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Nat Immunol. Author manuscript; available in PMC 2010 Feb 1.
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Costimulatory molecule ICOS plays a critical role in the development of TH-17 and follicular T-helper cells by regulating c-Maf expression and IL-21 production

Abstract

The inducible costimulatory molecule (ICOS) has been suggested to play an important role in the development of interleukin 17 (IL-17)-producing T helper cells (TH-17 cells) and of follicular helper cells (TFH cells), specialized helper T cells (CD4+CXCR5+ICOShigh) required for antibody class switching and germinal center formation. Here we show that ICOS, while not essential for the differentiation of TH-17 cells, was critical for maintaining effector-memory TH-17 cells as ICOS-deficient mice demonstrated a defect in the expansion of TH-17 cells after IL-23 stimulation. In addition, we found that TFH cells produced IL-17 and that ICOS-deficient mice demonstrated a reduced frequency of TFH with a defect in IL-17 production. Both TH-17 and TFH cells showed increased expression of the transcription factor c-Maf—normally associated with TH2 cells— and that loss of c-Maf results in a defect in IL-21 production, and consequently a defect in the maintenance of IL-23R expression and expansion of TH-17 and TFH cells. These data suggest that c-Maf induced by ICOS regulates IL-21 production that, in turn, regulates expansion of TH-17 cells and TFH cells.

INTRODUCTION

Interleukine 17-producing T helper cells (TH-17 cells) have been recently described as functionally new CD4 helper T cell subset that plays an important role in the pathogenesis of many organ-specific autoimmune diseases in animal models and an increase in IL-17 expression has been associated with human autoimmune diseases including multiple sclerosis1,2, rheumatoid arthritis3 and psoriasis4. Furthermore, IL-17-producing T cells with specificity for myelin antigen have been shown to be more efficient than TH1 cells at transferring autoimmunity in experimental autoimmune encephalomyelitis (EAE), an animal model of multiple sclerosis5. There is great interest in understanding the regulation of TH-17 differentiation. IL-6 and TGF-β are sufficient for differentiating naïve CD4 T cells into IL-17 producing T cells in vitro, and these cytokines are required for TH-17 differentiation in vivo as well6,7. Another crucial factor for the development of pathogenic TH-17 cells is IL-23 since IL-23p19 deficient mice, which show a defect in TH-17 development and are resistant to EAE5,8. Initial studies on TH-17 differentiation, using total CD4+T cells including effector-memory T cell populations, were interpreted to suggest that IL-23 was a differentiation factor for T H-17 cells5,8,9 However, it is now appreciated that naïve CD4+ T cells do not express IL-23R and that IL-23 alone is not capable of driving TH-17 cell differentiation of naïve T cells7. Instead, IL-23 acts on previously differentiated TH-17 cell to expand, stabilize and maintain the TH-17 phenotype5,6,10

In addition to IL-6, IL-21, a member of the IL-2 cytokine family, has been shown to be involved in TH-17 differentiation; in combination with TGF-β, IL-21 induces expression of IL-17, transcription factor RORγt and the IL-23 receptor (IL-23R) in naïve CD4+ T cells. In vivo, IL-21 can generate TH-17 cells even in IL-6-deficient mice, and both IL-21-deficient and IL-21R-deficient mice are defective in generating TH-17 cells. Furthermore, once they have developed, TH-17 cells secrete high amounts of IL-21, which then acts to amplify the TH-17 response in an autocrine fashion11,12.

However, TH-17 cells are not the only T cells that produce IL-21. Another type of CD4+ T helper cell, T follicular helper cells (TFH cells), also produces high amounts of this cytokine13-14 The T cell-dependent B cell response occurs within particular structures in the secondary lymphoid organs, the germinal centers (GC). TFH cells provide cognate help to B cells in the GC dynamic microenvironment that results in somatic hypermutation, class switch recombination and selection of high-affinity B cells15,16. TFH cells have been shown to be distinct from conventional T helper cells (e.g., TH1 and TH2 cells) and were first characterized based on expression of the chemokine receptor CXCR5. After antigen activation, TFH cells begin to express CXCR5 while downregulating expression of CCR7, which enables the cells to respond to the follicle-associated chemokine CXCL13. CXCR5+CD4+ TFH cells then migrate to follicles where they support GC formation and B cell responses. TFH cells express other activation markers as well, including CD69, CD95, CD40L, and inducible T cell costimulator (ICOS), which has been implicated in TFH cell development 17,18

Concerning the functional role of ICOS for development of T helper cells besides TFH cells, previous work has suggested that ICOS is also essential for TH-17 cell development9. ICOS is a member of the CD28 family of coreceptor molecules that is induced on T cells after activation19; its ligand ICOS-L (B7h, GL50, LICOS, B7RP-1) is constitutively expressed at low levels on B cells, macrophages and dendritic cells, and ICOS-L expression is further upregulated upon activation of these cells. Although ICOS- and ICOS-L-deficient mice have defects in CD4+ T helper cell responses, it is unclear where ICOS acts in TH-17 cell developmental pathway and if ICOS affects the differentiation, amplification or maintenance and/or stabilization of TH-17 cells.

