD88 as thesignal transducer appear to be involved in the complex recognitionof BCG.

In IL-21R–deficient mice, the level of circulating IgEis high, whereas that of IgG1 is low (23, 46). Similarly, inhuman B cells, IL-21 inhibits IgE production and stimulatesIgG4 (analogous to mouse IgG1) production (19). These resultssuggest that IL-21 differentially regulates IgE and IgG1 (IgG4in humans) class switching. In fact, Suto et al. (18) reportedthat IL-21 specifically suppresses IgE production by inhibitinggerm line C ${varepsilon}$ transcripts. Our present findings do not excludethis possibility. IL-21 has also been reported to induce apoptosisin resting and activated B cells by reducing the expressionlevels of apoptosis-related genes (25, 26). However, in thisreport, we have shown that IL-21 selectively induces apoptosisin B ${varepsilon}$ , but not B ${gamma}$ , cells (Fig. 4 D). Thus, our findings that BCG-activatedIL-21–expressing V ${alpha}$ 14 NKT cells suppressed IgE productioneven after class switching (Fig. 4 C) suggests that the roleof IL-21 on B ${varepsilon}$ cells is to control cell growth and viability,rather than to regulate the differentiation and maturation ofthese cells.

We found that expression of a proapoptotic gene, Bmf, was significantlyhigher in B ${varepsilon}$ cells than in B ${gamma}$ cells (Fig. 5 A). Under physiologicalconditions, Bmf, which is a BH3 domain–only Bcl-2 familymember that inhibits Bcl-2 function and accelerates apoptosis,binds to myosin V motors via the dynein light chain 2 domainof Bmf (34). In response to certain cellular damage signals,Bmf is supposed to be released from the myosin V motors andtrigger apoptosis (34). Because Bmf from B ${varepsilon}$ cells induced apoptosisand a mutation in the BH3 domain of Bmf failed to induce apoptosis(Fig. S3), we confirmed that Bmf expressed in B ${varepsilon}$ cells is functional,and that the BH3 domain is important for the binding to Bcl-2and is essential for its proapoptotic activity. In fact, thebinding of Bmf with Bcl-2 was up-regulated by IL-21R signaling(Fig. 5 C). Therefore, BCG-mediated B ${varepsilon}$ cell apoptosis is dueto the augmented formation of Bmf–Bcl-2 complexes generatedby IL-21R signaling in B ${varepsilon}$ cells.

Finally, we defined the mechanism of BCG-induced IL-21–dependentsuppression of IgE production in humans (Fig. 6). In a broadercontext, these findings may explain the mechanisms underlyingthe BCG-mediated suppression of allergic diseases and the epidemiologicaldata indicating a reduction in the morbidity of allergic diseasesin patients who have been infected with Mycobacterium tuberculosis.Interestingly, IL-21–mediated B cell responses in C57BL/6mice differ from those in BALB/c mice (26), suggesting thatthere is a genetic polymorphism with respect to the outcomeof IL-21 signaling in B cells. In fact, a recent report indicatedthat polymorphisms in the IL-21R gene locus differentially affectserum IgE levels in humans (47). In this study, consistent withour data, the levels of IL-21 expression induced by BCG stimulationvaried among the individuals examined (Fig. 6 C). These resultssuggest that the response to BCG in humans is dependent, atleast in part, on genetic background. The specific genes responsiblefor the heterogeneity in BCG-mediated IL-21 production havenot been identified. However, this observation may be appliedto the development of diagnostic or therapeutic strategies inwhich the levels of IL-21 expression are used to evaluate theefficacy of BCG treatment, or in determining the potential benefitof therapy using bacterial products such as CpG for allergicdiseases.

MATERIALS AND METHODS

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ABSTRACT
RESULTS
DISCUSSION
MATERIALS AND METHODS
REFERENCES

Mice.
7–10-wk-old female BALB/c mice were purchased from JapanCREA Inc. V ${alpha}$ 14 NKT-deficient (V ${alpha}$ 14 NKT KO) mice on a BALB/c background(48), IRAK-4 KO (49), TLR2 KO, TLR4 KO, and MyD88 KO mice (50,51) have been described. TLR2 and TLR4 double KO mice were generatedby breeding. Mice were kept under specific pathogen-free conditions,maintained on an OVA-free diet, and treated in accordance withthe guidelines for animal care at RIKEN Research Center forAllergy and Immunology.

