Spontaneous Autoimmune Diabetes in Monoclonal T Cell Nonobese Diabetic Mice

doi:10.1084/jem.186.10.1663

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© The Rockefeller University Press, 0022-1007/1997/11/1663/ $5.00
The Journal of Experimental Medicine, Volume 186, Number 10, November 17, 1997 1663-1676

Articles

Spontaneous Autoimmune Diabetes in Monoclonal T Cell Nonobese Diabetic Mice

Joan Verdaguer, Dennis Schmidt, Abdelaziz Amrani, Brad Anderson, Nuzhat Averill, and Pere Santamaria

From the Department of Microbiology and Infectious Diseases, and Julia McFarlane Diabetes Research Centre, The University of Calgary, Faculty of Medicine, Calgary, Alberta, Canada T2N 4N1

Abstract

Top
Abstract
Materials and Methods
Results
Discussion
References

It has been established that insulin-dependent diabetes mellitus(IDDM) in nonobese diabetic (NOD) mice results from a CD4⁺and CD8⁺ T cell–dependent autoimmune process directed against the pancreatic beta cells. The precise roles that betacell–reactive CD8⁺ and CD4⁺ T cells play in the diseaseprocess, however, remain ill defined. Here we have investigatedwhether naive beta cell–specific CD8⁺ and CD4⁺ T cellscan spontaneously accumulate in pancreatic islets, differentiateinto effector cells, and destroy beta cells in the absence ofother T cell specificities. This was done by introducing K^d–or I-A^g7–restricted beta cell–specific T cell receptor (TCR) transgenes that are highly diabetogenic in NOD mice (8.3-and 4.1-TCR, respectively), into recombination-activating gene(RAG)-2–deficient NOD mice, which cannot rearrange endogenousTCR genes and thus bear monoclonal TCR repertoires. We showthat while RAG-2^–/– 4.1-NOD mice, which only bearbeta cell–specific CD4⁺ T cells, develop diabetes asearly and as frequently as RAG-2⁺ 4.1-NOD mice, RAG-2^–/–8.3-NOD mice, which only bear beta cell–specific CD8⁺T cells, develop diabetes less frequently and significantlylater than RAG-2⁺ 8.3-NOD mice. The monoclonal CD8⁺ T cellsof RAG-2^–/– 8.3-NOD mice mature properly, proliferatevigorously in response to antigenic stimulation in vitro, andcan differentiate into beta cell–cytotoxic T cells invivo, but do not efficiently accumulate in islets in the absenceof a CD4⁺ T cell–derived signal, which can be providedby splenic CD4⁺ T cells from nontransgenic NOD mice. Theseresults demonstrate that naive beta cell– specific CD8⁺and CD4⁺ T cells can trigger diabetes in the absence of otherT or B cell specificities, but suggest that efficient recruitmentof naive diabetogenic beta cell–reactive CD8⁺ T cells to islets requires the assistance of beta cell–reactiveCD4⁺ T cells.

Address correspondence to Dr. Pere Santamaria, Department ofMicrobiology and Infectious Diseases, The University of Calgary,Faculty of Medicine, 3330 Hospital Dr. NW, Calgary, Alberta,Canada T2N 4N1. Phone: 403-220-8735; FAX: 403-270-8520; E-mail:psantama{at}acs.ucalgary.ca

Insulin-dependent diabetes mellitus (IDDM)¹ in nonobese diabetic(NOD) mice, which spontaneously develop a form of diabetes closelyresembling human IDDM, is the result of a CD4⁺ and CD8⁺ T cell–dependentautoimmune process directed against the pancreatic beta cells (1, 2). Although the role of T cells as effectors of beta cell damage in IDDM is well established, the nature of the cells and immunological mechanisms that initiate diabetogenesis in genetically susceptible mice remain to be elucidated.

Adoptive T cell transfer studies using spleen cells from prediabeticNOD mice have demonstrated that transfer of IDDM into immunodeficientNOD mice requires both CD4⁺ and CD8⁺ T cells (3–6). However,splenic CD4⁺ T cells from NOD mice and some, though not all,preactivated I-A^g7–restricted, beta cell–specificCD4⁺ T cell clonotypes can home into pancreatic islets anddestroy beta cells in the absence of CD8⁺ T cells (6–13).Since beta cells do not express MHC class II molecules (I-A^g7;references 14, 15), it has been proposed that naive autoreactiveCD4⁺ T cells may differentiate into effector cells by engagingautoantigens that are purportedly shed from the beta cells bya yet to be determined initial insult, in the context of I-A^g7 molecules on local APCs (1, 16).

Studies of β2-microglobulin–deficient NOD mice (17–19) and anti-CD8 mAb-treated NOD mice (20), which do not bearmature CD8⁺ T cells and develop neither diabetes nor insulitis,have suggested that development of insulitis in NOD mice issomehow regulated by CD8⁺ T cells. Although these studies couldnot rule out a general influence of MHC class I molecules and/orCD8⁺ T cells on the insulitogenic activity of naive autoreactiveCD4⁺ T cells (20), they argued in favor of the hypothesis thatthe initial beta cell insult that triggers the shedding ofbeta cell autoantigens and subsequent CD4⁺ T cell activationmay be mediated by beta cell–cytotoxic CD8⁺ T cells, whichare consistently present in pancreatic islets of NOD mice (16,21– 26). This view is compatible with two other observations: that restoring expression of MHC class I molecules on beta cells of β2-microglobulin–deficient NOD mice restoresinsulitis susceptibility (27), and that splenocytes from prediabeticNOD mice cannot efficiently transfer insulitis into β2-microglobulin–deficientNOD.scid mice (28).

This hypothesis, however, is in apparent conflict with other observations that support the alternative view that diabetogenesisis initiated by MHC class II–restricted autoreactive CD4⁺ T cells. For example, splenic CD4⁺ T cells from prediabeticNOD mice can transfer insulitis into NOD.scid mice withoutCD8⁺ T cell cotransfer, and splenic CD8⁺ T cells from diabeticNOD mice cannot home into pancreatic islets of irradiated NODmice or NOD.scid mice in the absence of CD4⁺ T cells (6, 29).Furthermore, since beta cells do not express the costimulatoryB7.1 or B7.2 molecules (30), naive beta cell–specificMHC class I–restricted CD8⁺ T cells are unlikely to differentiateinto cells capable of effecting beta cell damage unless theirtarget beta cell autoantigens are shed from the beta cell byan earlier insult, and later presented to them by APCs capableof processing exogenous antigens through the MHC class I pathway.Finally, and most importantly, genetic susceptibility and resistanceto both insulitis and IDDM are profoundly affected by polymorphismsof MHC class II genes (2, 31), which control the developmentand function of CD4⁺, but not CD8⁺, T cells.

The autoreactive T cells that affect the initial beta cell insult in spontaneous IDDM should be able to home into pancreaticislets, differentiate into effector cells, and effect betacell damage in the absence of other T cells. To investigatethe independent insulitogenic and diabetogenic potential ofnaive beta cell–reactive CD4⁺ or CD8⁺ T cells in spontaneousIDDM, we have compared the ability of NOD mouse islet-derived,I-A^g7– or K^d–restricted, beta cell–specificTCRs to: (a) accelerate diabetogenesis in TCR-transgenic NODmice, and (b) trigger insulitis and diabetes in TCR-transgenic,recombination-activating gene (RAG)- 2^–/– NOD mice,which cannot rearrange endogenous TCR genes and thus bear monoclonalTCR repertoires. We show that unlike naive diabetogenic CD4⁺T cells, which require neither mature B cells nor CD8⁺ T cellsto accumulate in islets and destroy beta cells, naive diabetogenicCD8⁺ T cells are largely dependent on CD4⁺ T cells to efficientlyaccumulate in pancreatic islets and cause diabetes. On the basisof these findings, we propose that recruitment of the firstautoreactive CD8⁺ T cells into pancreatic islets of NOD miceis preceded and/or accompanied by the recruitment of autoreactiveCD4⁺ T cells.