As mentioned above, ICOS also plays a role in controlling TFH cell development and function. Both ICOS-deficient and ICOS-L-deficient mice have defects in humoral immunity characterized by decreased levels of IgE and IgG1 in the serum and defects in antibody class switching and in GC formation20,21. In addition, patients who have a total defect in ICOS expression, ICOSnull patients, exhibit a profound defect in B cell maturation and immunoglobulin isotype switching22,23; such ICOS deficiency is associated with an impaired development of CXCR5+ TFH cells and humoral immune responses both in humans and mice24,25. Both TFH and TH-17 cells produce IL-21, a cytokine required for the amplification of TH-17 cells. Here we examined the relationship between TH-17 and TFH cells with the aim of shedding new light on the role of ICOS in these T helper cells. Although initial work suggested that ICOS was critical for TH-17 differentiation9, this study preceded our current understanding of the steps involved in TH-17 cell differentiation30.

In the study here we demonstrate that TH-17 cell differentiation from naive CD4+ T cells did not require ICOS, instead ICOS was critical for TH-17 maintenance and function by regulating IL-21 production, which contributes to the expression and the maintenance of IL-23R. Furthermore, we found that both TH-17 cells and TFH cells express high relative levels of the transcription factor c-Maf and that loss of c-Maf results in a defect in IL-21 production and expansion of TH-17 and TFH cells, similar phenotypes to those produced by loss of ICOS. Thus, c-Maf induced by ICOS regulates IL-21 production that, in turn, regulates expansion of TH-17 cells and TFH cells.

RESULTS

ICOS is not crucial for TH-17 differentiation

ICOS is important for T cell effector function, especially for the development of TH2 responses26,27 and it was recently suggested that ICOS also plays a role in the differentiation of Th17 cells9. To reassess a role for ICOS in the primary differentiation of TH-17 cells, we sorted naïve CD4+CD62Lhigh T cells from wild-type or ICOS-deficient (Icos-/-) B6 mice and differentiated them in vitro in the presence of IL-6 and TGF-β. After 5 days of culture in these conditions, we observed a similar frequency of IL-17 secreting cells in Icos-/- and wild-type CD4+T cell cultures (Fig. 1a) and similar amounts of IL-17 cytokine production as detected by ELISA (Fig. 1b). These results indicate that ICOS is not required for primary TH-17 differentiation in vitro.

Figure 1
ICOS is not crucial for T -17 differentiation in vitro

As TH-17 cells have been shown to be the major pathogenic population in the induction of EAE and other autoimmune diseases5,28,29, we next studied the role of ICOS in driving TH-17 differentiation during the course of EAE. We analyzed the priming of T cells following immunization of wild-type and Icos-/- mice with MOG35-55 peptide emulsified in CFA. Draining lymph nodes (dLN), spleen and central nervous system (CNS; brain and spinal cord) of the animals were harvested during the priming phase at day 10 post-immunization, before any clinical signs of disease (Fig. 2). Intracellular cytokine staining showed an equivalent frequency of CD4+ splenocytes that produced IL-17 or IFN-γ in wild-type and Icos-/- mice. Interestingly, CD4+ T cells in the dLN of Icos-/- mice showed an even higher production of IL-17 compared to wild-type mice (5% versus 2.5%) but the percentage of IFN-γ producing CD4 T cells was not significantly different between the two strains. Furthermore, when we analyzed the CD4+ T cells infiltrating the CNS, we noticed that there were more CD4+ T cells producing IL-17 in Icos-/- mice as compared to WT mice (56% versus 36%) (Fig. 2a). However, this increased frequency in TH-17 cells did not persist throughout the course of disease. When we analyzed the mice after the first signs of disease or at the peak of the disease, the percentage of IL-17 cells is about the same in wild-type and Icos-/- mice (data not shown).

Figure 2
ICOS is not crucial for TH-17 differentiation in vivo nor for induction of acute EAE

We also compared the antigen specific responses of wild-type and Icos-/- CD4+ T cells to MOG35-55 peptide. For this we immunized wild-type and Icos-/- mice with MOG35-55 peptide emulsified in CFA, harvested the draining lymph nodes 5 days after immunization and cultured the cells in the presence of the immunizing peptide. In these conditions, lymph node cells from the Icos-/- mice showed a higher proliferation in vitro in response to the immunizing antigen than the cells from wild-type mice (Fig. 2b) and produced more IL-17, less IL-10, but the same amount of IFN-γ, as detected by cytokine ELISA or intracellular cytokine staining (Fig. 2c,d). This difference in the priming of T cells is associated with a slight, but a significant increase in severity of EAE in Icos-/- mice (Fig. 2e). There were no differences in the incidence of the disease but the mean maximum disease score was higher in Icos-/- mice as compared to wild-type mice (3.42 ± 0.92 versus 2.5 ± 0.53) (Table 1). Taken together, these data suggest that co-stimulation of CD4+ T cells by ICOS is not required for the differentiation or priming of TH-17 cells or for the development of acute EAE. These results are consistent with previously published results, where Icos-/- mice were shown to have a more severe form of EAE20 that was associated with decreased IL-10 and increased IL-17 production during the acute phase of the disease.

