Cutting Edge: NKT Cells Constitutively Express IL-23 Receptor and ROR{gamma}t and Rapidly Produce IL-17 upon Receptor Ligation in an IL-6-Independent Fashion

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Cutting Edge: NKT Cells Constitutively Express IL-23 Receptor and ROR ${gamma}$ t and Rapidly Produce IL-17 upon Receptor Ligation in an IL-6-Independent Fashion¹

Aleksandra V. Rachitskaya²^,*^,, Anna M. Hansen²^,*, Reiko Horai^*, Zhuqing Li^*, Rafael Villasmil^*, Dror Luger^*, Robert B. Nussenblatt^* and Rachel R. Caspi³^,*

^* Laboratory of Immunology, National Eye Institute, National Institutes of Health, Bethesda, MD 20892; and Howard Hughes Medical Institute-National Institutes of Health Research Scholars Program, Bethesda, MD 20814

Abstract

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Abstract
Introduction
Materials and Methods
Results and Discussion
Disclosures
References

Th17 cells require IL-6 and TGFβ for lineage commitmentand IL-23 for maintenance. Unexpectedly, naive IL-6^–/–splenocytes stimulated with anti-CD3 and IL-23 produced normalamounts of IL-17 during the first 24 h of culture. These rapidIL-6-independent IL-17 producers were identified as predominantlyDX5⁺ TCRβ⁺ NKT cells, and a comparable response could befound using the invariant NKT-specific ligand ${alpha}$ -galactosylceramide.Human NKT cells also produced IL-17. NKT cells constitutivelyexpressed IL-23R and ROR ${gamma}$ t. Ligation of either TCR or IL-23Rtriggered IL-17 production and both together had a synergisticeffect, suggesting independent but convergent pathways. IL-17production was not restricted to a particular subset of NKTcells but they were NK1.1 negative. Importantly, in vivo administrationof ${alpha}$ -galactosylceramide triggered a rapid IL-17 response in thespleen. These data suggest an important biological role forinnate IL-17 production by NKT cells that is rapid and precedesthe adaptive IL-17 response.

Introduction

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Abstract
Introduction
Materials and Methods
Results and Discussion
Disclosures
References

Interleukin 17A is a major proinflammatory cytokine producedby a newly described lineage of helper T cells, Th17 cells.These cells are reported to require IL-6 and TGFβ for lineagecommitment and IL-23 for maintenance (1, 2) and have been implicatedas major effector cells in such prototypic murine models ofautoimmunity as experimental autoimmune encephalomyelitis andcollagen-induced arthritis (3, 4).

NKT cells are unique cells of the innate immune system thatare defined by coexpression of NK lineage markers, such as NK1.1and CD49b/DX5 in mice and CD56 in humans, with a TCR (5) andare characterized by their ability to rapidly produce immunoregulatorycytokines, such as IL-4 and IFN- ${gamma}$ , upon engagement of their TCR(6). Although there is still some debate over what defines anNKT cell, they are currently divided into three categories basedon their reactivity to the glycolipid ${alpha}$ -galactosylceramide ( ${alpha}$ -GalCer),⁴TCR ${alpha}$ -chain diversity, and CD1d dependency. Type I classical"invariant" NKT cells (iNKT cells) have invariant V ${alpha}$ 14-J ${alpha}$ 18 TCR ${alpha}$ -chains and react to ${alpha}$ -GalCer in a CD1d-dependent manner. TypeII nonclassical NKT cells do not react to ${alpha}$ -GalCer and have diverseTCR ${alpha}$ -chains but are also CD1d dependent. Type III NKT cellsare CD1d independent, do not respond to ${alpha}$ -GalCer, and possessdiverse TCR ${alpha}$ -chains.