Materials and Methods

Top
Abstract
Materials and Methods
Results
Discussion
References

Production of TCR-transgenic, RAG-2^–^/– NOD Mice.
The H-2K^d–restricted, beta cell–cytotoxic CD8⁺T cell clone NY8.3 was chosen as donor of TCR- ${alpha}$ (V ${alpha}$ n.1-J ${alpha}$ 34) andTCR-β transgenes (Vβ8.1-Dβ2.1-Jβ2.4) togenerate 8.3-NOD mice. This T cell clone was isolated fromislets of an acutely diabetic NOD mouse (24), uses a TCR- ${alpha}$ –CDR3sequence homologous or identical to those used by many NODislet-derived beta cell–cytotoxic CD8⁺ T cells (25, 26),and is diabetogenic in adoptive T cell transfer experiments(24, 32). 4.1-NOD mice (expressing the TCR- ${alpha}$ and -β rearrangementsof the I-A^g7–restricted beta cell–specific CD4⁺ T cell clone NY4.1) and 8.3–TCR-β–transgenicNOD mice (expressing the TCR-β rearrangement of NY8.3)are described elsewhere (26, 33). Transgenic constructs bearingthe functional VDJβ and VJ ${alpha}$ rearrangements of NY8.3 (25),upstream regulatory sequences, and the TCR-β enhancer (forthe TCR-β construct) or the TCR- ${alpha}$ or IgH enhancers (forthe TCR- ${alpha}$ construct) were generated as described (26, 33). Afterremoving prokaryotic sequences by digestion with PvuI and SalI(TCR-β), ClaI and SacII (TCR- ${alpha}$ –IgHenh), or ClaI andSalI (TCR- ${alpha}$ – ${alpha}$ enh), the constructs (21.5, 12.7, or 14.5kb, respectively) were coinjected into fertilized (SJL x C57BL/6)F2 eggs (DNX, Princeton, NJ). Offspring were screened for integrationof the transgenes by Southern blotting using VDJβ andVJ ${alpha}$ cDNA probes. Two transgenic founder mice expressing thetransgenes (8.3–AN6B7– TCR- ${alpha}$ /β with the TCR- ${alpha}$ – ${alpha}$ enhconstruct, and 8.3–IgH3A– TCR- ${alpha}$ /β with the TCR- ${alpha}$ –IgHenhconstruct) were backcrossed with NOD/Lt mice (I-A^g7, I-E^–,K^d, D^b, from The Jackson Laboratory, Bar Harbor, ME) for threeto six generations to generate 8.3–TCR- ${alpha}$ /β–transgenicNOD (8.3-NOD) mice. Studies of mice derived from these twodifferent founders yielded similar results.

RAG-2^–/– NOD mice were generated by backcrossingthe RAG-2 mutation of RAG-2^–/– C57BL/6 mice (34;a gift from F. Alt, Boston Children's Hospital, Boston, MA)onto the NOD background for 10 generations, followed by intercrossingof N10 heterozygotes. RAG-2^–/– 4.1-NOD and RAG-2^–/–8.3-NOD mice (also referred to as monoclonal T cell NOD mice)were generated by backcrossing the TCR transgenes of 4.1-NODand 8.3-NOD mice onto RAG-2^–/– NOD mice. Mice werescreened for inheritance of the transgenes and mutated or wild-typeRAG-2 alleles by PCR of tail DNA. All mice were housed in aspecific pathogen-free facility at The University of Calgary.

Cell Lines, Antibodies, and Flow Cytometry.
H-2K^d –transfected L929 cells (L929-Kd) were obtainedfrom J. Yewdell (National Institutes of Health, Bethesda, MD).NOD mouse–derived NIT-1 and MIN6N8a insulinoma cellswere provided by E.H. Leiter (The Jackson Laboratory) and J.-I.Miyazaki (University of Tokyo, Tokyo, Japan), respectively.WEHI-164 clone 13 cells were provided by D. Remick (Universityof Michigan, Ann Arbor, MI). A hybridoma secreting the Vβ8.1/8.2-specificmAb KJ16 was a gift from P. Marrack (National Jewish Centerfor Immunology, Denver, CO). Hybridomas secreting mAbs 1411-2C11(anti-CD3), GK1.5 (anti-CD4), RA3-6B2 (anti-CD45RA/B220), F4/80(antimacrophage), and M1/70.15.11.5.HL (anti–Mac-1) wereobtained from the American Type Culture Collection (Rockville, MD). Anti-Lyt-2 (CD8 ${alpha}$ )-PE (53-6.7), anti-L3T4-FITC or anti-L3T4-biotin(CD4) (H129.19), anti-CD2-biotin (RM2-5), anti-CD5 (53-7.3)-biotin,anti-CD11a-biotin (M17/4), anti-CD24- biotin (M1/69), anti-CD28-biotin(37.51), anti-CD44-FITC (IM7), anti-CD45RB-FITC (23G2), anti-L-selectin-biotin(CD62L) (MEL-14), anti-CD69-biotin (H1.2F3), anti-Vβ8.1/8.2-FITC (MR5-2), and anti-H-2K^d-FITC (SF1-1.1) were purchased from PharMingen (San Diego, CA). Anti-IL-2R-FITC (CD25) (AMT13)was purchased from Cedarlane Laboratories (Hornby, Ontario,Canada). Mouse IgG-absorbed FITC-conjugated goat anti–ratIgG and FITC-conjugated goat anti–mouse IgG were obtainedfrom CALTAG (San Francisco, CA) and Becton Dickinson (San Jose,CA), respectively. Streptavidin-PerCP was obtained from BectonDickinson. Thymi, spleens, and islet-derived T cell lines wereanalyzed by three-color flow cytometry using a FACScan®(Becton Dickinson) as described elsewhere (26).

TNF- ${alpha}$ Secretion.
Splenocytes from 8.3-NOD mice were depleted of CD4⁺ T cellsusing anti-CD4 mAb (GK-1.5)–coated magnetic beads, asdescribed (26). The remaining cells were analyzed by flow cytometryand adjusted to 10⁴ CD8⁺ T cells/100 µl of complete medium(CM; RPMI 1640 media containing 10% heat-inactivated fetalbovine serum [GIBCO BRL, Gaithersburg, MD], 50 U/ml penicillin,50 µg/ml streptomycin (Flow Laboratories, McLean, VA),and 50 µM 2-ME [Sigma Chemical Co., St. Louis, MO]) andchallenged with beta cells (NIT-1 or MIN6N8a) or control targetcells (L929-Kd) (10⁴ cells/100 µl) for 24 h. The culturesupernatants (100 µl) were assayed for the presence ofTNF- ${alpha}$ by measuring their cytolytic effect on WEHI-164 clone 13cells (35) using a colorimetric assay (Cell Proliferation KitII, Boehringer Mannheim, Mannheim, Germany). rTNF- ${alpha}$ (R&DSystems, Minneapolis, MN) was used to generate the standardcurves. In some experiments, splenic CD8⁺ T cells were preactivatedwith plate-bound anti-CD3 mAb (1411-2C11, 10 µg/ml) for3 d at 37°C in 5% CO₂ (26) and expanded with 0.5 U/ml ofrIL-2 (Takeda, Osaka, Japan) for 7 d before being assayed fortheir ability to secrete TNF- ${alpha}$ in response to beta cells.

Proliferation Assays.
Pancreatic islet cells were prepared from 5–8-wk-oldNOD mice as described (26). Splenic CD8⁺ T cells (2 x 10⁴)were incubated, in triplicate, with ${gamma}$ -irradiated (3,000 rad)islet cells (3–100 x 10³/well) in 96–round-bottomedwell tissue culture plates for 3 d at 37°C in 5% CO₂. Cultureswere pulsed with 1 µCi of [³H]thymidine during the last18 h of culture and harvested. Thymidine incorporation was measuredby scintillation counting. Specific proliferation was calculatedby substracting background proliferation (cpm of cultures containing islet cells alone and cpm of cultures of T cells alone) fromislet cell–induced proliferation (cpm of cultures containingT cells and islet cells). For anti–TCR-β stimulation,CD8⁺ T cells (2 x 10⁴) were added, in triplicate, to ELISA-gradewells precoated with 10-fold serial dilutions of KJ16 mAb (anti-Vβ8.1/8.2)–containingascites (1:10–1:10,000; reference 26), incubated for 48h, pulsed with [³H]thymidine for 18 h, harvested, and analyzedby scintillation counting.

Limiting Dilution Analyses.
To determine the peripheral frequency of beta cell–reactiveCD8⁺ T cells, 12 replicate cultures of 10-fold serial dilutionsof splenocytes (10¹–10⁵ cells/well) were stimulated withirradiated (2,500 rads) NOD islets (8/well) for 4 d, expandedin rIL-2 (0.5 U/ml) for 10 d, and restimulated with islets andrIL-2. Control plates received rIL-2, but not islets. The resultingcultures were split, challenged with 10⁴ NIT-1 cells or L929-Kdcells for 24 h, and the supernatants were collected to measurethe contents of TNF- ${alpha}$ . Cultures that secreted TNF- ${alpha}$ in responseto MIN6N8a cells (absorbance values two standard deviationsbelow the average values of control cultures) but not L929-Kdcells were considered to contain beta cell–reactive CD8⁺ T cells. Frequencies were calculated by Poisson statistics.

Generation of Spleen- and Islet-derived CD8⁺ T Cell Lines and Clones.
CD4⁺ T cell–depleted spleen cells (10⁴ cells/well in 96-wellplates) were stimulated with irradiated NOD islets for 3 d, and the activated cells expanded with 0.5 U/ml rIL-2 for 10–14d. Growing cultures were split and individual subcultures assayedat this point for serine esterase content (see below) or betacell reactivity.