Table 1
EAE in wild-type and ICOS KO mice

Because TH-17 cells have been shown to be constitutively present in the intestinal lamina propria30, we analyzed the presence of IL-17-producing T cells in the gut of Icos-/- mice. We found considerable variability in the frequency of IL-17-producing cells in the gut of Icos-/- and wild-type mice and there were no significant differences in the frequency of TH-17 cells in the gut of these mice. Thus, ICOS may not be the critical regulator of TH-17 cells in the gut (Supplementary Fig. 1a).

IL-17 expression in TFH cells

Because IL-21 is a cytokine associated with both TFH and TH-17 cells, we examined whether there is a functional relationship between these two CD4+ T helper cell subsets. To address this question, we immunized C57BL/6 wild-type mice with MOG35-55 peptide emulsified in CFA. At day 6 we harvested the dLN and spleen and sorted the cells based on the expression of CD4, CXCR5 and ICOS. Subsequently, we stimulated the cells for 4 hours with PMA-ionomycin and compared the expression of TH-17 cell-associated molecules such as IL-21, IL-17 and IL-23R in TFH cells (CD4+ICOShighCXCR5+) and non-TFH cells (CD4+CXCR5-) by RT-PCR. Consistent with what has been previously reported31, we detected a higher IL-21 expression in TFH cells compared to non-TFH cells. Additionally, compared to non-TFH cells, we could also detect higher expression of IL-17 and IL-23R in TFH cells derived either from lymph node or spleen (Fig. 3a). Furthermore, in vitro expansion of T cells from naive mice, by stimulation with anti-CD3 and IL-23, resulted in a higher proportion of IL-17-producing cells among TFH cells (5 fold) compared to the CD4+CXCR5- (non-TFH cell) fraction (8% versus 2%), whereas these cell populations contained similar percentages of IFN-γ producing cells (Fig. 3b).

Figure 3
TFH cells produce IL-17

The above data showed that TFH cells in wild-type mice are enriched in the expression of IL-17 production. However, one interpretation of the data is that higher expression of IL-17 in TFH cells compared to that in CD4+CXCR5- non-TFH cells could simply be due to the extent of activation of the cells. Indeed, TFH cells consist of uniformly activated CD4+ cells, whereas CD4+CXCR5- T cells consist of a mixture of activated and non-activated T cells. To resolve this issue, we sorted three different T cell populations from dLN and spleen of immunized mice: CD4+ICOShiCXCR5+ TFH cells, activated CD4+ICOShiCXCR5- and non-activated CD4+ICOSloCXCR5- T cells, and then compared the expression of IL-21, IL-17 and IL-23R in these cell fractions. As anticipated, the expression of IL-17, IL-21 and IL-23R in non-activated CD4+ T cells (CD4+ICOSloCXCR5-) was low but when we compared the level of expression in activated CD4+ ICOShi T cells and TFH cells, we detected higher expression of IL-21, IL-17 and IL-23R in the CD4+ICOShiCXCR5+ TFH cells compared to the activated ICOShi effector T cells (Fig. 3c). We then expanded the numbers of the three populations of CD4+ T cells in vitro by stimulating them with IL-12 or IL-23 for 4 days and then we measured cytokines produced by the cells. Under these conditions, CD4+ICOShiCXCR5+ TFH cells produced about 2-fold more IL-17 compared to the activated CD4+ICOShiCXCR5- T cells, whereas when expanded in presence of IL-12 all three cell populations expressed equivalent amounts of IFN-γ (Fig. 3d). These data show that the heterogeneous population of TFH is enriched in IL-17 producing cells that express high level of IL-23R and that are capable of producing substantial amounts of IL-17 in response to IL-23.

Development of IL-17-secreting TFH requires ICOS

As ICOS has been shown to be crucial for the development of TFH cells, IL-21 production and GC formation both in mice24,25 and humans23, we examined the impact of the lack of ICOS in the generation of IL-17-secreting TFH cells. We immunized wild-type and Icos-/- mice with MOG35-55 peptide emulsified in CFA and at day 6 sorted TFH cells based on the expression of CD4 and CXCR5 (Fig 4a). As reported earlier25,32, we observed a profound decrease in the number of CD4+CXCR5+ cells in the dLN and the spleen of Icos-/- mice, though some CD4+CXCR5+ cells were clearly present (Fig 4a.). When we compared the expression of IL-21 and IL-17 in the TFH cells in wild-type mice and the few CD4+CXCR5+ cells in the Icos-/- mice, the latter cells showed substantially decreased IL-21 and IL-17 production, even when adjusted for numbers (Fig. 4b,c).

