Defective invariant natural killer T-cells (iNKT cells) have been implicated in the etiology of type 1 diabetes in nonobese diabetic (NOD) mice. In a genome scan of a cross between NOD and C57BL/6 mice, the most significant locus controlling the number of iNKT cells, referred to as Nkt1, was recently mapped to distal chromosome 1. Here, using congenic mice for this chromosomal segment, we definitively demonstrate the existence of Nkt1 and show that introgression of the C57BL/6 allele onto the NOD background improves both the number of iNKT cells and their rapid production of cytokines elicited by α-galactosylceramide treatment, explaining at least half of the difference between the NOD and C57BL/6 strains. Using new subcongenic lines, we circumscribed the Nkt1 locus to a 8.7-cM segment, between the NR1i3 and D1Mit458 markers, that notably includes the SLAM (signaling lymphocytic activation molecule) gene cluster, recently involved in murine lupus susceptibility. However, despite a significant correction of the iNKT cell defect, the Nkt1 locus did not alter the course of spontaneous diabetes in congenic mice. Our findings indicate a complex relationship between iNKT cells and autoimmune susceptibility. Congenic lines nonetheless provide powerful models to dissect the biology of iNKT cells.

The development of type 1 diabetes results from T-cell–mediated destruction of insulin-producing β-cells in the pancreas (1). Expression of effector lymphocytes seems to be caused in large part by a defect of immunoregulatory cells (2), among which invariant natural killer T-cells (iNKT cells) are currently the focus of considerable attention. This unique population of αβ-T-cells shows an invariant T-cell antigen receptor (TCR) α-chain, including Vα14Jα18 in the mouse and Vα24JαQ in humans, and also expresses natural killer cell receptors (3). Most remarkably, these cells are capable of rapidly producing large amounts of cytokines on stimulation by glycolipid-type ligands that must be presented by the major histocompatibility complex class I–like CD1d molecule (4). Although α-galatosylceramide (α-GalCer), a glycolipid isolated from marine sponge, has long been used as a surrogate antigen for iNKT cells, their endogenous ligand has been only recently characterized (5).

Remarkably, mice of the nonobese diabetic (NOD) strain, the well-established murine model of spontaneous type 1 diabetes (6), exhibit both a numerical and a functional defect of their iNKT cells as early as 3 weeks of age compared with nondiabetic strains (79). The protective role of iNKT cells is strongly suggested by adoptive transfer experiments (10) and by the study of NOD mice transgenic for a Vα14-Jα18 TCR (11) or for CD1d overexpressed in pancreatic islets (12). Conversely, diabetes is exacerbated in CD1d knockout NOD mice, which are devoid of iNKT cells (13,14). Finally, diabetes can be prevented by in vivo treatment with α-GalCer (15,16), opening a path for the therapeutic manipulation of this cell subset.

Interstrain differences suggest that the number and function of iNKT cells might be under genetic control (8). Recently, a genome-wide screen of a cross between NOD and C57BL/6 mice localized two main loci controlling iNKT cell number: Nkt1 on distal chromosome 1 and Nkt2 on chromosome 2 (17). Importantly, the Nkt2 locus overlapped with the Idd13 locus for insulin-dependent diabetes (Idd) susceptibility, suggesting that the iNKT cell defect of NOD mice might be a genetically determined component of their diabetes susceptibility. Consistent with this finding, mice congenic for certain Idd loci, including Idd6, Idd9, and Idd13, showed a significant modulation of their iNKT cell number and function (18,19). In contrast, however, diabetes-free mice of the NOD-related nonobese diabetes-resistant (NOR) strain harbor the same iNKT cell defect as NOD mice, whereas lupus-prone mice demonstrate an increased number and activity of iNKT cells (18). Taken together, these observations indicate that there is no simple relationship between the genetic control of iNKT cell variation and that of autoimmune susceptibility.

Although the Nkt1 locus does not map to a known Idd locus, we previously characterized a major quantitative trait locus in the same chromosomal region that controls the increased IgG1 and IgG2b serum levels of NOD mice compared with C57BL/6 mice (20). Moreover, this region was also associated with the propensity of NOD mice to express anti-nuclear autoantibodies (21). We had also derived reciprocally congenic strains for this chromosomal region. Such strains provide an essential tool both to confirm the existence of a locus controlling a complex trait as well as to undertake its detailed analysis. Here, we have used these congenic strains and new subcongenic lines to further investigate the Nkt1 locus and its potential influence on type 1 diabetes.