Allergic sensitization and BCG.
Allergic epicutaneous sensitization was performed as describedpreviously (27). In brief, a 1-cm² sterile patch infused with100 µl of PBS solution with or without 100 µg OVA(grade V; Sigma-Aldrich) was placed on the shaved back of miceand fixed in place with a bio-occlusive dressing and an elasticbandage. Patches were left on for 48 h and removed. The sensitizationcourse was repeated at the same skin site every week for 4 wk.For BCG vaccination, mice were given a weekly i.p. injectionof BCG (500 µg/mouse) or PBS at the time of OVA sensitization.The attenuated BCG (strain Tokyo) was purchased from the JapanBCG Laboratory.

Flow cytometry.
Cells were stained with antibodies after adding 2.4G2 (BD Biosciences)for Fc blocking. The following antibodies were used: FITC–anti-CD19(1D3), FITC–anti-IgE (R35-72), APC–anti-IgG1 (X59),FITC–anti-TCRß (H57-597), APC–anti–IL-12p40/70(C15.6), and PE–anti-CD11c (HL3; BD Biosciences). PE-conjugated ${alpha}$ -GalCer–loaded CD1d tetramer ( ${alpha}$ -GalCer/CD1d tetramer) wasprepared as described previously (52). For intracellular staining,BM-DCs were fixed and permeabilized with BD Cytofix and Cytopermkits after staining with PE–anti-CD11c. They were thenstained with APC–anti–IL-12p40/70. FACS analysisof at least 10,000 cells and cell sorting were performed witha FACSCalibur (BD Biosciences) with FlowJo software (TreeStar)or with a MoFlo cell sorter (DakoCytomation).

Cell preparations and cultures.
2 x 10⁶ BM-DCs obtained by culturing BM for 6 d with 10 ng/mlGM-CSF were further cultured in the presence or absence of BCG,CpG, LPS (Invivogen), PGN from Escherichia coli (Invivogen),or 10 µg/ml anti-CD3 mAb (2C11; BD Biosciences) for 48h at 37°C. For blocking experiments, mAb against CD1d orIL-12p40/p70 (clones 1B1 and C17.8, respectively; BD Biosciences),or an isotype control was added at a concentration of 20 µg/mlafter 2.4G2 treatment. TCRß⁺ cells or V ${alpha}$ 14 NKT cellswith a purity of >98% were obtained from liver MNCs (52)using an Auto MACS (Miltenyi Biotec) after staining with FITC–anti-TCRßand sorting with anti-FITC magnetic beads (Miltenyi Biotec).V ${alpha}$ 14 NKT cells were then isolated from TCRß⁺ cellsby MoFlo using PE– ${alpha}$ -GalCer/CD1d tetramer. ConventionalT or CD4⁺ T cells were isolated from an ${alpha}$ -GalCer/CD1d tetramer^–fraction of TCRß⁺ liver MNCs. B ${varepsilon}$ and B ${gamma}$ cells generatedfrom splenic CD19⁺ cells in the presence of 10 µg/ml sCD40L(ALX-850-075; Qbiogene) and 20 ng/ml of recombinant IL-4 (PeproTech)for 3 d (33) were cultured for 30 h for the apoptosis assayor for an additional 5 d to investigate IgE responses.

ELISA.
Cytokines (IL-12p70 and IL-6) and Ig subclasses (IgG1, IgG2a,and IgE) were measured by ELISA using kits or sets of antibodies(BD Biosciences) according to the manufacturer's protocol. Specificantibodies were also measured as described previously (7).