Figure 4
ICOS-deficient TFH cells are defective in IL-17 production

Because TFH cells are characterized by the expression of ICOS and CXCR5, it is not possible to sort TFH cells from the Icos-/- mice on the basis of a CXCR5+ICOShi phenotype. Therefore to clearly address the role of ICOS-ICOSL pathway on the development of IL-17 producing TFH cells, we also analyzed the production of IL-17 and IL-21 in TFH cells (CD4+ICOShiCXCR5+) derived from the Icosl-/- (ICOS-L-deficient) mice. Consistent with the Icos-/- data, TFH cells derived from the Icosl-/- mice showed a defect in the production of IL-21 and IL-17 (Supplementary Fig. 1b).

We also compared the capacity of the TFH cells from wild-type and Icos-/- mice to respond to IL-23. We sorted CD4+CXCR5+ T cells from immunized wild-type and Icos-/- mice and restimulated them with antigen presenting cells (APCs), anti-CD3 and IL-23 for 4 days. We then stained the CD4+CXCR5+ T cells for intracellular expression of IL-17 and IFN-γ. Compared to TFH cells from wild-type mice, TFH cell from Icos-/- mice produced much less IL-17 but more IFN-γ (Fig. 4d). Finally, because the data indicated that ICOS was required for IL-17 production by TFH cells, we measured IL-23R expression by RT-PCR in sorted TFH cells from dLN and spleen from wild-type and Icos-/- mice to determine the importance of IL-23R for IL-17 production. Indeed, we found a profound decrease in IL-23R expression in Icos-/- TFH cells (Fig. 4e). We also observed a similar defect in IL-23R expression in TFH (CD4+ICOShiCXCR5+) cells from ICOS-L-deficient mice (Supplementary Fig.1b). These data show that ICOS is important for the generation of the IL-17-producing TFH cells, but not IFN-γ-producing T cells, and that TFH cells are compromised in Icos-/- mice.

Defective secondary TH-17 responses of Icos-/- T cells

Since Icos-/- had no defect in TH-17 differentiation in the presence of IL-6 plus TFG-β, we compared the responsiveness of Icos-/- and wild-type T cells to IL-23. We first cultured total CD4+ T cells from unimmunized wild-type or Icos-/- mice in the presence of IL-23 to expand in vivo differentiated TH-17 cells. During activation in the presence of IL-23, we observed a decrease in expansion of IL-17-producing cell numbers in Icos-/- mice (Fig. 5a). Since in vivo differentiated TH-17 cells reside in the memory pool of T cells, we sorted the subset of effector-memory CD62LloCD4+ T cells from unimmunized WT and Icos-/- mice and then stimulated the cells with IL-23. Under these conditions we found that the reduced numbers of TH-17 cells was even more profound: Icos-/- effector-memory CD4+ T cells produced 5-fold less TH-17 cells in presence of IL-23 compared to wild-type effector-memory CD4+ T cells (Fig 5a). To further study this effect of ICOS-deficiency, we differentiated naive wild-type or Icos-/- CD4+ T cells with IL-6 and TGF-β in vitro for 5 days and then further cultured the cells in the presence of IL-23 for another 3-4 days: under these conditions, Icos-/- CD4+ T cells yielded a 2- to 3-fold lower frequency of IL-17-producing T cells than did wild-type CD4+ T cells (Fig. 5b). Moreover, IL-17-producing CD4+ T cells in the dLN from wild-type mice immunized with MOG35-55 peptide expanded in numbers in the presence of IL-23 ex vivo (5-7% to ∼30%), IL-17 producing CD4+ T cells from Icos-/- mice did not expand further in the presence of IL-23 (Fig. 5c). Thus, these data suggest that Icos-/- cells do not have a primary defect in TH-17 differentiation, but rather exhibit a defect in the expansion in cell numbers in response to IL-23.