NOD, C57BL/6J, and congenic mice were bred in our animal facility under specific pathogen-free conditions. Congenic strains for distal chromosome 1, including L1 (formerly designated NOD.C57BL/6-fcgr2) and L1R (formerly C57BL/6.NOD-fcgr2), were previously described (20) and have been backcrossed for 20 generations. Subcongenic strains, L2, L3, L6, and L7 (Fig. 1) were derived from L1 mice backcrossed with the NOD parent and by genotypic selection of mice carrying a chromosomal interval of interest. Homozygous mice were then obtained by brother-sister matings. Genomic DNA was genotyped for chromosome 1 microsatellite markers referenced in the Mouse Genome Database (available from www.informatics.jax.org).

Reagents.

A synthetic form of α-GalCer (KRN-7000; Pharmaceutical Research Laboratory, Kirin Brewery, Tokyo) was used. Empty and α-GalCer–loaded CD1d tetramers labeled with allophycocyanin (APC) were prepared in our laboratory. Monoclonal antibodies (mAbs) were purchased from BD PharMingen (San Diego, CA) and included fluorescein isothiocyanate (FITC)-labeled anti–αβ-TCR (clone H57-597), phycoerythrin-labeled anti-CD4 (clone RM4-5), phycoerythrin-labeled anti-interleukin (IL)-4 (clone 11B11), phycoerythrin-labeled anti–γ-interferon (IFN-γ) (clone XMG1.2), and corresponding isotype control antibodies. The Fc-receptor–blocking mAb (anti-CD16/CD32, clone 24G2, culture supernatant) was added to staining mixtures to prevent nonspecific binding by labeled mAbs.

In vivo challenge with α-GalCer and cytokine production.

Mice were injected with α-GalCer (1 μg/dose, i.p. and i.v.) diluted in saline and were bled 90 min later. In some experiments, splenocytes (2.5 × 106 per ml) were prepared from treated animals and cultured without further stimulation for 90 min in RPMI 1640 Glutamax culture medium supplemented with 10% heat-inactivated FCS, 10 mmol/l HEPES, pH 7.4, 1 mmol/l sodium pyruvate, 100 units/ml penicillin, 0.1 mg/ml streptomycin, and 0.05 mmol/l β-mercapto-ethanol. IFN-γ and IL-4 contents were measured in supernatants and in sera by sandwich enzyme-linked immunosorbent assay (ELISA).

Priming with α-GalCer–pulsed dendritic cells.

Dendritic cells were grown from bone marrow cells cultured in RPMI 1640 supplemented with 200 units/ml granulocyte macrophage colony-stimulating factor (R&D Systems, Minneapolis, MN) as previously described (22). After 10 days, dendritic cells (5 × 104 cells per well) were pulsed or not pulsed with α-GalCer (100 ng/ml) for 40 h and then injected intravenously into 6- to 7-week-old mice (5 × 104 dendritic cells per mouse). Sera were collected 24 h later and assayed for cytokine content by sandwich ELISA.

Cell preparation and flow cytometry analysis.

Single-cell suspensions of splenocytes were prepared by standard techniques. Livers were perfused with PBS and pressed through a 70-μm cell strainer, and cells were washed three times. Hepatic lymphocytes were then separated, using a 35% Percoll solution (Amersham Pharmacia Biotech, Uppsala, Sweden), and red cells were lysed in hemolysis buffer. Spleen and liver cells were then incubated with appropriate dilutions of different fluorochrome-coupled mAbs, fixed in 4% paraformaldehyde, and analyzed using a FACScalibur cytometer and CellQuest v3.3 software (BD Biosciences, Mountain View, CA). Dead cells were excluded, using forward and side scatter parameters. A minimum of 1.5 × 105 events gated from live lymphoid cells were acquired in each run. Gates on populations of interest contained at least 1 × 103 events. The absolute number of iNKT cells was calculated from the percentage of the CD1d tetramer–positive cells and the total cell number harvested from each organ.

For detection of intracellular IL-4 and IFN-γ in iNKT cells, cells were stained with APC-labeled CD1d/α-GalCer tetramer and FITC-labeled anti–αβ-TCR mAbs. Fixed cells were then permeabilized with PBS containing 1% BSA and 0.5% saponin and further stained with phycoerythrin-labeled anti–IL-4, phycoerythrin-labeled anti–IFN-γ, or control phycoerythrin-labeled isotype for 30 min at room temperature. The percentages of cytoplasmic IL-4–and IFN-γ–expressing cells were determined by cytometry.

Assessment of diabetes.