Islet-infiltrating CD8⁺ T cell lines were isolated from prediabeticor acutely diabetic mice as described previously (26). In brief, isolated islets were cultured in CM containing 0.5 U/ml ofrIL-2, and the lymphocytes obtained after 4–5 d wereanalyzed by flow cytometry to determine their phenotype, depletedof CD4⁺ T cells by negative selection with GK1.5 mAb-coatedimmunobeads, used for messenger RNA extraction, cloned in 96-wellplates under limiting dilution conditions (1–5 cells/well),and stimulated once with irradiated NOD islets in the presenceof rIL-2. Growing cultures were split into three subculturesand assayed within 10 d of cloning for beta cell specificity(TNF- ${alpha}$ release in response to NIT-1 or L929-Kd cells) and serineesterase content, or expanded further to obtain sufficient cellsfor cytotoxicity assays.

Determination of Serine Esterase Content.
Confluent 96-well plate subcultures were lysed with 1% TritonX-100 and the lysates analyzed for serine esterase activity(26, 36). Absorbance readings two standard deviations abovethe mean of negative cultures (nonstimulated splenocytes) wereconsidered positive.

Cytokine Reverse Transcription-PCR.
Total cellular RNA was extracted from islet-derived T celllines depleted of CD4⁺ T cells (>98% CD8⁺) by the guanidiumisothiocyanate-phenol-chloroform method, and 2 µg usedin a reverse transcription reaction using oligo(dT)_12–18(GIBCO BRL) as a primer. The cDNAs were amplified by PCR usingpreviously described primers specific for several cytokines,including IL-2, IFN- ${gamma}$ , IL-4, IL-10, TNF- ${alpha}$ , and for hypoxanthinephosphoribosyl transferase (HPRT) as internal control (37).The PCR products were electrophoresed in a 1.5% agarose geland detected by ethidium bromide staining.

⁵¹Cr–Release Assays.
Single islet cells (5 x 10⁵) from NOD (H-2^g7: I-A^g7, K^d, D^b)and C57BL/6 (H-2^b: I-A^b, K^b, D^b) mice were labelled with [⁵¹Cr]sodiumchromate (DuPont New England Nuclear, Boston, MA), resuspendedat 10⁵ cells/ml, and seeded at 10⁴ cells/100 µl/well.Effector cells (islet-derived CD8⁺ T cell clones) were addedto each well, in duplicate, at several target/effector ratios.Plain medium was added to a set of target cells for examinationof spontaneous cell lysis. Total cell lysis was determined bylysing the cells with 1% Triton X-100. The plates were centrifugedat 100 g for 3 min and incubated at 37°C for 8 h. Afterincubation, the plates were centrifuged and the supernatants (100 µl) harvested. The radioactivity of the supernatantswas measured in a gamma counter (LKB-Wallac, Turku, Finland).Specific ⁵¹Cr release was calculated as follows: percent lysis= 100 x (test cpm – spontaneous cpm)/(total cpm –spontaneous cpm).

Adoptive T cell Transfer.
Splenocytes from 4–5-wk-old nontransgenic female NOD micewere depleted of CD8⁺ T cells using anti-CD8 mAb (53-6.7)–coatedmagnetic beads (26). The remaining cells (containing <0.5%CD8⁺ T cells) were injected (8 x 10⁶ cells/mouse) into 5–8-wk-oldfemale RAG-2^–/– 8.3-NOD mice. Recipient mice weremonitored for diabetes or killed 10 wk after transfer for histology.Some RAG-2^–/– 8.3-NOD mice were transfused withsplenic T cells from nontransgenic NOD mice (1.5 x 10⁷ cells/mouse)enriched for CD4⁺ T cells (>92%) and depleted of CD8⁺ Tcells and B220⁺, F4/80⁺, Mac-1⁺, and 33D1⁺ cells (<0.4%)using mAb-coated immunobeads and affinity columns (R&D Systems).

Diabetes.
Diabetes was assessed by measuring urine glucose levels withDiastix strips (Miles, Ontario, Canada) twice a week. Animalswere considered diabetic after two consecutive readings $>=$ 3+.

Histopathology.
Submandibular salivary gland, thyroid, adrenal gland, kidney,liver, stomach, small intestine, colon, pancreas (one half),and muscle were fixed in formalin, embedded in paraffin, sectionedat 4.5 µM, stained with hematoxylin and eosin, and examinedfor inflammation. The degree of insulitis in the pancreas wasevaluated by scoring 15–30 islets/mouse in a blinded fashion using the following criteria: 0, normal islet; 1, periinsulitis;2, mononuclear cell infiltration in <25% of the islet; 3, mononuclear cell infiltration in 25–50% of the islet;4, >50% of the islet infiltrated. A second half of eachpancreas was snap frozen in liquid nitrogen, immersed in OCT,sectioned at 6–7 µM, fixed in cold acetone for10 min, and stained with anti-CD4 (GK1.5) and anti-CD8 (53-6.7)mAbs followed by anti–rat IgG-FITC, or with anti–ratIgG-FITC alone, and observed under a fluorescence microscope(26).

Statistical Analyses.
Statistical analyses were performed using Mann-Whitney U and ${chi}$ ² tests.

Results

Top
Abstract
Materials and Methods
Results
Discussion
References

Expression of the 8.3-TCR in 8.3-NOD Mice.
Three-color cytofluorometric studies showed that >97% CD4^–CD8⁺ thymocytes (Fig. 1 A) and lymph node CD8⁺ T cells (Fig. 1B) from 8.3-NOD mice expressed Vβ8.1/8.2⁺ TCRs, as comparedwith 18% of the CD4^–CD8⁺ thymocytes and lymph node CD8⁺T cells from nontransgenic NOD mice, indicating TCR-βtransgene expression. Although we do not have a TCR- ${alpha}$ –transgenicchain–specific mAb, and thus cannot directly quantitateits expression, three different lines of evidence indicate thatthe transgenic TCR- ${alpha}$ chain is expressed on a significant fractionof thymocytes and peripheral T cells from 8.3-NOD mice. First, $~$ 67% of CD4⁺CD8⁺ thymocytes from 8.3-NOD mice expressed highlevels of the transgenic TCR-β chain, as compared to only18% of CD4⁺CD8⁺ thymocytes from TCR-β–transgenicNOD mice, suggesting early TCR- ${alpha}$ chain expression and early upregulationof TCR- ${alpha}$ /β heterodimers on immature thymocytes (38–42).Second, thymocyte development in 8.3-NOD mice, but not 8.3–TCR-β–transgenicNOD mice, was skewed towards the CD4^–CD8⁺ subset (Fig.1 A), suggesting TCR- ${alpha}$ –transgene–dependent positiveselection of 8.3-CD8⁺ thymocytes as in other MHC class I–restrictedTCR- ${alpha}$ /β–transgenic models (38, 41, 43). As a result,the lymph nodes of 8.3-NOD mice consistently had many moreCD8⁺ T cells (>65%) and fewer CD4⁺ T cells (<15%) thanthe lymph nodes of 8.3– TCR-β–transgenic andnontransgenic NOD mice (with <25% CD8⁺ T cells and >40%CD4⁺ T cells) (Fig. 1 B). Finally, introduction of the 8.3–TCR- ${alpha}$ and –TCR-β transgenes into RAG-2^–/–NOD mice, which cannot rearrange endogenous TCR genes, resultedin the positive selection of CD8⁺, but not CD4⁺, Vβ8.1/8.2⁺T cells (see below). Taken together, these data indicate thatthe 8.3-TCR is expressed on a significant fraction of thymocytes and peripheral T cells from 8.3-NOD mice, and that 8.3–TCR- ${alpha}$ /β–transgene expression fosters the positiveselection of CD8⁺ T cells.

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Figure 1 Expression of the TCR- ${alpha}$ /β transgenes in 8.3-NOD mice. CD4, CD8, and Vβ8.1/8.2 profiles of thymocytes (A) and lymph node cells (B) from nontransgenic NOD, 8.3–TCR-β–transgenic NOD, and 8.3-NOD mice. (Top) CD4 versus CD8 contour plots of cell suspensions stained with anti-CD8-PE, anti-V β8.1/8.2-FITC, and anti-CD4-biotin plus Streptavidin-PerCP. The lower panels show the Vβ8.1/8.2 fluorescence histograms of each T cell subset after electronic gating. Numbers indicate the average percentage of cells (top) or the average number of Vβ8.1/8.2⁺ cells (bottom) in each subset. Data correspond to 3–9 mice/group. DP, double-positive cells; DN, double-negative cells.