Figure 5
ICOS-deficient T cells show a defect in secondary TH-17 responses

We next investigated whether IL-23 unresponsiveness was a reflection of reduced expression of IL-23R or reduced production of IL-21 during TH-17 differentiation. At the end of the differentiation, naive CD4+ T cells from Icos-/- mice differentiated in the presence of IL-6 and TGF-β showed, at day 5, 50% lower IL-23R expression but only a slight decrease in the expression of the IL-12Rβ1 common chain, when compared to wild-type TH-17 cells (Fig. 5d) whereas the percentage of IL-17-producing cells and the amount of IL-17 mRNA expression were equivalent in both cultures (data not shown). Those data were consistent with our observation that there is no defect in TH-17 differentiation in Icos-/- TH-17 (Fig. 1) and, furthermore, that differentiating TH-17 cells express lower amount of IL-23R. These data suggest that costimulation of conventional TH-17 cells through ICOS is necessary for either maximal IL-23R expression or maintenance of IL-23R expression. We also observed decreased IL-21 and IL-22 production by Icos-/- TH-17 cells (Fig. 5e and Supplementary Fig. 1c) during the primary differentiation with IL-6 and TGF-β. Because IL-21 has been implicated not only in TH-17 differentiation but also in IL-23R upregulation, it is possible that reduced expression of IL-23R in Icos-/- mice is secondary to reduced production of IL-21 by T cells.

ICOS regulates IL-21 production via c-Maf

To understand the mechanism by which ICOS regulates IL-21 production and differentiation of TH-17, and potentially TFH, cells, we undertook a microarray analysis of differentiated TH-17 cells. The result showed that transcription factor c-Maf was upregulated in TH-17 cells (data uploaded on ArrayExpress). As c-Maf has been shown to be downstream ICOS, we wondered whether c-Maf could be involved in TH-17 differentiation by regulating IL-21 and IL-23R expression. We first differentiated naïve CD4 T cells into TH-17 cells and observed that TH-17 cells differentiated with IL-6 plus TGF-β or IL-21 plus TGF-β expressed c-Maf and this expression was further increased by exposure to IL-23 (Fig. 6a). Expression of c-Maf in TH-17 cells was over 500 times higher than that of TH1 or TH2 cells. Similarly CD4+ICOShiCXCR5+ TFH cells showed higher expression of c-Maf compared to CD4+ICOShiCXCR5- and CD4+ICOSloCXCR5- non-TFH cells (Fig. 6a). We then measured c-Maf expression during TH-17 differentiation in Icos-/- cells that were stimulated with wild-type APC in presence of IL-6 and TFG-β. We found that Icos-/- TH-17 cells did not upregulate c-Maf expression, confirming the previously published observation that ICOS is crucial for c-Maf upregulation in TH0 effector cells35. Because c-Maf regulation occurs ‘downstream’ of ICOS signaling, we tested if c-Maf-deficient cells “phenocopy” ICOS-deficient cells. For this, we differentiated naïve CD4 T cells from c-Maf-deficient mice in the presence of IL-6 plus TGF-β for 4 days and then evaluated the frequency of IL-17-secreting cells. We observed a similar frequency of IL-17-secreting c-Maf-deficient and IL-17-secreting wild-type CD4+ T cells (Fig. 6b). Similar to ICOS, then, c-Maf is not required for TH-17 differentiation.

Figure 6
c-Maf in TH-17 differentiation

However, we speculated that, like ICOS, c-Maf would be required for maintenance of IL-17-producing cells after they have been differentiated. To test this we restimulated the naïve CD4 T cells from c-Maf-deficient mice above, stimulated with IL-6 and TGF-β for 4 days, with IL-23 for an additional 3 days. Again, like ICOS-deficient T cells, c-Maf-deficient T cells yielded a 2 fold lower frequency of IL-17-producing T cells compared to wild-type T cells (Fig. 6c). This decrease in the frequency of IL-17+ T cells in c-Maf-deficient mice was further confirmed by the production of IL-17 detected by ELISA (Fig. 6c). We also measured IL-23R expression during differentiation of c-Maf-deficient cells under TH-17 polarizing conditions (IL-6 and TGF-03 for 4 days). At an early time-point during primary differentiation (d3) of the cells we detected the same level of IL-23R expression in c-Maf-deficient and wild-type cells; however after secondary expansion (+ IL-23 for additional 4 days), expression of IL-23R was lower in c-Maf-deficient cells which correlates with the decrease in the frequency of the TH17 cells (Fig. 6d). Finally, because ICOS-deficient mice have a defect in IL-21 production, we also analyzed IL-21 production by c-Maf-deficient cells polarized under TH-17 conditions. Similar to ICOS-deficiency again, IL-21 production by c-Maf-deficient cells was reduced compared to wild-type cells (Fig. 6e). These data suggest that c-Maf is not necessary for inducing transcription of IL-23R, but more likely for maintaining IL-23R expression by inducing IL-21.

Because IL-21 has been shown to be crucial for GC formation and TFH development, we also investigated whether c-Maf was involved in the development of the TFH cells. For this, we immunized wild-type and c-Maf-deficient mice with TNP-OVA emulsified in CFA and analyzed the draining lymph nodes and the spleen after 7 days. We observed a profound decrease in the number of CD4+ICOShiCXCR5+ cells present in the dLN (Fig 6f) and the spleen of c-Maf-deficient mice (data not shown). Taken together, these data indicate that c-Maf participates in TFH cells and TH-17 development most likely by regulating IL-21 production.