RT-PCR.
Total RNA was extracted by RNAeasy (QIAGEN), and cDNA was synthesizedwith random primers after DNase treatment. The following RT-PCRprimer sets were used for mouse genes: IL-21, 5'-CCCTTGTCTGTCTGGTAGTCATC-3'and 5'-ATCACAGGAAGGGCATTTAGC-3'; IgE (C ${varepsilon}$ ), 5'-AGGAACCCTCAGCTCTACCC-3'and 5'-GCCAGCTGACAGAGACATCA-3'; mIL-21R, 5'-TGTCAATGTGACGGACCAGT-3'and 5'-CAGCATAGGGGTCTCTGAGG-3'; ${gamma}$ c, 5'-GTCGACAGAGCAAGCACCATGTTGAAACTA-3'and 5'-GGATCCTGGGATCACAAGATTCTGTAGGTT-3'; Bmf, 5'-CAGACCCTCAGTCCAGCTTC-3'and 5'-CGTATGAAGCCGATGGAACT-3'; Bcl-2, 5'-GGTGGTGGAGGAACTCTTCA-3'and 5'-CATGCTGGGGCCATATAGTT-3'; and HPRT, 5'-AGCGTCGTGATTAGCGATG-3'and 5'-CTTTTATGTCCCCCGTTGAC-3'. The numbers of PCR cycles wereas follows: 30 for HPRT; 35 for IgE, ${gamma}$ c, and IL-21R; 40 for IL-21and Bmf; and 45 for Bcl-2. The amounts of cDNA were standardizedby quantification of the housekeeping gene HPRT using primersfor mouse samples. The human IL-21 mRNA levels were quantifiedby real-time quantitative PCR on the ABI Prism 7000 sequencedetection system (Applied Biosystems) by using TaqMan assaykits and TaqMan Gene Expression Assays (primers and TaqMan probes).

Electrophoretic mobility shift assay.
2 x 10⁶ BM-DCs were stimulated with 50 µg/ml BCG or 1.0µM CpG-B for the indicated periods. Nuclear extracts wereprepared and used for Gel Shift Assay Systems (Promega) as describedpreviously (50).

B ${varepsilon}$ cell–derived Bmf and its mutants.
cDNAs encoding bmf were amplified from B ${varepsilon}$ cells by PCR usingprimers 5'-CCGAATTCGGATGGAGCCACCTCAGTGTGT-3' and 5'-GCGGCCGCCTGCATTCCTGGTGATCCAT-3'(EcoRI and NotI sites for cloning are underlined). The amplifiedproducts were cloned using the pGEM-T Easy Vector System (Promega).Mutant cDNAs were generated by PCR using point-mutated primerpairs.

Immunoprecipitation and Western blotting.
Interaction of Bmf with Bcl-2 in B ${varepsilon}$ cells was detected by immunoprecipitationwith anti–Bcl-2 mAb (clone 7; BD Transduction Laboratories)and subsequent immunoblotting with anti-Bmf rabbit antibody(Cell Signaling). The protein levels were visualized by ECL(GE Healthcare) using horseradish peroxidase–conjugatedProtein A/G (Pierce Chemical Co.).

Human studies.
All human specimens were obtained under informed consent. Theprotocol for the human research project has been approved bythe Ethics Committee of Chiba University and RIKEN, and conformedto the provisions of the Declaration of Helsinki in 1995. 10⁸PBMCs from healthy volunteers were prepared by Ficoll-Paquedensity gradient centrifugation and used for the cultures. Humanrecombinant IL-21 was purchased from BIOSOURCE Inc. Human totalIgE was measured with a sensitive immune assay (GE Healthcare).

Statistical analysis.
Statistical analyses were performed using the Student's t testor matched pairs t test. P < 0.05 was considered statisticallysignificant.

Online supplemental material.
Fig. S1 provides data demonstrating that MyD88 signaling inDCs is required for BCG-induced activation. Fig. S2 containsdata demonstrating IL-21 mRNA expression by NKT cells, CD4⁺T cells, and CD8⁺ T cells of murine and human origin. Fig. S3provides the data indicating proapoptotic activity of B ${varepsilon}$ cell–derivedBmf and functional domain analysis using mutant Bmf in Baf3cells. The online supplemental material is available at http://www.jem.org/cgi/content/full/jem.20062206/DC1.

	Acknowledgments

The authors thank Prof. Peter Burrows for critical reading andMs. Norie Takeuchi for secretarial assistance.

This work was partly supported by a grant from The Ministryof Education, Culture, Sports, Science and Technology (RR2002).

The authors have no conflicting financial interests.

Submitted: 13 October 2006
Accepted: 21 November 2006

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MATERIALS AND METHODS
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