Functional Responsiveness and Activation State of Peripheral CD8⁺ T Cells in 8.3-NOD Mice.
To investigate whether peripheral T cells displaying the 8.3-TCRwere functionally responsive to beta cells, we compared theproliferative activity of CD4⁺ T cell–depleted splenicCD8⁺ T cells from 8.3-NOD and 8.3–TCR-β–transgenicNOD mice in response to irradiated NOD islet cells. As shownin Fig. 2 A, CD8⁺ T cells from 8.3-NOD, but not 8.3–TCR-β–transgenicNOD mice, proliferated vigorously in these assays, both inthe presence and absence of exogenous rIL-2. The increasedproliferative activity of splenic CD8⁺ T cells from 8.3-NODversus 8.3–TCR-β–transgenic NOD mice resultedfrom an increased frequency of beta cell–reactive CD8⁺T cells (measured at $~$ 1/17 versus 1/4,000 splenic CD8⁺ T cells,respectively; Fig. 2 B), rather than from differences in theirgeneral proliferative activity, since CD8⁺ T cells from bothtypes of mice proliferated equally well in response to a plate-boundanti-Vβ8.1/8.2 mAb (KJ16; Fig. 2 C). Therefore, 8.3-NODmice export numerous beta cell–specific CD8⁺ T cellsto the periphery, and these autoreactive CD8⁺ T cells are nottolerant to antigen stimulation in vitro.

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Figure 2 Responsiveness and peripheral frequency of beta cell–specific CD8⁺ T cells in 8.3-NOD mice. (A) Proliferation of splenic CD8⁺ T cells from 8.3-NOD and 8.3–TCR-β–transgenic NOD mice to islet cells. 2 x 10⁴ splenic CD8⁺ T cells were incubated with ${gamma}$ -irradiated islet cells for 3 d, pulsed with [³H]thymidine, harvested, and counted. Bars show the standard error of the means. (B) Peripheral frequency of beta cell–reactive CD8⁺ T cells in 8.3-NOD and 8.3–TCR-β–transgenic NOD mice. 12 replicate cultures of serial dilutions of splenocytes (10¹– 10⁵ cells/well) were stimulated with irradiated NOD islets (8/well) for 4 d, expanded in rIL-2 (0.5 U/ml) for 10 d and restimulated once with islets and rIL-2. The cultures were then challenged with 10⁴ NIT-1 or L929-Kd cells for 24 h, and the supernatants collected to measure their TNF- ${alpha}$ content. Cultures that secreted TNF- ${alpha}$ in response to NIT-1, but not L929-Kd, cells were considered to contain beta cell–reactive CD8⁺ T cells. (C) General proliferative activity of splenic CD8⁺ T cells of 8.3-NOD and 8.3–TCR-β–transgenic NOD mice. 2 x 10⁴ splenic CD8⁺ T cells were incubated with 10-fold serial dilutions of plate-bound KJ16 in rIL-2–containing CM for 3 d, pulsed with [³H]thymidine, harvested, and counted.

Three-color cytofluorometric analyses of splenic CD8⁺ T cellsfrom diabetic 8.3-NOD and nontransgenic NOD mice with mAbsagainst memory and activation markers (CD25, CD44, CD69, andCD62L²) did not reveal any significant differences (data notshown), suggesting that the numerous beta cell–reactiveCD8⁺ T cells of 8.3-NOD mice are quiescent. This was furtherinvestigated by comparing the ability of naive splenic CD8⁺T cells from 8.3-NOD and 8.3–TCR-β–transgenicNOD mice to secrete TNF- ${alpha}$ in response to stimulation with betacells. As shown in Table 1, splenic CD8⁺ T cells from 8.3-NODmice did not secrete TNF- ${alpha}$ when challenged with NOD-derived beta cells unless they had been previously activated in vitro with plate-bound anti-CD3 mAb and rIL-2. As expected, islet-derivedCD8⁺ T cells from both 8.3-NOD and 8.3– TCR-β–transgenicNOD mice (enriched for in vivo–activated beta cell–specificCD8⁺ T cells) secreted high levels of TNF- ${alpha}$ when challengedwith NOD beta cells, but not L929-Kd fibroblasts. It thus appearsthat the beta cell–reactive CD8⁺ T cells of 8.3-NOD micedo not undergo spontaneous activation in the periphery.

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Table 1 Secretion of TNF- ${alpha}$ by Splenic- and Islet-derived CD8⁺ T Cells from 8.3-TCR-transgenic NOD Mice (pg/ml)

Acceleration of Diabetes in 8.3-NOD Mice.
We next investigated whether positive selection of the betacell–specific 8.3-TCR in 8.3-NOD mice had any pathogenicsignificance. We therefore followed 8.3-NOD mice of the N3-N6backcrosses of the founder mice onto the NOD background fordevelopment of diabetes, and compared the cumulative incidencecurves of these mice with those of nontransgenic NOD mice and8.3–TCR-β–transgenic NOD mice (26). As shownin Fig. 3 A, female and male 8.3-NOD mice developed diabetesmuch earlier than female and male 8.3–TCR-β–transgenic(N4-N7), nontransgenic NOD littermates (N3-N5) or NOD/Lt mice(ages at onset: 43 ± 10 versus 88 ± 12, 120 ±19 and 119 ± 26 d, respectively, for females, P <0.0001;and 66 ± 15 versus 109 ± 33, 173 ± 35,and 157 ± 28 d, respectively, for males, P <0.0001). Despite the dramatic acceleration of diabetes onset in 8.3-NODmice, the cumulative incidence of diabetes and the kineticsof disease penetrance in the 8.3-NOD, 8.3–TCR-β–transgenic,nontransgenic NOD littermates, and NOD/ Lt mouse populationswere remarkably similar (females: 73.1% versus 86, 78, and84%, respectively; males: 50% versus 50, 31, and 46%, respectively;Fig. 3 A). No major differences in disease penetrance werenoted among 8.3-NOD mice of the N3-N6 generations. In females,for example, the incidence and age at onset of diabetes foreach generation were: N3, 6/8 mice at 40 ± 4 d; N4,5/6 mice at 45 ± 6 d; N5, 2/3 mice at 37 ± 3d; and N6, 6/9 mice at 51 ± 13 d. The same was truefor 8.3–TCR-β–transgenic NOD mice (26), andfor nontransgenic NOD littermates (N3 females: 3/3 mice at 140± 5 d; N4 females: 6/ 8 mice at 117 ± 46 d; andN5 females: 5/7 mice at 117 ± 14 d). Taken together,these data indicate that the 8.3-TCR is highly diabetogenicin the NOD background, and suggest that the events that triggerdiabetes in 8.3-NOD mice are similar to those that triggerdiabetes in nontransgenic NOD mice.

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Figure 3 8.3–TCR- ${alpha}$ /β– transgene expression and diabetogenesis. (A) Incidence of IDDM in female (26 8.3–, 21 8.3–TCR-β–transgenic, and 114 nontransgenic) and male (24 8.3–, 30 8.3–TCR-β–transgenic, and 59 nontransgenic) NOD mice. (B) Progression of insulitis in nontransgenic, 8.3– TCR-β–transgenic, and 8.3-NOD mice (4–7 mice/age group; 15–30 islets/mouse). Bars show the standard deviation of the means. *, P <0.0001 (Mann-Whitney U test). (C) Flow cytometry profile of islet-derived T cells from diabetic 8.3-NOD mice. Islets from acutely diabetic 8.3-NOD mice were cultured in rIL-2–containing CM for 3–5 d and the resulting cells studied by flow cytometry as in Fig. 1. (D) Phenotype of islet-infiltrating T cells in 8.3-NOD versus nontransgenic NOD mice. Pancreas sections were stained with anti-CD8 (53.6-7) or anti-CD4 (GK1.5) mAbs and FITC-labeled anti–rat IgG, and observed under a fluorescence microscope. Original magnification: 200.

Pathogenic Basis of Disease Acceleration in 8.3-NOD Mice.
To elucidate the mechanisms underlying disease accelerationin 8.3-NOD mice, we followed the progression of insulitis in3–6-wk-old 8.3-NOD, 8.3–TCR-β–transgenic and nontransgenic NOD mice. Unexpectedly, the insulitis scoresof 3-wk-old 8.3-NOD mice were significantly lower than theinsulitis scores of age-matched 8.3–TCR-β–transgenicand nontransgenic NOD mice (Fig. 3 B). In contrast, the insulitisscores of 6-wk-old 8.3-NOD mice were significantly more severethan those of 8.3–TCR-β–transgenic and nontransgenicNOD mice (Fig. 3 B). It thus appears that insulitis in 8.3-NODmice starts later, but progresses much faster, than in 8.3–TCR-β–transgenicand nontransgenic NOD mice. As expected, most of the islet-derivedT cells of acutely diabetic 8.3-NOD mice were CD8⁺ and expressedthe transgene-encoded Vβ8.1 element (Fig. 3 C). Immunopathologicalstudies of pancreata from these mice confirmed that the insulitislesions of 8.3-NOD mice contained many more CD8⁺ T cells, andfewer CD4⁺ T cells, than the lesions of nontransgenic (Fig.3 D) and 8.3– TCR-β–transgenic NOD mice (26).Between 3 and 27% of all the islet-derived, beta cell–reactiveCD8⁺ T cell clones from these mice (but 0% of the spleen-derived,beta cell–reactive CD8⁺ T cell clones) contained serineesterase activity and were cytotoxic to NOD (H-2K^d, D^b), butnot C57BL/6 (H-2K^b, D^b) islet cells in vitro (data not shown). We thus conclude that acceleration of diabetes in 8.3-NOD mice results from massive recruitment of highly diabetogenic,beta cell–cytotoxic CD8⁺ T cells (and CD4⁺ T cells) to pancreatic islets early in the disease process.