DISCUSSION

In this study we demonstrated that conventional TH-17 cells do not require ICOS costimulation for their differentiation or to acquire pathogenic potential to induce EAE, but rather that ICOS is necessary for the IL-23-driven expansion of already differentiated TH17 cells. We further show that the defect in expansion of differentiated TH-17 cells and in development of IL-17-secreting TFH cells in ICOS-deficient mice is in part due to a defect in the upregulation of a transcription factor c-Maf. ICOS-deficient and c-Maf-deficient TH-17 cells show a decrease of IL-21 production and consequently a decrease in IL-23R expression, suggesting that ICOS may be involved in regulating IL-23R expression in differentiating TH-17 and TFH cells via the transcription factor c-Maf. c-Maf induced by ICOS must regulate IL-21 production which participates to amplify TH-17 cells and stabilizes these cells by inducing IL-23R expression. Since IL-23 is critical for expanding and maintaining IL-17 production, this highlights one of the mechanisms by which ICOS may regulate IL-21, IL-17 and TFH cell development by regulating c-Maf expression.

It was first proposed that ICOS is required for TH-17 cell differentiation9H. However, since ICOS-deficient mice are more susceptible to EAE than are wild-type mice20 and TH-17 cells are critical for the induction of EAE, these paradoxical results raised the question at which step ICOS is required for TH-17 development. Using ICOS-deficient mice we re-analyzed the role of ICOS in various steps of TH-17 differentiation. In vitro, there is no defect in acute TH-17 differentiation in Icos-/- mice. On the contrary, in vivo, in immunized mice there is an increase in IL-17 production and a decrease in IL-10 production during the priming phase in Icos-/- mice and this may be one of the reasons why Icos-/- mice show increased susceptibility to EAE. This observation is consistent with previous reports showing that Icos-/- mice are more susceptible to EAE and experimental autoimmune uveoretinitis20,36. Our studies indicate that the increased susceptibility to EAE and EAU is not due to primary defect in the generation of TH-17 cells following immunization, but most likely due to loss of IL-10-producing T cells. Indeed, IL-10 secretion by T cells is stimulated by ICOS signaling19,37,38 and IL-10 is a key immunoregulatory cytokine involved in the induction of T regulatory type 1 (Tr1) cells, the function of Foxp3+ Treg cells and the suppression of autoimmunity39,40.

Icos-/- mice have been shown to have a defect in the development of TFH cells and here we show that they have a defect in IL-21 production. Since IL-21 is an amplification factor for TH-17 cells and is produced at high levels by TFH cells, we examined the link between TH-17 cells and TFH cells and observed an enhanced expression of molecules associated with TH-17 cells, including IL-17, IL-21 and IL-23R, in IL-17-producing TFH cells. IL-17 has previously been associated with the development of autoantibody responses and deficiency in IL-17 or blockade of IL-17 also has been shown to decrease autoantibody responses29,41. A recent study further showed that IL-17 is crucial for autoreactive germinal center development in autoimmune BXD2 mice. In that study, IL-17-producing T cells and IL-17R+ B cells were found co-localized in GCs and IL-17 was shown to play a role in GC formation in vivo42. This suggests that IL-17 not only induces tissue inflammation by acting on the IL-17R expressed on the parenchymal and other tissue cells, but it could also function on B cells to promote the GC reaction. Since a fraction of CXCR5- and ICOS-expressing TFH cells were IL-17-producing cells, our results suggest that the IL-17 producing cells observed by Hsu et al42 are most likely TFH cells.

The crucial role of ICOS in GC development and TFH generation is well established; ICOS- or ICOS-L-deficient mice develop fewer and smaller GC after immunization, associated with impaired T cell-dependent B cell responses and impaired isotype class switching20,21,43,44.More recently, similar impairments in B cell responses have been reported in ICOS-deficient patients25. Furthermore, Sanroque mice, which carry a disruptive mutation in roquin, a repressor of ICOS, develop severe autoimmune, lupus-like disease associated with high expression of IL-21, accumulation of CXCR5+ICOShi T cells, increased formation of GC and increased production of auto-antibodies45,46. Whether these mice also show enhanced expression of IL-17- and TH-17-associated genes in the TFH cells has not been addressed, but our results suggest that part of the phenotype observed in the Sanroque mice may also be due to enhanced IL-17 production by TH-17 and TFH cells. Taken together, these observations suggest that the defects in the number of TFH cells and in GCs reaction, as well as a defect in class switching, in ICOS-deficient mice and ICOS-deficient patients may partly be due to a defect in IL-21 production which acts as an autocrine growth factor to expand TFH cells.