The 10-week-old female mice were followed for glycosuria (Glukotests; Roche Diagnostics, Basel, Switzerland) once a week. Mice were recorded as diabetic when the glucose concentration was >500 mg/dl on three consecutive readings.

Data analysis.

Data were expressed as the means ± SE, and differences between means were evaluated by Student’s t test or the nonparametric Wilcoxon–Mann-Whitney test. A log-rank test was used to compare incidences of type 1 diabetes. P values ≤0.05 were reported.

In vivo α-GalCer induced production of IFN-γ and IL-4 in congenic mice.

One of the original features of iNKT cells is their capacity to promptly release large amounts of both of the prototypical T helper-1 and -2 cytokines, IFN-γ and IL-4, after in vivo treatment with their cognate ligand, α-GalCer. To test an effect of the distal chromosome 1 region on iNKT cells, we injected congenic and parent mice once with the ligand and assessed their serum levels of cytokines 2 h later. As shown in Fig. 2A and B (left panels), IFN-γ and IL-4 were detected in sera within 2 h of treatment with α-GalCer at levels significantly higher in congenic L1 than in parent NOD mice (1.67 ± 0.39 vs. 0.45 ± 0.08 ng/ml for IFN-γ, P = 0.01, and 1.71 ± 0.38 vs. 0.99 ± 0.13 ng/ml for IL-4, P = 0.05). Conversely, the reciprocal L1R congenic mice showed decreased levels compared with their C57BL/6 parents (Fig. 2A and B, right panels). Similarly, freshly explanted spleen cells from α-GalCer–primed L1 mice released higher levels of the cytokines compared with NOD splenocytes (0.11 ± 0.03 vs. 0.04 ± 0.01 ng/ml for IFN-γ, P = 0.008, and 0.08 ± 0.02 vs. 0.02 ± 0.01 ng/ml for IL-4, P = 0.012) (not displayed on Fig. 2). Altogether, this first series of experiments based on congenic stocks definitively demonstrated the existence of a locus on chromosome 1 controlling iNKT cell activity, likely closely related to that previously identified as Nkt1 by linkage analysis (17).

We then assessed the in vivo α-GalCer response in L2 and L3 subcongenic mice to narrow down the interval of interest. Both lines were derived from L1 and harbor complementary intervals (Fig. 1). As shown in Fig. 2A and B (left panels), serum levels of cytokines were significantly higher in L2 than in NOD mice (P = 0.001 for IFN-γ and P = 0.002 for IL-4) and comparable to those of their L1 parents, whereas L3 mice responded similarly to NOD mice. Based on this observation, the Nkt1 locus was therefore mapped to a 15-cM interval toward the distal end of the chromosome, excluding its most telomeric segment.

To investigate whether the differential response of congenic mice was caused by an alteration at the level of the presenting cells or of the responding cells, the source of dendritic cells was made constant. Thus, dendritic cells from NOD mice were prepared, pulsed or not with α-GalCer, and injected into L2, L3, or NOD mice. As illustrated in Fig. 2C, for IFN-γ production, the response of L2 mice to dendritic cells pulsed with the glycolipid was higher than that of L3 and NOD mice. This observation suggested that the Nkt1 locus might exert its control at the level of iNKT cells directly.

Numerical and functional profiles of iNKT cells in L2 and L3 subcongenic mice.

Spleen and liver iNKT cells were enumerated in NOD and in subcongenic mice by flow cytometry, using a CD1d tetramer probe. As shown in the dot plot (Fig. 3A), iNKT cells could be clearly resolved among total lymphocytes by the binding of the α-GalCer–loaded CD1d tetramer and the expression of an intermediate level of αβ-TCR. Relative frequencies of iNKT cells are known to vary widely with tissues. In both the spleen and in the liver, L2 mice showed a significant increase in the proportions and in the absolute numbers of iNKT cells compared with NOD or L3 mice (Fig. 3B). By comparison with the parent strains, the numbers of iNKT cells in L2 mice (1.33 × 105 ± 0.12 × 105 in the liver and 6.3 × 105 ± 0.2 × 105 in the spleen) were intermediate between those of NOD (9.4 × 104 ± 2.2 × 104 and 4.9 × 105 ± 2.4 × 104) and C57BL/6 parent mice (2.5 × 105 ± 2.2 × 104 and 7.3 × 105 ± 7 × 104).

The CD4 marker was reported to delineate two functionally distinct subsets of iNKT cells (23,24). A detailed analysis in the liver indicated that both the proportions and the absolute numbers of CD4+, but not CD4, iNKT cells were significantly influenced by the L2 interval (Fig. 4).