In the present study we initially set out to examine the roleof IL-6 in the production of IL-17 in the primary immune responseby using anti-CD3 and IL-23 stimulation. In contrast to thepreviously reported critical role of IL-6 in the differentiationof Th17 cells, we found that during the first 24 h of stimulationIL-6-knockout (IL-6 KO) splenocytes produced as much IL-17 aswild-type (WT) splenocytes. Detailed characterization revealedthat this early IL-6-independent IL-17 production originatedlargely from NKT cells. We show here for the first time thatIL-6 is not required for innate IL-17 production by NKT cells.Consistent with this, NKT cells constitutively express IL-23Rand ROR ${gamma}$ t, similarly to memory T cells and unlike NK and naiveT cells. IL-17 production is triggered by ligation of eitherthe TCR alone or the IL-23R alone, and engagement of both hasa synergistic effect. We show for the first time that humanNKT cells produce IL-17 upon stimulation and that the administrationof an iNKT ligand, ${alpha}$ -GalCer, to mice results in a rapid IL-17response in the spleen, suggesting evolutionary conservationand in vivo relevance of this phenomenon.

Materials and Methods

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Abstract
Introduction
Materials and Methods
Results and Discussion
Disclosures
References

Mice

C57BL/6 (WT) and IL-6 KO mice were purchased from The JacksonLaboratory. J ${alpha}$ 18 KO mice, CD1d KO mice and IL-23 receptor KOmice were generated as previously described (7, 8, 9) and maintainedin the animal facilities of the National Institutes of Healthin Bethesda MD or the National Institutes of Health in Frederick,MD in full compliance with institutional guidelines.

Flow sorting and intracellular cytokine analysis

Pooled splenocytes from naive mice or human peripheral mononuclearcells from the buffy coat of healthy donors (National Institutesof Health blood bank, protocol no. 99-C-0168) were sorted intoNK, NKT, and T cell populations based on expression of DX5,TCR β-chain, and CD62L using a BD FACSAria cell sorter.iNKT cells were isolated by the binding of CD1d tetramers (ProImmune)loaded with ${alpha}$ -GalCer (Alexis Biochemicals/Axxora). Populationswere enriched by autoMACS (Miltenyi Biotech) before sorting.Final purity was 85–99%. Cells were stained for extracellularand intracellular markers as described (BD Biosciences protocol;www.bdbiosciences.com/pdfs/manuals/00-6088-559311-B.pdf). AllAbs were purchased from BD Biosciences and flow cytometry wasanalyzed using a FACSCalibur (BD Biosciences) and FlowJo software(Tree Star).

Culture conditions

Mouse cell culture was performed in HL-1 medium supplementedwith 1% fresh frozen mouse serum. Cells were stimulated eitherby adding 2.5 µg/ml anti-CD3 (clone 145-2C11) directlyinto cell culture or by using plates precoated with anti-CD3at 10 µg/ml. Where indicated, 10 ng/ml recombinant murineIL-23 was added (R&D Systems). ${alpha}$ -GalCer was used at 100 ng/ml,presented by CD11c-positive cells isolated by autoMACS (MiltenyiBiotech). Mouse IL-17A and IFN- ${gamma}$ protein were detected in supernatantsby DuoSet ELISA-matched Ab pairs (R&D Systems) as per themanufacturer’s instructions.

Purified human NKT cells were stimulated for 24 h with anti-CD3(10 µg/ml; BD Biosciences) cross-linked with anti-mouse-IgG(5 µg/ml; Sigma-Aldrich) and recombinant human IL-23 (100ng/ml; eBioscience). IL-6 was neutralized using goat-anti-humanIL-6 (10 µg/ml; R&D Systems) and effective neutralizationwas confirmed by ELISA. Cytokine levels in supernatants weremeasured by multiplex ELISA (SearchLight; Pierce Biotechnology).

mRNA expression analysis

RNA was isolated using TRIzol (Invitrogen Life Technologies)and an RNeasy mini kit (Qiagen) before reverse transcriptionusing SuperScript III (Invitrogen Life Technologies). Quantitativereal-time PCR was performed using a 7900HT sequence detectionsystem (Applied Biosystems). TaqMan eukaryotic 18S ribosomalRNA endogenous control (VIC/MGB probe) and primer/probe setsfor the murine IL-23 receptor, RORc, IL-17A, and IFN- ${gamma}$ (FAM/MGBprobe) were from Applied Biosystems.