Upon antigen-specific activation and differentiation, TH-17 cells may have several different fates: a population of differentiated TH-17 cells become effector TH-17 cells, downregulate CCR7, upregulate CCR6 and migrate to the target organs where they mediate their effector function54; some TH-17 cells maintain the expression of CCR7, stay in the secondary lymphoid organs and become IL-17-producing central memory cells; and a population of TH-17 cells that express high level of ICOS and IL-23R, that downregulate CCR7 and upregulate CXCR5, become part of the heterogeneous TFH cell pool that migrates to follicles where they interact with B cells to induce GC formation. Our data suggest that ICOS mediates TFH cell development most likely by regulating IL-21 production, and consequently could act indirectly to regulate the IL-23R expression on these cells. This raised an issue of how ICOS regulates IL-21 expression and expansion of TH-17 cells and TFH cells. Our data suggest that the transcription factor c-Maf, which is downstream of ICOS, regulates IL-21 production and subsequently IL-23R expression in developing TH-17 and TFH cells. The study by Hsu et al. found enhanced production of IL-23 by non-lymphoid cells with increased numbers of TFH cells in the spleen of autoimmune BXD2 mice42, suggesting that IL-23 may be important for expansion of IL-17+ TFH cells as well. Whether there is a generalized defect in TFH cells in IL-23R-deficient mice or just IL-17-producing cells remains to be clarified. Nevertheless, our observations suggest a role for ICOS in regulating IL-23R expression and IL-17 production by TH-17 cells and TFH cells. Therefore, a decrease in TFH and TH-17 cell responses in ICOS-deficient might be due to a defect in c-Maf upregulation, IL-21 production and consequently a defect in upregulation of IL-23R on TH-17 and TFH cells. Whereas IL-21 and IL-23 are not crucial for initial TH-17 differentiation, they are crucial for expansion and maintenance of differentiated TH-17 cells. Since our data show that ICOS regulates IL-23R on differentiating TH-17 cells, lack of IL-23R upregulation in ICOS-deficient cells might be one of the reasons why ICOS-deficient mice show a defect in memory TH-17 responses. ICOS has previously been shown not only to costimulate T cell activation, but also induce T cell survival in other T cell subsets47,48. It is likely that ICOS is playing a similar role in survival of TFH cells as well by regulating IL-21 production and IL-23R expression in IL-17-secreting TFH cells. Taken together our data suggest that ICOS regulates the fate of differentiated IL-17-producing T cells via induction of c-Maf transcription factor that in turn induces IL-21.

METHODS

Animals and induction of EAE

ICOS-deficient (Icos-/-) mice were backcrossed onto the C57BL/6 background for 10 generations. Genotyping of Icos-/- mice was performed by PCR as previously described49. Chimeric c-Maf-deficient (Maf-/-) mice were generated in the laboratory of I-Cheng Ho by reconstituting RAG-deficient (Rag-/-) Balb/c mice with fetal liver cells from c-Maf-deficient mice. All mice for experiments were 8-12 wk old. EAE was induced by injecting mice subcutaneously (into the flanks) with 100 μl of an emulsion containing 100 μg of MOG35-55 peptide (MEVGWYRSPFSRVVHLYRNGK) and 250 μg of M. tuberculosis extract H37-Ra (Difco) in Complete Freund's Adjuvant (CFA). In addition, mice received 200 ng of pertussis toxin (List biological Laboratories via Cedarlane Ltd) intraperitoneally (i.p.) on days 0 and 2. Clinical signs of EAE were assessed according to the following score: 0, no signs of disease; 1, loss of tone in the tail; 2, hind limb paresis; 3, hind limb paralysis; 4, tetraplegia; 5, moribund. Mice were kept in a conventional pathogen-free facility at the Harvard Medical School. All experiments were carried out in accordance with guidelines prescribed by the Institutional Animal Care and Use Committee (IACUC) at Harvard Medical School.

Preparation of CNS mononuclear cells

Mice were perfused through the left cardiac ventricle with cold PBS. The forebrain and cerebellum were dissected and spinal cords flushed out with PBS by hydrostatic pressure. CNS tissue was cut into pieces and digested with collagenase D (2.5 mg/ml, Roche Diagnostics) and DNaseI (1 mg/ml, Sigma) at 37 °C for 45 min. Mononuclear cells were isolated by passing the tissue through a cell strainer (70 m), followed by a percoll gradient (70%/37%) centrifugation. Mononuclear cells were removed from the interphase, washed and resuspended in culture medium for further analysis.

T cell proliferation

For proliferation assays, mice were immunized with peptide-CFA as described above. A single-cell suspension was prepared from the draining lymph nodes or spleens on day 5 after immunization. Cells were cultured in DMEM-10% FCS supplemented with 5 × 10-5 M mercaptoethanol, 1 mM sodium pyruvate, nonessential amino acids, L-glutamine, and 100 U penicillin/100 g streptomycin per ml. During the last 16 h, cells were pulsed with 1 μCi of [3H]thymidine (PerkinElmer) followed by harvesting on glass fiber filters and analysis of incorporated [3H]thymidine in a β-counter (1450 Microbeta, Trilux, PerkinElmer).