Next, we assessed cytokine expression at the single-cell level in iNKT cells. Mice were treated in vivo by α-GalCer, and the magnitude of IL-4 and IFN-γ expression in iNKT cells was determined 2 h after stimulation by intracellular fluorescence staining. A representative experiment is depicted in Fig. 5. Liver iNKT cells from L2 mice had an improved expression of IL-4 and IFN-γ compared with NOD mice. In contrast, L3 mice behaved as NOD mice (data not shown). These findings indicate that the L2 segment alters both the number and the cytokine production of iNKT cells.

Numerical profiles of iNKT cells in L6 and L7 subcongenic mice.

To refine the localization of the Nkt1 locus, we derived two additional subcongenic strains: L6 from L2, and L7 from L1 (Fig. 1). Both of these new strains lack the proximal part of the interval, most notably that including the Fcgr2 locus, whereas they share 8.7 cM of the distal end of the L2 segment. As shown in Fig. 6, the absolute numbers of liver iNKT cells in L6 and L7 mice were higher than those of NOD mice and similar to those of L2 mice. This observation situates the Nkt1 locus in the L6 segment, between the NR1i3 and D1Mit458 markers.

The C57BL/6 allele at the Nkt1 locus does not affect diabetes incidence in NOD mice.

Given the well-established immunoregulatory role of iNKT cells, it was important to investigate the effect of the Nkt1 locus on diabetes susceptibility in NOD mice. As shown in Fig. 7, the course of spontaneous diabetes was very similar in the L2 and the control NOD mice housed at same time and in the same conditions. Up to 60% of L2 mice were diabetic at 30 weeks of age (Fig. 7). Also, the inflammatory infiltrate of the islets of Langerhans was not different in NOD and L2 mice (not shown).

The genetic basis of numerical and functional variations of iNKT cells among mouse strains has been the matter of several recent investigations. Three studies exploited available congenic strains and therefore investigated predefined genetic segments (18,19,25). These strains had been developed to determine the genetic basis of quantitative antibody response or of susceptibility to autoimmune diseases, including type 1 diabetes and systemic lupus erythematosus. In contrast, two other studies were aimed at a genomewide screen of loci influencing iNKT cells (17,26). Altogether, these studies indicated that the number and function of iNKT cells behave as complex traits, having a strain-dependent polygenic and heterogeneous genetic control. The most notable loci mapped to chromosomes 1, 2, 4, 6, 11, and 18.

The genome scan conducted by Esteban et al. (17) was particularly relevant to the current study because it involved the NOD and C57BL/6J strains and identified two main loci. The strongest of these loci, Nkt1, was located on distal chromosome 1 in a region not reported to influence diabetes susceptibility in the NOD strain but that nonetheless was already known for its role in controlling serum levels of IgG (20) and production of anti-nuclear autoantibodies in NOD mice (21). Using mice congenic for this interval, which had been previously derived in our laboratory, we were able to obtain definitive proof of the existence of Nkt1. These congenic mice also provided us with a powerful tool to further investigate the effect of this region on both iNKT cell activity and diabetes susceptibility. We found that the locus affects both the number of iNKT cells and the rapid burst of cytokines induced by α-GalCer, explaining at least half of the difference between the NOD and C57BL/6 strains. It was detected by transferring the C57BL/6 allele onto the NOD background and vice versa, indicative of its strong significance. Interestingly, it concerned preferentially the CD4+ subset of iNKT cells. This finding is consistent with this subset being the major producer of cytokines on activation with α-GalCer (27,28 and A.H., unpublished results). Whether the locus is expressed intrinsically in iNKT cells remains to be investigated. However, our experiment showing that the genotype of iNKT cells responding to fixed-genotype stimulatory dendritic cells influences their response strongly is consistent with this possibility.

Using subcongenic strains, we narrowed down the Nkt1 interval to a segment of 8.7 cM between markers NR1i3 and D1Mit458. Several genes of immunological importance map within the new interval. They most notably include the signaling lymphocytic activation molecule (SLAM)/CD2 family cluster (CD244, CD229, CS1, CD48, CD84, and Ly108), which are major candidates to explain the loss of self-tolerance in NZM2410 lupus mice, corresponding to the Sle1 locus (29,30). The NOD strain appears to share the same haplotype in this region as NZW mice, the donor strain of the susceptibility allele in NZM2410 mice. The SLAM/CD2 family members have been shown to regulate important aspects of lymphocyte function, such as proliferation, cytokine secretion, and cytotoxicity (31). Their intracellular domain binds to an adaptor molecule, SLAM-associated protein, and this interaction was shown to be critical for T-cell signaling (32). Moreover, recent studies showed that SLAM-associated protein is a crucial regulator of iNKT cell ontogeny in both humans and mice (3335). However, which SLAM member(s) is expressed and interacts with SLAM-associated protein in NKT cells is currently not known.