Statistical analysis and data presentation

All experiments were repeated at least twice with identicalresults. Figures show data from representative experiments.Graphs and data analysis were done using GraphPad Prism (GraphPadSoftware).

Results and Discussion

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Abstract
Introduction
Materials and Methods
Results and Discussion
Disclosures
References

Rapid initial production of IL-17 upon primary stimulation is IL-6 independent and derives from NKT cells

Splenocytes from untreated IL-6 KO and WT mice were activatedin vitro by stimulation with anti-CD3 and IL-23. Unexpectedly,there was significant IL-17 production observed by ELISA alreadywithin 24 h of stimulation, which was similar in IL-6 KO andtheir WT counterparts (Fig. 1A). This was in sharp contrastto previous reports that IL-6 was required for IL-17 production(1, 2). Beyond 24 h, IL-17 production by IL-6 KO splenocytesreached a plateau whereas with WT cells it continued to increase,suggesting that the window for IL-6 independent IL-17 productionis brief. The rapid kinetics and unexpected IL-6 independenceof this early IL-17 production suggested a TCR-bearing cellpopulation other than naive conventional T cells. To dissectthis further, naive spleen cells were fractionated by flow sortingbased on expression of TCRβ and the NK cell marker DX5into NKT cells (DX5⁺TCRβ⁺), T cells (DX5^–TCRβ⁺),and NK cells (DX5⁺TCRβ^–) and were stimulated withIL-23 and plate-bound anti-CD3 for 16 h. Analysis of culturesupernatants by ELISA (Fig. 1B) and the cells by intracellularcytokine staining (Fig. 1C) revealed substantial productionof IL-17 by NKT cells. No IL-17 production was detectable inNK cells and only a trace level was found within T cells, whichwas most likely attributable to the memory T cells in this population(as shown in Fig. 2).

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FIGURE 1. Rapid initial production of IL-17 is IL-6 independent and derives from NKT cells in mice and in humans A, Spleen cells from C57BL/6 and IL-6 KO mice were cultured with anti-CD3 and IL-23. IL-17 was measured in culture supernatants by ELISA at the time points indicated. B and C, NKT, NK, and T cells sorted from spleens were stimulated for 16 h with anti-CD3 and IL-23. IL-17 production within these populations was measured by ELISA (B) and intracellular staining (C) for IL-17 protein. D, IL-17 production by sorted NKT cells stimulated with ${alpha}$ -GalCer presented by CD11c⁺ APC. E, IL-17 production by CD56⁺TCRβ⁺ human NKT cells after stimulation with anti-CD3 IL-23, as measured by ELISA. ${alpha}$ -CD3, anti-CD3.

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FIGURE 2. NKT cells constitutively express IL-23R and ROR ${gamma}$ t mRNA, but expression of IL-17A requires triggering by receptor engagement. A, Naive T cells (Tn), memory T cells (Tmem), NK cells, and NKT cells were isolated from untreated mice by FACS. Constitutive levels of IL-23R and ROR ${gamma}$ t mRNA were quantitated in unstimulated cells using real-time PCR. Data were normalized to 18S and expressed relative to expression in naive T cells B, Changes in ROR ${gamma}$ t mRNA were measured 16 h after stimulation. Data are normalized to 18S and expressed relative to expression in unstimulated memory T cells. C, Changes in IL-17A expression in cell populations isolated from WT and IL-6 KO mice as measured by ELISA. All data represent at least three experiments that were highly reproducible. ${alpha}$ CD3, anti-CD3.

Further confirmation that the rapid early IL-17 producers wereNKT cells was obtained by using the iNKT-specific ligand ${alpha}$ -GalCer.Intracellular staining of sorted DX5⁺TCRβ⁺ cells afterstimulation with ${alpha}$ -GalCer and purified CD11c⁺ APC revealed adistinct population of IL-17 producers (Fig. 1D).