Spontaneous Diabetes in Monoclonal 8.3-NOD and 4.1-NOD Mice.
Comparison of the natural history of diabetes in 8.3-NOD miceto that in mice expressing the TCR rearrangements of a betacell–specific, I-A^g7–restricted CD4⁺ T cell clone(4.1-NOD mice) (33), revealed a remarkable similarity (i.e.,similar acceleration of the disease). To investigate whetherthe highly diabetogenic CD8⁺ and CD4⁺ T cells of these micecould spontaneously accumulate in pancreatic islets, differentiateinto beta cell–cytotoxic effectors, and destroy beta cellsin the absence of T cells displaying endogenous TCRs, we introducedthe 8.3- and 4.1-TCR transgenes into RAG-2^–/– NODmice, which cannot rearrange endogenous TCR or Ig genes (34).As expected, virtually all of the lymph node T cells of RAG-2^–/–4.1-NOD mice and RAG-2^–/– 8.3-NOD mice were CD4⁺ Vβ11⁺ or CD8⁺Vβ8.1/8.2⁺ T cells, respectively (Fig.4 A).

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Figure 4 Diabetogenesis in TCR-transgenic RAG-2^–/– NOD mice. (A) Flow cytometry profiles of lymph node cells from RAG-2^–/– 4.1-NOD mice (left) and RAG-2^–/– 8.3-NOD mice (right). (B) Incidence of diabetes in RAG-2^–/– 4.1-NOD (n = 29 females and 35 males), RAG-2^–/– 8.3-NOD (n = 12 females and 20 males), and RAG-2^–/– NOD mice (n = 20 females and 20 males). The few cells of the opposite T cell subset that appear in the flow cytometry profiles of these mice are the result of nonspecific staining of dead cells. (C) Phenotype of islet-infiltrating T cells in RAG-2^–/– 4.1-NOD and RAG-2^–/– 8.3-NOD mice. Most of the few CD8⁺ T cells in RAG-2^–/– 4.1-NOD mice, and the few CD4⁺ T cells in RAG-2^–/– 8.3-NOD mice were the result of background staining, as they were also seen in anti–rat IgG-FITC–stained tissue.

Surprisingly, RAG-2^–/– 4.1-NOD mice developed diabetesslightly earlier than, and almost as frequently as, RAG-2⁺4.1-NOD mice (ages at onset: 36 ± 10 versus 44 ± 13 d for females; and 39 ± 13 versus 56 ± 27d for males; incidences of 72 versus 76% for females, and 60versus 73% for males, respectively). In contrast, RAG-2^–/–8.3-NOD mice developed diabetes much less frequently (33 versus 73% for females, P <0.0001; and 26 versus 50% for males, P <0.0001), and significantly later than RAG-2⁺ 8.3-NODmice (ages at onset: 111 ± 16 versus 43 ± 10 dfor females, P <0.002; and 94 ± 50 versus 66 ±15 d for males, P <0.05). We are confident that insulitisand diabetes in RAG-2^–/– 4.1-NOD and RAG-2^–/–8.3-NOD mice were triggered by T cells expressing the transgenicTCRs, for two reasons. First, nontransgenic RAG-2^–/–NOD mice developed neither diabetes (Fig. 4 B) nor insulitis(data not shown). Second, the pancreatic islets of diabeticRAG-2^–/– 4.1-NOD and RAG-2^–/– 8.3-NODmice almost exclusively contained CD4⁺ or CD8⁺ T cells, respectively(Fig. 4 C). A few cells of the opposite T cell subset werealso seen in these mice (Fig. 4 C); however, these cells were probably the result of background staining since they were also seen in sections stained with anti–rat IgG-FITCalone (data not shown). These results demonstrate that (a)4.1-CD4⁺ T cells can accumulate efficiently in pancreatic islets and trigger diabetes in the absence of mature B cells and T cells expressing endogenous TCRs, and (b) although 8.3-CD8⁺T cells can also cause diabetes in the absence of B cells andT cells expressing endogenous TCRs, they do so much less efficientlythan in their presence.

Absence of Extra-pancreatic Pathology in TCR-transgenic RAG-2^–^/– NOD Mice.
Since nontransgenic NOD mice can also develop inflammationof other organs, notably the submandibular salivary glandsand the thyroid (44), we investigated the presence of sialitisin diabetic TCR-transgenic RAG-2^–/– NOD mice. Sialitiswas invariably present in all the 8.3-NOD, 4.1-NOD, and nontransgenicNOD mice that were investigated (n = 2–7 mice/group),but completely absent in RAG-2^–/– NOD, RAG-2^–/–4.1-NOD, and RAG-2^–/– 8.3-NOD mice (n = 7–10mice/group). Inflammation of the thyroid, adrenal glands, kidney,liver, gut, stomach, or muscle was also absent in all thesemice. It thus appears that the inflammatory potential of 4.1-CD4⁺and 8.3-CD8⁺ T cells is tissue specific.

Normal CD8⁺ T Cell Development but Slow Progression of Insulitis in RAG-2^–/– 8.3-NOD Mice.
Experiments were next performed to elucidate the mechanismsunderlying disease deceleration in RAG-2^–/– 8.3-NODversus RAG-2⁺ 8.3-NOD mice. Three-color cytofluorometric studies using mAbs against several differentiation markers, includingthe transgenic TCR, MHC class I (K^d), CD5, CD24, CD44, andCD69, revealed that the CD4⁺CD8⁺ and CD4^–CD8⁺ thymocytesof RAG-2^–/– 8.3-NOD mice and RAG-2⁺ 8.3-NOD micewere phenotypically similar (Fig. 5 A). Likewise, no phenotypicdifferences were noted between the peripheral CD8⁺ T cellsof RAG-2^–/– 8.3-NOD mice and those of RAG-2⁺ 8.3-NODmice with respect to several markers, including Vβ8.1/8.2,CD2, CD11a, CD28, CD44, CD45RB, CD62L and CD69 (Fig. 5 B).Furthermore, splenic CD8⁺ T cells from both types of mice proliferatedequally well in response to islet cells in vitro (Fig. 5 C).It thus appears that the 8.3-CD8⁺ T cells of RAG-2^–/–8.3-NOD mice are phenotypically and functionally similar tothose of RAG-2⁺ 8.3-NOD mice.

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Figure 5 Phenotype and functional activity of CD8⁺ T cells from RAG-2^–/– versus RAG-2⁺ 8.3-NOD mice. (A) Flow cytometry profiles of CD4⁺CD8⁺ (left) and CD4^–CD8⁺ thymocytes (right) from 8.3-NOD mice (dotted line) and RAG-2^–/– 8.3-NOD mice (solid line) for maturation markers. Thymocytes were analyzed by three-color cytofluorometry as in Fig. 1. Panels show the fluorescence histograms of each marker on gated CD4⁺CD8⁺ and CD4^–CD8⁺ thymocytes. (B) Flow cytometry profiles of splenic CD8⁺ T cells from 8.3-NOD mice (dotted line) and RAG-2^–/– 8.3-NOD mice (solid line) for activation and memory markers. (C) Proliferative activity of splenic CD8⁺ T cells from 8.3-NOD mice and RAG-2^–/– 8.3-NOD mice in response to islet cells. (D) Reverse transcription-PCR analysis for cytokine gene expression of islet-derived CD8⁺ T cells from 8.3-NOD mice and RAG-2^–/– 8.3-NOD mice. M, 1Kb ladder. (E) Kinetics of insulitis in RAG-2^–/– 8.3-NOD mice.