Intracellular cytokine staining

For intracellular cytokine staining, cells were isolated as described above and stimulated in culture medium containing phorbol 12-myristate 13-acetate (PMA, 50 ng/ml, Sigma), ionomycin (1 μg/ml, Sigma) and monensin (GolgiStop 1 μl/ml, BD Biosciences) at 37 °C, in a humidified 10% CO2 atmosphere for 4 h. After staining of surface markers (CD4), cells were fixed and permeabilized using Cytofix-Cytoperm and Perm/Wash buffer (BD Biosciences) according to the manufacturer's instructions. All antibodies to cytokines (IFN-γ, IL-17, IL-10) including the corresponding isotype controls were obtained from BD Biosciences and used a 1:200 dilution. Cells were incubated at 4 °C for 20 min and washed twice in Perm-Wash before analysis.

Cytokine ELISA

Lymph nodes cells from immunized mice were cultured with MOG35-55 peptide (100μg/ml). Supernatant from the cultures were harvested 48 hours after activation and secreted cytokines were determined by Enzyme-linked ImmunoSorbent assay using purified coating and biotinylated detection antibodies for IL-17 (R&D Systems), IFN-γ and IL-10 (BD Bioscience). Detection antibodies were measured using horseradish peroxidase-conjugated streptavidin (Endogen), developed using 3.3',5.5'-Tetramethyl-benzidine (TMB) liquid substrate system (SIGMA) and stopped with 0.5M H2SO4.

In vitro T cell differentiation

Spleen cells from 2D2 mice were stimulated with 50 μg/ml MOG35-55 peptide in the presence or absence of IL-23 (20 ng/ml). For differentiating naïve T cells in vitro, CD4+ T cells were purified using anti-CD4 beads (Miltenyi) or further FACS sorted into naive CD4+CD62Lhi cells. CD4+ T cells were stimulated with C57BL/6 irradiated spleen cells and 1 μg/ml of anti-CD3 (145-2C11) for 3-5 days in the presence of cytokines: human TGF-β1 (3 ng/ml), mouse IL-6 (20 ng/ml) or IL-23 (20 ng/ml) (all R&D Systems) for TH-17 differentiation, mIL-12 (5ng/ml; BD Pharmingen) and anti-mIL-4 (10 μg/ml, clone 11B11) for TH1 differentiation and mIL-4 (10 ng/ml; R&D system) and anti-m-IL-12 (10 μg/ml, BD Pharmingen) for TH2 differentiation.

Real-time PCR

RNA was extracted using the RNAeasy columns (Qiagen). Complementary DNA was transcribed as recommended (Applied Biosystems) and used as template for quantitative PCR. The expression of IL-17, IL-21, IL-23R was determined using specific primers and probes (Applied Biosystems). The Taqman analysis was performed on the AB 7500 Fast System (Applied Biosystem). The gene expression was normalized to the expression of the housekeeping gene β-actin.

Microarray analysis

Mouse spleen CD4+CD44LowCD62LHigh cells were stimulated with 2ug/ml anti-CD3 (eBioscience), 2ug/ml anti-CD28 (eBioscience) in the presence (TH-17 condition) or absence (TH0 condition) of hTGFβ-1 (1ng/ml eBioscience) and mouse IL-6 (10ng/ml eBioscience). Cells were collected after 24 hours of culture using RNAeasy columns (Qiagen) for total RNA isolation. Isolated total RNA from TH0 and TH-17 conditioned cells were submitted for the microarray gene transcription comparison analysis using Affymetrix Mouse 430A 2.0 array chips.

Statistical evaluation

Statistical evaluations of cell frequency measurements were performed using the unpaired Student's t-test for samples with unknown and potentially disparate variances.

ACKNOWLEDGEMENT

We thank D. Kozoriz for cell sorting. Anneli Jaeger, Sue Liu and Loise Francisco for useful comments. This work was supported by the National Institutes of Health (1R01NS045937-01, 2R01NS35685-06, 2R37NS30843-11, 1R01A144880-03, P01NS38037-04 and 1R01NS046414 to V.K.K. 2P01A139671-07 and 1P01AI56299 to V.K.K. and A.H.S, and R37 AI38310 to A.H.S) and National Multiple Sclerosis Society (RG-2571-D-9) and the European Commission as a Marie Curie postdoctoral fellowship to A.B. M.M. is supported by the Deutsche Forschungsgemeinschaft. V.K.K. is a recipient of the Javits Neuroscience Investigator Award from the US National Institutes of Health.

Supplementary Material

Splmnt Fig

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