Our findings in mice prompted us to investigate innate productionof IL-17 in humans. NKT cells were purified from the buffy coatof healthy human donors and stimulated with human anti-CD3/IL-23for 24 h. Analysis of the supernatants by ELISA for IL-17 contentdemonstrated that human NKT cells, like mouse NKT cells, produceIL-17 without the need for exogenous IL-6 (Fig. 1E). To examinethe IL-6 dependence of this response, we neutralized IL-6 invitro and found no effect on IL-17 production (data not shown).

NKT cells constitutively express the IL-23 receptor and the transcription factor ROR ${gamma}$ t

A crucial role of IL-6 in the differentiation of Th17 cellsis thought to be the up-regulation of the IL-23 receptor (IL-23R)and the Th17 lineage-specific transcription factor ROR ${gamma}$ t (10).The rapidity and IL-6 independence of the IL17 response of NKTcells suggested that they might constitutively express thesemolecules. Previous studies have identified constitutive expressionof IL-23R on memory, but not naïve, T cells (11). We quantitatedboth IL-23R and ROR ${gamma}$ t mRNA expression by real-time PCR in naiveT cells (DX5^–TCRβ⁺CD62L⁺), memory T cells (DX5^–TCRβ⁺CD62L^–),NK cells (DX5⁺TCRβ^–), and NKT cells (DX5⁺TCRβ⁺)sorted from C57BL/6 spleen. The data revealed that IL-23R andROR ${gamma}$ t are constitutively expressed in NKT cells and T memorycells (Fig. 2A). Although ROR ${gamma}$ t was constitutively expressed,no IL-17 production was evident within any population beforestimulation (Fig. 2C). This is consistent with the notion thatexpression of ROR ${gamma}$ t is necessary, but not sufficient, for IL-17production and that a trigger for IL-17 transcription is downstreamof ROR ${gamma}$ t. This is further supported by the finding that despitehigh levels of IL-17 protein found in culture supernatants within16 h of stimulation, the increase in ROR ${gamma}$ t mRNA was quite modest(Fig. 2B), suggesting that constitutive expression could explainmuch of the observed induction of IL-17. Thus, the differentialrequirement for IL-6 in IL-17 induction in naive T cells vsNKT cells can be explained at least in part by constitutiveexpression of IL-23R and ROR ${gamma}$ t observed in the latter. Notably,T cells with memory phenotype displayed a similar ability asthat of NKT cells to rapidly produce IL-17 after TCR ligationin an IL-6-independent manner (Fig. 2C). This suggests that,in a naive host, NKT cells may fill a parallel niche in hostresponse to that filled by memory T cells in an Ag-experiencedhost.

Activation of NKT cells through the TCR and IL-23 receptor is independent but synergistic

We next analyzed the relative contributions of TCR ligationand IL-23 to NKT-derived IL-17 production by using C57BL/6 WTand IL-23R KO mice. Flow cytometric analysis revealed anti-CD3alone and IL-23 alone induced approximately equal numbers ofWT NKT cells to produce similar levels of IL-17, as detectedby ELISA (Fig. 3). Although the combination of both had an additiveeffect on the frequency of IL-17-producing cells, a synergisticeffect in the amount of IL-17 production was evident from boththe mean fluorescence intensity of intracellular IL-17 stainingand by an ELISA of secreted IL-17 protein. IL-17 productionby TCR ligation was unaffected in IL-23R KO NKT cells although,as expected, these cells did not respond to IL-23. These observationssuggest that IL-17 production via TCR activation is not dependenton concomitant IL-23R stimulation and vice versa. However, theadditive/synergistic effect of both signals together would suggestthat they combine quantitatively to control IL-17 levels inthe cell.