We then investigated whether the islet-derived CD8⁺ T cellsof RAG-2^–/– 8.3-NOD mice had differentiated into Th1-like CTLs (Tc1) in situ. We first isolated CD8⁺ T cellsfrom the pancreatic islets of acutely diabetic RAG-2⁺ 8.3-NODand RAG-2^–/– 8.3-NOD mice and determined theircytokine profile by reverse transcription-PCR. As shown inFig. 5 D, the islet-derived CD8⁺ T cells of both types of micetranscribed messenger RNA for IL-2, IFN- ${gamma}$ , IL-10, and TNF- ${alpha}$ ,but not IL-4. We then determined the percentage of serine esterase–containingT cell clones among those capable of secreting TNF- ${alpha}$ specificallyin response to NOD beta cells shortly after their isolationfrom islets. Interestingly, the percentage of serine esterase–positiveclones per mouse was, on average, greater than that observedin 8.3-NOD mice (43 versus 13%; data not shown). Thus, lackof CTL generation does not appear to account for the relativediabetes resistance of RAG-2^–/– 8.3-NOD mice.

Finally, to determine whether deceleration of diabetes in RAG-2^–/–8.3-NOD mice resulted from slow progression of insulitis, wescored the degree of insulitis in cohorts of 5–35-wk-oldnondiabetic RAG-2^–/– 8.3-NOD mice. We found thatmost of these mice had very mild or no insulitis and that,when present, it progressed much slower than in RAG-2⁺ 8.3-NODmice (compare Figs. 5 E and 3 B). It thus appears that therate-limiting factor of diabetogenesis in RAG-2^–/–8.3-NOD mice is the ability of these mice to develop insulitis.

CD4⁺ T Cells Can Trigger the Recruitment of Naive CD8⁺ T Cells in RAG-2^–^/– 8.3-NOD Mice.
To investigate whether nontransgenic splenocytes other thanCD8⁺ T cells could foster the recruitment of the diabetogenic 8.3-CD8⁺ T cells of RAG-2^–/– 8.3-NOD mice intoislets, we transfused CD8⁺ T cell–depleted splenocytesfrom young nontransgenic NOD mice into RAG-2^–/–8.3-NOD mice or RAG-2^–/– NOD mice. As shown inTable 2, spleen cell–transferred RAG-2^–/–8.3-NOD mice developed severe insulitis, owing to massive infiltrationof islets by B cells and CD4⁺ and CD8⁺ T cells, and four offive mice developed diabetes shortly after transfer (at 36± 16 d). In contrast, none of the seven spleen cell–transfusedRAG-2^–/– NOD mice had developed diabetes or insulitisby 8–10 wk after transfer. To ascertain whether diabetesin RAG-2^–/– 8.3-NOD mice was triggered by CD4⁺T cells, we injected purified splenic CD4⁺ T cells from youngnontransgenic NOD mice into two RAG-2^–/– 8.3-NODmice. As shown in Table 2, both mice developed severe insulitis(containing CD4⁺ and CD8⁺ T cells, but not B cells) and diabetes shortly after transfer (35 ± 22 d). These results demonstrate that the peripheral naive CD8⁺ T cells of RAG-2^–/–8.3-NOD mice can be induced to migrate into pancreatic islets by splenic CD4⁺ T cells from nontransgenic NOD mice.

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Table 2 Nontransgenic CD4⁺ T Cells Can Trigger the Recruitment and Activation of Autoreactive CD8⁺ T Cells in RAG-2^–^/– 8.3-NOD Mice

	Discussion

Top Abstract Materials and Methods Results Discussion References

Although it is well established that IDDM is a T lymphocyte–dependentautoimmune disease, the role of particular T cell subsets inthe disease process remains a matter of intense debate. Theemerging consensus, however, seems to be that diabetogenesisis initiated by autoreactive CD8⁺ T cells, that its progressionrequires the recruitment of autoreactive CD4⁺ T cells, and thatclinically relevant beta cell destruction is effected by bothCD4⁺ and CD8⁺ T cells recruited to the site later on in theprocess (45). This postulate would predict that naive, but potentiallydiabetogenic, autoreactive CD8⁺ T cells would be able to homeinto pancreatic islets and affect beta cell damage in the absenceof other T cell specificities. Here we have tested this hypothesisby comparing the ability of TCR transgenes derived from betacell–specific CD8⁺ or CD4⁺ T cells to trigger and/or to accelerate diabetogenesis in RAG-2⁺ and/or RAG-2^–/– TCR-transgenic NOD mice. We have shown that both TCR transgeneshave similar diabetogenic potential when expressed in wild-typeNOD mice, but not when expressed in RAG-2^–/– NODmice; although CD4⁺ T cells expressing the 4.1-TCR remainedhighly diabetogenic when maturing in the absence of endogenousT cells, CD8⁺ T cells expressing the 8.3-TCR did not. We havealso shown that these autoreactive CD8⁺ T cells do not requireCD4⁺ T cell help to mature properly, to proliferate in responseto antigenic stimulation, or to differentiate into CTLs, but that they require a CD4⁺ T cell–derived signal to efficiently home into pancreatic islets and effect clinically relevantbeta cell damage.

Expression of the TCR- ${alpha}$ and -β rearrangements of the betacell–cytotoxic CD8⁺ T cell clone NY8.3 in NOD mice skewedT cell development towards the CD8⁺ T cell subset, as expected,and accelerated the onset of IDDM by several months, as a resultof massive recruitment of naive CD8⁺ (and CD4⁺) T cells intopancreatic islets. Since the 8.3-TCR uses a TCR- ${alpha}$ –CDR3sequence that is highly homologous to that of TCRs used bymany NOD islet-derived beta cell–cytotoxic CD8⁺ T cells(25), we are confident that this TCR is representative of alarge fraction of MHC class I–restricted autoreactiveTCRs recruited to pancreatic islets in spontaneous IDDM. Thedramatic acceleration of diabetes in 8.3-NOD mice was not surprising,since it was consistent with the less dramatic, but significant,acceleration of diabetes that we had seen in transgenic NOD mice expressing only the TCR-β rearrangement of NY8.3 (26). The observation that disease acceleration occurred in 8.3-NOD and 8.3–TCR-β–transgenic NOD miceseemed, at first, to support the hypothesis that autoreactiveCD8⁺ T cells play a critical role in disease initiation. Thishypothesis, which is largely based on the observation thatβ2-microglobulin–deficient (17–19) and anti-CD8mAb-treated NOD mice (20) develop neither diabetes nor insulitis,proposes that CD8⁺ T cells affect the initial beta cell insultthat exposes beta cell autoantigens to APCs and diabetogenic CD4⁺ T cells in autoimmune diabetes. Two other observationsin 8.3-NOD and 8.3–TCR-β–transgenic NOD mice, however, argued against this scenario. First, the age at onset of insulitis in 8.3-NOD mice was delayed when compared tothe age at onset of insulitis in 8.3–TCR-β–transgenic and nontransgenic NOD mice, which have many fewer beta cell–reactiveCD8⁺ T cells than 8.3-NOD mice. Second, despite the large abundanceof beta cell–reactive CD8⁺ T cells in the peripherallymphoid organs of 8.3-NOD mice, and the dramatic accelerationof diabetes onset, the overall incidence of diabetes in thesemice was virtually identical to that seen in 8.3–TCR-β–transgenicand nontransgenic NOD mice. These observations, which are reminiscentof the inability of splenic CD8⁺ T cells from diabetic NOD miceto transfer insulitis into NOD.scid mice (6), suggested thatautoreactive (8.3-like) CD8⁺ T cells might function more aseffectors of beta cell damage, than as initiators of diabetogenesis.The invariable presence of beta cell–cytotoxic CD8⁺ Tcells in pancreatic islets of prediabetic and acutely diabeticnontransgenic NOD mice (21–25), and the ability of someislet-derived CD8⁺ CTL clones to effect beta cell destructionin vivo in the absence of CD4⁺ T cells (16, 32), are compatiblewith this view.

Studies of RAG-2^–/– 8.3-NOD mice provided additionalsupport for this interpretation of the data; these mice developeddiabetes less frequently and significantly later than 8.3-NODmice, thus indicating that 8.3-CD8⁺ T cells had lost most oftheir diabetogenic potential in the absence of B cells andendogenous T cells. Cytofluorometric and functional studiesof thymic and peripheral 8.3-CD8⁺ T cells of RAG-2^–/–8.3-NOD and 8.3-NOD mice indicated that deceleration of diabetesin RAG-2^–/– 8.3-NOD mice was not due to abnormalmaturation of 8.3-CD8⁺ T cells, to their inability to proliferatein response to beta cell autoantigen in vitro, or to their inabilityto differentiate into beta cell–cytotoxic effectors inthe absence of CD4⁺ Th cells. The fact that 8.3-CD8⁺ T cellsare not dependent on CD4⁺ Th cells for proliferation and differentiationinto CTLs is surprising, but not unprecedented. MHC class II–deficient(46) or CD4-deficient (47) mice, for example, have decreased helper activity for antibody responses, but have unimpaired CTL responses against viruses. Alternatively, the in vitro beta cell–cytotoxic potential of the islet-derived CD8⁺T cells of these mice is not acquired in vivo and is an artifact of in vitro manipulation, a possibility that we cannot ruleout at present. Whether this is the case or not, our data suggest that decelerated diabetogenesis in RAG-2^–/– 8.3-NOD mice results from a difficulty of naive 8.3-CD8⁺ T cells to home into and/or accumulate in pancreatic islets in the absenceof CD4⁺ T cells; nondiabetic mice did not have, or only hada low degree of, insulitis, and splenic CD4⁺ T cells from nontransgenicNOD mice were able to trigger the recruitment of diabetogenic8.3-CD8⁺ T cells into pancreatic islets when transfused intoRAG-2^–/– 8.3-NOD mice.