It should be also stressed that the SLAM/CD2 gene cluster extends over just 400 Kb, a minor portion of the current Nkt1 interval, which contains numerous other potential candidates. Therefore, additional subcongenic strains with smaller intervals will be necessary before a detailed investigation of the polymorphism and expression of candidates can be undertaken.

Experiments of several types point to a relationship between type 1 diabetes susceptibility and iNKT cells, at least in mice. Findings obtained with transgenic mice and after pharmacological treatments clearly indicate a strong impact of iNKT cells on the course of type 1 diabetes (1113,15,16). In addition, analysis of iNKT cells in NOD mice congenic with a protective interval, including Idd6 and Idd9.1, favors a role for iNKT cells in spontaneous diabetes because these protective intervals modify the number and the function of iNKT cells (18,19). Conversely, the NOR strain shows depressed number and function of iNKT cells similar to NOD mice (18), even though the Idd13 locus, which contributes to diabetes resistance in NOR mice and maps on chromosome 2 (36), overlaps with the Nkt2 locus and significantly attenuates iNKT cell activity when transferred onto the C57BL/6 background (18). Therefore, our present finding that the Nkt1 locus does not affect the course of spontaneous diabetes in NOD.C57BL/6-Nkt1 (L2 or L6) mice is not entirely unexpected.

Several explanations should be considered to account for such complexity. First, IL-4 plays a significant role in the protection against diabetes afforded by iNKT cells after activation by αGalCer (37), and it was also put forward as the mediator of protection against diabetes in Vα14Jα81 transgenic mice (11). In these model systems, however, large amounts of IL-4 are made artificially available. In contrast, in NOD congenic mice, the improvement of IL-4 production is physiological and limited in magnitude, and it is probably not sufficient to alter the course of diabetes significantly. Other genetic factors might then be necessary and interact with Nkt1 to restore the defect of iNKT cells beyond a certain threshold required for a significant effect on the course of diabetes. Importantly, such interactions might influence the outcome of autoimmunity in both directions and be either beneficial or detrimental to the host. This concern was recently highlighted in systemic lupus erythematosus, where iNKT cells can play both a protective and a pathogenic role in a manner that is genetically determined (38). The development of mice congenic for two or more loci should therefore shed more light on the relationship with type 1 diabetes susceptibility and iNKT cell functions.

Second, other mechanisms might be involved as well. They might depend on different cytokines or even be independent of cytokines, such as cell-cell contacts (39). Such mechanisms have not been yet investigated in genetic studies. Altogether, these observations indicate that the genetic models provide a powerful tool to dissect the complexity of iNKT cell activation mechanisms and their role in pathophysiology. Their study should also help to better anticipate the outcome of pharmacological activation of iNKT cells.

The distal chromosome 1 region is of broad significance in the immune response, as suggested by its involvement in several animal models of systemic lupus (29,40,41) and in anti-nuclear antibody production in NOD mice (21). This region has also been mapped to susceptibility to collagen-induced arthritis (42) and it was linked to murine cerebral malaria (43). Finally, the human equivalent synteny, which lies on distal chromosome 1q, was linked to type 1 diabetes susceptibility (44,45). This region, therefore, seems to be an important one to investigate the genetic basis of autoimmune disorders, notably including type 1 diabetes.

This work was supported by funds from INSERM, CNRS, University Paris 5 René Descartes, and the Programme National de Recherche sur le Diabète (PNRD) and by fellowships from the Ministère de la Recherche (A.-C.R.-C), the Fondation pour la Recherche Médicale (to R.M.), and the Association pour la Recherche sur le Cancer and the Académie de Médecine (to R.Z.).

We are especially indebted to Kirin Brewery (Gumma, Japan) for providing α-GalCer, to Mitchell Kronenberg (La Jolla Institute for Allergy and Immunology, San Diego, CA), and to Peter Van Endert (INSERM U580) for providing plasmids containing CD1d and B2m genes and helping with CD1d/α–GalCer-tetramer preparation. We are most grateful to Guy Fluteau, Laure Eloy, and Séverine Diem for technical assistance and to Fabrice Valette and Mickaël Garcia for animal care.

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A.-C.R.-C. and R.M. contributed equally to this work.

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