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FIGURE 3. Activation of NKT cells through TCR and IL-23 receptor is independent and synergistic. NKT cells isolated from WT C57BL/6 or IL-23R KO mice were stimulated for 16 h with anti-CD3 ( ${alpha}$ CD3) alone, IL-23 alone, or a combination of the two. The frequency of IL-17-producing cells was measured by intracellular staining, and the corresponding IL-17A levels in culture supernatants were quantitated by ELISA.

IL-17-producing NKT cells are not restricted to a particular NKT subset and are NK1.1 negative

NKT cells are currently divided into three types based on theirreactivity to ${alpha}$ -GalCer, TCR ${alpha}$ -chain diversity, and CD1d dependency.iNKT cells (type I), are easily identifiable with ${alpha}$ -GalCer-loaded,labeled CD1d tetramers, but there are no specific reagents toidentify type II (TCR ${alpha}$ diverse and CD1d dependent) and type III(TCR ${alpha}$ diverse and CD1d independent) NKT cells. Therefore, toexamine IL-17 production by all NKT cell types, we used a combinationof iNKT-specific techniques and genetically modified mice. NKTpopulations were sorted based on expression of DX5 and TCRβfrom the spleens of WT C57BL/6 (containing all subsets of NKTcells), J ${alpha}$ 18 KO (lacking iNKT cells), and CD1d KO (lacking bothiNKT and type II NKT cells) mice. IL-17 production in responseto ${alpha}$ -GalCer was evident only in WT mice, confirming that iNKTcells are capable of IL-17 production (Fig. 4A). Notably, NKTcells from both KO mice responded to TCR stimulation with IL-17production, allowing us to conclude that in addition to iNKTcells, type II and type III NKTs are able to produce IL-17 (Fig.4B).

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FIGURE 4. IL-17-producing NKT cells are not restricted to a particular NKT subset and are NK1.1 negative. A and B, NKT cells from C57BL/6, J ${alpha}$ 18 KO, and CD1d KO mice were purified by flow sorting and stimulated for 16 h with ${alpha}$ -GalCer/CD11c (A) or anti-CD3/IL-23 (B). C, IL-17 and IFN- ${gamma}$ production by DX5⁺NK1.1⁺ and DX5⁺NK1.1^– NKT cells sorted from WT C57BL/6 mice and plated at 1 x 10⁶/ml. D, iNKT cells were isolated from C57BL/6 spleen based on CD1d-tetramer stain and further sorted by DX5 and NK1.1 expression. Resulting populations were plated at 2 x 10⁵/ml and stimulated as indicated. Samples were pooled for analysis and data are representative of at least two experiments. ${alpha}$ CD3, anti-CD3.

Following the recent report of Michel et al. (12) showing thatNK1.1-negative iNKT cells from the liver and lungs of mice produceIL-17, we examined NK1.1 phenotype dependence. We sorted DX5⁺TCRβ⁺NKT cells from spleen based on their expression of NK1.1 andstimulated them with anti-CD3/IL-23 (because NK1.1 is rapidlydown-regulated following TCR ligation, it could not be usedafter stimulation). IL-17 production was considerably higherin NKT cells lacking NK1.1 expression (Fig. 4C). IL-23R expressionand ROR ${gamma}$ t expression were also substantially higher in the "IL-17-ready"NK1.1-negative than in the NKT1.1⁺ population (Fig. 4C), supportingthe interpretation that their constitutive expression underliesthe rapid production of IL-17.

Visualization of intracellular IL-17 in iNKT cells poses similartechnical issues to that of NK1.1, as the invariant TCR is rapidlydown-regulated after activation, just as IL-17 production isoccurring. Therefore, to examine the relationship between NK1.1expression and IL-17 in the iNKT subset, iNKT cells were isolatedfrom naive spleen by sorting with ${alpha}$ -GalCer/CD1d tetramers andwere separated into NK1.1-positive and -negative fractions.Stimulation of these populations with anti-CD3/IL-23 or with ${alpha}$ -GalCer induced high levels of IL-17 production within 24 hin only the NK1.1^– population (Fig. 4D).