There are several possible mechanisms by which CD4⁺ T cellsmay foster the recuitment and/or accumulation of 8.3-CD8⁺ Tcells in islets. CD4⁺ T cells, and/or the numerous macrophagesthat are recruited to the site by CD4⁺ T cells (our unpublishedobservation), may secrete cytokines and/or chemokines that areessential for the recruitment of naive CD8⁺ T cells to the site(48). The observation that certain activated, beta cell–reactiveCD8⁺ clones can transfer diabetes into NOD.scid mice in theabsence of CD4⁺ T cells (16) is not incompatible with thisview; the homing potential of lymphocytes is a function oftheir activation state (49). An alternative, but not mutuallyexclusive, possibility is that since beta cells do not expressB7 costimulatory molecules (30), which are essential in T cellactivation and differentiation, accumulation of 8.3-CD8⁺ Tcells in islets may require the shedding of their target betacell autoantigen by a CD4⁺ T cell–mediated beta cell insultfollowed by its presentation by APCs capable of diverting exogenous antigens to the MHC class I antigen-processing pathway (e.g.,dendritic cells; reference 50). The fact that some RAG-2^–/–8.3-NOD mice do develop diabetes does not necessarily argueagainst this scenario; because of their unnaturally high frequency,some of the beta cell–reactive CD8⁺ T cells of thesemice may undergo activation in response to cross-reactive antigensor to autoantigenic molecules that are occasionally shed frombeta cells even in the absence of any autoimmune-mediated betacell damage.

The nature and specificity of the CD4+ T cells that may affectthe initial beta cell insult that results in the recruitmentand activation of naive MHC class I–restricted CD8⁺ Tcells (8.3-like) and other beta cell–cytotoxic effectorsin spontaneous IDDM is unknown. Although studies of individualTCR specificities do not allow to draw definitive conclusionsabout the relative roles of CD4⁺ versus CD8⁺ T cells in theinitiation of autoimmune diabetes, four different lines of evidencesuggest that 4.1-like CD4⁺ T cells may be capable of playingsuch a role. First, insulitis in 4.1-NOD mice appeared earlierthan in 8.3-NOD mice (33). Second, 4.1-NOD developed diabetesmore frequently than, but as early as, 8.3-NOD mice (33). Third,RAG-2^–/– 4.1-NOD mice developed diabetes as frequentlyand as early as 4.1-NOD mice, demonstrating that, unlike 8.3-CD8⁺T cells, 4.1-CD4⁺ T cells can efficiently home into and accumulatein pancreatic islets, differentiate into effector cells, andcause diabetes without the assistance of B cells or other Tcells. Finally, and most importantly, the 4.1-TCR has the uniqueability of engaging several distinct MHC class II moleculeson thymic bone marrow–derived APCs with consequencesthat are highly reminiscent of the MHC class II–linkedresistance of nontransgenic mice to insulitis and diabetes;antidiabetogenic MHC class II molecules can prevent the developmentof insulitis and diabetes by abrogating the development of4.1-like CD4⁺ T cells (33). The above hypothesis that diabetogenesismight be initiated by 4.1-like CD4⁺ T cells is not incompatiblewith the large body of evidence indicating that developmentof insulitis in nontransgenic NOD mice requires CD8⁺ T cellsand/or MHC class I molecules on beta cells (3–6, 17–20, 27, 28). Development of full-blown insulitis in nontransgenicNOD mice may require both an initial beta cell insult by 4.1-likeCD4⁺ T cells and the immediate recruitment and activation ofMHC class I–restricted CD8⁺ T cells. As pointed out abovefor RAG-2^–/– 8.3-NOD mice, the fact that diabetogenesisin RAG-2^–/– 4.1-NOD mice bypasses the need forCD8⁺ T cells does not contradict this view; the high frequencyof beta cell–reactive CD4⁺ T cells in 4.1-NOD mice mayoverwhelm the mechanisms that, in nontransgenic NOD mice, wouldprevent these cells from reaching an insulitogenic mass uponactivation.

We do not yet know why 4.1-like CD4⁺ T cells are so highlydiabetogenic; however, since beta cells do not normally expressMHC class II molecules (14, 15), it would not be unreasonableto speculate that the diabetogenic potential of 4.1-CD4⁺ Tcells stems from their ability to strongly engage autoantigen/I-A^g7complexes that are already present on the surface of localAPCs before any previous beta cell insult (e.g., secreted proteins).The fact that RAG-2^–/– 4.1-NOD mice do not developsialoadenitis, which is invariably present in nontransgenicNOD mice, does indeed suggest that both the recruitment andactivation of 4.1-CD4⁺ T cells are driven by local APCs. Sucha strong interaction between local APCs and 4.1-CD4⁺ T cellsmay trigger the upregulation of Fas ligand on the T cells,endowing them with the ability to kill bystander beta cells that have been induced (perhaps by cytokines) to express Fas(51). In fact, islet-derived 4.1-CD4⁺ T cells from 4.1-NOD miceare efficient killers of Fas cDNA-transfected fibroblasts invitro (our unpublished observations). These activated CD4⁺ Tcells may also be able to damage beta cells by activating thecytocidal activity (free radical production and cytokine secretion)of the numerous macrophages that they recruit to the site.

Our results do not imply that diabetogenesis in nontransgenicNOD mice is initiated by cells expressing the 4.1-TCR, nor dothey rule out the possibility that there might be CD8⁺ T cellspecificities with an independent ability to home into pancreaticislets and affect the initial beta cell insult before the recruitmentof CD4⁺ T cells into pancreatic islets (i.e., those recruitedto islets early in the disease process; reference 16). However,the strikingly different natural histories of diabetes in RAG-2^–/–8.3-NOD versus RAG-2^–/– 4.1-NOD mice, and the abilityof antidiabetogenic MHC class II molecules to prevent diabetogenesisin 4.1-NOD mice by interfering with the developmental biologyof the highly diabetogenic 4.1-TCR, lend support to our hypothesisthat diabetogenesis in nontransgenic NOD mice may be initiatedby 4.1-like CD4⁺ T cells, rather than by 8.3-like CD8⁺ T cells.

	Acknowledgments

We thank M. Davis, S. Hedrick, E.H. Leiter, P. Marrack, J.-I.Miyazaki, D. Remick, T. Utsugi, J. Yewdell, and J.-W. Yoonfor reagents; K. Hirasawa for advice on immunopathology; R.Sangha and R. Sparkes for help with histology; R. Dawson andL. Mock for animal care; L. Bryant for assistance with flowcytometry; and H. Kominek for editorial assistance.

Submitted: 7 July 1997
Revised: 25 August 1997

J. Verdaguer was supported by a postdoctoral fellowship fromCIRIT (Comissió Interdepartamental de Reçercai Innovació Tecnològica) Generalitat de Catalunya,Barcelona, Spain. P. Santamaria is a scholar of the MedicalResearch Council of Canada. This research was supported by grantsfrom the Medical Research Council of Canada, the Natural Sciencesand Engineering Council of Canada, and the Juvenile Diabetes Foundation International.

¹ Abbreviations used in this paper: CM, complete medium; HPRT,hypoxanthine phosphoribosyl transferase; IDDM, insulin-dependentdiabetes mellitus; NOD, nonobese diabetic; RAG, recombination-activatinggene.