Administration of ${alpha}$ -GalCer elicits a rapid IL-17 response in vivo

To examine whether an innate IL-17 response can be induced fromNKT cells in vivo, we injected ${alpha}$ -GalCer into C57BL/6 mice (10µg/mouse) and assessed the relative expression of IL-17A,IFN- ${gamma}$ , and ROR ${gamma}$ t mRNA by real-time quantitative RT-PCR in thespleen. ${alpha}$ -GalCer injection induced a rapid, transient expressionof IL-17 mRNA that peaked 6 h after ${alpha}$ -GalCer treatment and declinedthereafter, returning to baseline at 24 h (Fig. 5A). Interestingly,ROR ${gamma}$ t was expressed at baseline and was not up-regulated by ${alpha}$ -GalCeradministration (Fig. 5C), consistent with our findings in vitro.Because it has recently been suggested that IL-21 may play arole similar to that of IL-6 in the induction of ROR ${gamma}$ t and subsequentIL-17 expression in Th17 cells (10, 13), we also examined thekinetics of IL-21 expression. We found that it lagged considerablybehind the rapid, dramatic increase in IL-17 RNA (Fig. 5D),making it unlikely that IL-21 is a prerequisite for innate IL-17expression. Together, our data suggests that neither IL-21 norIL-6 are required for the production of innate IL-17 by activatedNKT cells.

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FIGURE 5. ${alpha}$ -GalCer elicits a rapid IL-17 response in vivo without up-regulating ROR ${gamma}$ t. Mice were injected with 10 µg of ${alpha}$ -GalCer and spleens collected at 6, 12, and 24 h after treatment. Samples were examined for IL-17, IFN- ${gamma}$ , ROR ${gamma}$ t, and IL-21 mRNA expression by real-time PCR. mRNA levels are expressed as fold increase over unstimulated samples (0 h). Data represent mean ± SEM (n = 6) _*, p < 0.05; _*_*, p < 0.01.

We also examined a more physiologically relevant iNKT ligand,glycosphingolipid derived from the bacteria Sphingomonas wittichii(provided by Dr. P. Savage, Brigham Young University, Provo,UT) and found that a similar pattern of response was observed,albeit the fold increase of mRNA over background was lower thanthat observed with ${alpha}$ -GalCer (not shown). This is consistent withfindings showing that the activity of this compound is lowerthan that of ${alpha}$ -GalCer in stimulating cytokine production by NKTcells (12).

In conclusion, our data show that innate IL-17 production byNKT cells is not restricted to a particular NKT subset and differssignificantly from adaptive IL-17 produced by Th17 effectorcells. Unlike the adaptive response, innate IL-17 productionby NKT cells is rapid, IL-6 independent, and mediated by engagementof TCR and constitutively expressed IL-23R. In addition, ROR ${gamma}$ tis also constitutively expressed in NKT cells and de novo inductiondoes not appear to be required for a dramatic increase in levelsof IL-17. It follows that the role of IL-17 from NKT cells islikely to differ considerably from the proinflammatory roleof IL-17 from Th17 cells, which are implicated to be the effectorcells in various models of autoimmunity (3, 4). Previous datafrom our laboratory indicated that IL-4 and IFN- ${gamma}$ produced byNKT cells are associated with protection from autoimmunity andthe significance of innate IL-17 production by NKT cells toautoimmune disease is currently under investigation.

Acknowledgments

We are grateful to Dr. Dan Cua of Schering-Plough, DNAX division,for providing the IL-23R^–/– mice. We also thankDr. Jun Tang, National Eye Institute, National Institutes ofHealth for his assistance with real-time PCR of ROR ${gamma}$ t expression.

Disclosures

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Materials and Methods
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The authors have no financial conflict of interest.

Footnotes

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

¹ This work was supported by National Institutes of Health, NationalEye Institute intramural funding.

² A.V.R. and A.M.H. contributed equally to this study.

³ Address correspondence and reprint requests to Dr. Rachel R.Caspi, Laboratory of Immunology, National Eye Institute, NationalInstitutes of Health, 10 Center Drive, 10/10N222, Bethesda,MD 20892. E-mail address: rcaspi{at}helix.NIH.gov

⁴ Abbreviations used in this paper: ${alpha}$ -GalCer, ${alpha}$ -galactosylceramide;iNKT, invariant NKT; KO, knockout; WT, wild type.

Received for publication August 14, 2007. Accepted for publication February 16, 2008.

References

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Abstract
Introduction
Materials and Methods
Results and Discussion
Disclosures
References

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I. Godinez, M. Raffatellu, H. Chu, T. A. Paixao, T. Haneda, R. L. Santos, C. L. Bevins, R. M. Tsolis, and A. J. Baumler
Interleukin-23 Orchestrates Mucosal Responses to Salmonella enterica Serotype Typhimurium in the Intestine
Infect. Immun., January 1, 2009; 77(1): 387 - 398.
[Abstract] [Full Text] [PDF]

M.-L. Michel, D. Mendes-da-Cruz, A. C. Keller, M. Lochner, E. Schneider, M. Dy, G. Eberl, and M. C. Leite-de-Moraes
Critical role of ROR-{gamma}t in a new thymic pathway leading to IL-17-producing invariant NKT cell differentiation
PNAS, December 16, 2008; 105(50): 19845 - 19850.
[Abstract] [Full Text] [PDF]

H. Yokote, S. Miyake, J. L. Croxford, S. Oki, H. Mizusawa, and T. Yamamura
NKT Cell-Dependent Amelioration of a Mouse Model of Multiple Sclerosis by Altering Gut Flora
Am. J. Pathol., December 1, 2008; 173(6): 1714 - 1723.
[Abstract] [Full Text] [PDF]

A. Terashima, H. Watarai, S. Inoue, E. Sekine, R. Nakagawa, K. Hase, C. Iwamura, H. Nakajima, T. Nakayama, and M. Taniguchi
A novel subset of mouse NKT cells bearing the IL-17 receptor B responds to IL-25 and contributes to airway hyperreactivity
J. Exp. Med., November 24, 2008; 205(12): 2727 - 2733.
[Abstract] [Full Text] [PDF]

K. Shibata, H. Yamada, R. Nakamura, X. Sun, M. Itsumi, and Y. Yoshikai
Identification of CD25+ {gamma}{delta} T Cells As Fetal Thymus-Derived Naturally Occurring IL-17 Producers
J. Immunol., November 1, 2008; 181(9): 5940 - 5947.
[Abstract] [Full Text] [PDF]

Y. I. Koh, H. Y. Kim, E. H. Meyer, M. Pichavant, O. Akbari, T. Yasumi, P. B. Savage, R. H. DeKruyff, and D. T. Umetsu
Activation of Nonclassical CD1d-Restricted NK T Cells Induces Airway Hyperreactivity in {beta}2-Microglobulin-Deficient Mice
J. Immunol., October 1, 2008; 181(7): 4560 - 4569.
[Abstract] [Full Text] [PDF]

R. S. Grajewski, A. M. Hansen, R. K. Agarwal, M. Kronenberg, S. Sidobre, S. B. Su, P. B. Silver, M. Tsuji, R. W. Franck, A. P. Lawton, et al.
Activation of Invariant NKT Cells Ameliorates Experimental Ocular Autoimmunity by A Mechanism Involving Innate IFN-{gamma} Production and Dampening of the Adaptive Th1 and Th17 Responses
J. Immunol., October 1, 2008; 181(7): 4791 - 4797.
[Abstract] [Full Text] [PDF]

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Cutting Edge: NKT Cells Constitutively Express IL-23 Receptor and RORt and Rapidly Produce IL-17 upon Receptor Ligation in an IL-6-Independent Fashion1

Cutting Edge: NKT Cells Constitutively Express IL-23 Receptor and ROR ${gamma}$ t and Rapidly Produce IL-17 upon Receptor Ligation in an IL-6-Independent Fashion¹