References

Top
Abstract
Materials and Methods
Results
Discussion
References

1 Serreze DV & Leiter EH. Genetic and pathogenic basis of autoimmune diabetes in NOD mice, Curr Opin Immunol, 1994, 6, 900–906.[Medline]

2 Tisch R & McDevitt HO. Insulin-dependent diabetes mellitus, Cell, 1996, 85, 291–297.[Medline]

3 Bendelac A, Carnaud C, Boitard C & Bach J-F. Syngeneic transfer of autoimmune diabetes from diabetic NOD mice to healthy neonates. Requirement for both L3T4⁺ and Lyt-2⁺T cells, J Exp Med, 1987, 166, 823–832.[Abstract/Free Full Text]

4 Miller BJ, Appel MC, O'Neil JJ & Wicker LS. Both the Lyt-2⁺ and L3T4⁺T cell subsets are required for the transfer of diabetes in non-obese diabetic mice, J Immunol, 1988, 140, 52–58.[Abstract]

5 Yagi H, Matsumoto M, Kunimoto K, Kawaguchi J, Makino S & Harada M. Analysis of the roles of CD4+ and CD8+ T cells in autoimmune diabetes of NOD mice using transfer to NOD athymic nude mice, Eur J Immunol, 1992, 22, 2387–2393.[Medline]

6 Christianson SW, Shultz LD & Leiter EH. Adoptive transfer of diabetes into immunodeficient NOD-scid/scid mice. Relative contributions of CD4+ and CD8+ T-cells from diabetic versus prediabetic NOD.NON-thy-1a donors, Diabetes, 1993, 42, 44–55.[Abstract]

7 Reich EP, Sherwin RS, Kanagawa O & Janeway CA Jr. An explanation for the protective effect of the MHC class II I-E molecule in murine diabetes, Nature (Lond), 1989, 341, 326–328.[Medline]

8 Haskins K & McDuffie M. Acceleration of diabetes in young NOD mice with a CD4+ islet-specific T cell clone, Science (Wash DC), 1990, 249, 1433–1436.[Abstract/Free Full Text]

9 Nakano N, Kikutani H, Nishimoto H & Kishimoto T. T cell receptor V gene usage of islet beta cell–reactive T cells is not restricted in non-obese diabetic mice, J Exp Med, 1991, 173, 1091–1097.[Abstract/Free Full Text]

10 Bradley BJ, Haskins K, LaRosa FG & Lafferty K. CD8+ T cells are not required for islet destruction induced by a CD4+ islet-specific T-cell clone, Diabetes, 1992, 41, 1603–1608.[Abstract]

11 Daniel D, Gill RG, Schloot N & Wegmann D. Epitope specificity, cytokine production profile and diabetogenic activity of insulin-specific T cell clones isolated from the NOD mouse, Eur J Immunol, 1994, 25, 1056–1062.

12 Katz JD, Benoist C & Mathis D. T helper cell subsets in insulin dependent diabetes, Science (Wash DC), 1995, 268, 1185–1188.[Abstract/Free Full Text]

13 Peterson JD & Haskins K. Transfer of diabetes in the NOD-scid mouse by CD4 T cell clones. Differential requirements for CD8 T cells, Diabetes, 1996, 45, 328–336.[Abstract]

14 Signore A, Pozzilli P, Gale EAM, Andreani D & Beverley PCL. The natural history of lymphocyte subsets infiltrating the pancreas of NOD mice, Diabetologia, 1989, 32, 282–289.[Medline]

15 McInerney MF, Rath S & Janeway CA Jr. Exclusive expression of MHC class II proteins on CD45+ cells in pancreatic islets of NOD mice, Diabetes, 1991, 40, 648–651.[Abstract]

16 Wong FS, Visintin I, Wen L, Flavell RA & Janeway CA Jr. CD8 T cell clones from young NOD islets can transfer rapid onset of diabetes in NOD mice in the absence of CD4 T cells, J Exp Med, 1996, 183, 67–76.[Abstract/Free Full Text]

17 Katz J, Benoist C & Mathis D. Major histocompatibility complex class I molecules are required for the development of insulitis in non-obese diabetic mice, Eur J Immunol, 1993, 23, 3358–3360.[Medline]

18 Wicker LS, Leiter EH, Todd JA, Renjilian RJ, Peterson E, Fisher PA, Podolin PL, Zijlstra M, Jaenisch R & Peterson LB. β2-microglobulin–deficient NOD mice do not develop insulitis or diabetes, Diabetes, 1994, 43, 500–504.[Abstract]

19 Serreze DV, Leiter EH, Christianson GJ, Greiner D & Roopenian DC. Major histocompatibility complex class I–deficient NOD-β2m^nullmice are diabetes and insulitis resistant, Diabetes, 1994, 43, 505–508.[Abstract]

20 Wang B, Gonzalez A, Benoist C & Mathis D. The role of CD8+ T cells in initiation of insulin-dependent diabetes mellitus, Eur J Immunol, 1996, 26, 1762–1769.[Medline]

21 Hayakawa M, Yokono K, Nagata M, Hatamori N, Ogawa W, Miki A, Mizoguti H & Baba S. Morphological analysis of selective destruction of pancreatic beta cells by cytotoxic T lymphocytes in NOD mice, Diabetes, 1991, 40, 1210–1217.[Abstract]

22 Nagata M & Yoon J-W. Studies on autoimmunity for T-cell–mediated beta cell destruction, Diabetes, 1992, 41, 998–1008.[Abstract]

23 Shimizu J, Kanagawa O & Unanue E. Presentation of beta cell antigens to CD4+ and CD8+ T cells of non-obese diabetic mice, J Immunol, 1993, 151, 1723–1730.[Abstract]

24 Nagata M, Santamaria P, Kawamura T, Utsugi T & Yoon J-W. Evidence for the role of CD8+ cytotoxic T cells in the destruction of pancreatic beta cells in NOD mice, J Immunol, 1994, 152, 2042–2050.[Abstract]

25 Santamaria P, Utsugi T, Park B-J, Averill N & Yoon J-W. Beta cell–cytotoxic CD8+ T-cells from nonobese diabetic mice use highly homologous T-cell receptor ${alpha}$ -chain CDR3 sequences, J Immunol, 1995, 154, 2494–2503.[Abstract]

26 Verdaguer J, Yoon J-W, Anderson B, Averill N, Utsugi T, Park B-J & Santamaria P. Acceleration of spontaneous diabetes in TCRβ-transgenic nonobese diabetic mice by beta cell–cytotoxic CD8+ T-cells expressing identical endogenous TCR ${alpha}$ chains, J Immunol, 1996, 157, 4726–4735.[Abstract]

27 Kay TWH, Parker JL, Stephens LA, Thomas HE & Allison J. RIP-β2-microglobulin transgene expression restores insulitis, but not diabetes, in β2-microglobulin^nullnonobese diabetic mice, J Immunol, 1996, 157, 3688–3693.[Abstract]

28 Serreze DV, Chapman HD, Varnum DS, Gerling I, Leiter EH & Shultz LD. Initiation of autoimmune diabetes in NOD/Lt mice is MHC class I-dependent, J Immunol, 1997, 157, 3978–3986.

29 Thivolet C, Bendelac A, Bedossa P, Bach JF & Carnaud C. CD8+ T cell homing to the pancreas in the nonobese diabetic mouse is CD4+ T cell-dependent, J Immunol, 1991, 146, 85–93.[Abstract]

30 Stephens LA & Kay TWH. Pancreatic expression of B7 co-stimulatory molecules in the non-obese diabetic mouse, Int Immunol, 1995, 7, 1885–1895.[Abstract/Free Full Text]

31 Vyse TJ & Todd JA. Genetic analysis of autoimmune disease, Cell, 1996, 85, 311–318.[Medline]

32 Utsugi T, Yoon J-W, Park B-J, Imamura M, Averill N, Kawazu S & Santamaria P. Major histocompatibility complex class I–restricted infiltration and destruction of pancreatic islets by NOD mouse-derived β-cell cytotoxic CD8+ T-cell clones in vivo, Diabetes, 1996, 45, 1121–1131.[Abstract]

33 Schmidt D, Verdaguer J, Averill N & Santamaria P. A mechanism for the MHC-linked resistance to autoimmunity, J Exp Med, 1997, 186, 1059–1075.[Abstract/Free Full Text]

34 Sinkai Y, Rathbun G, Lam K-P, Oltz EM, Stewart V, Mendelsohn M, Charron J, Datta M, Young F, Stall AM & Alt FW. RAG-2–deficient mice lack mature lymphocytes owing to inability to initiate V(D)J rearrangement, Cell, 1992, 68, 855–867.[Medline]

35 Spevik T & Niessen-Meyer J. A highly sensitive cell line, WEHI 164 clone 13, for measuring cytotoxic factor/tumor necrosis factor from human monocytes, J Immunol Methods, 1986, 95, 99–106.[Medline]

36 Taffs, R., and M. Sitkovsky. 1992. Granule enzyme exocytosis assay for cytotoxic T lymphocyte activation. In Current Protocols in Immunology. J.E. Coligan, A.M. Krusbeek, D.H. Margulies, E.M. Shevach, and W. Strober, editors. John Wiley and Sons, New York. 3.16.1–3.16.8.

37 Wesselingh SL, Levine B, Fox RJ, Choi S & Griffin DE. Intracerebral cytokine mRNA expression during fatal and non-fatal alpha-virus encephalitis suggests a predominant type 2 T cell response, J Immunol, 1994, 152, 1289–1297.[Abstract]

38 Kisielow P, Bluthmann H, Staerz UD, Steinmetz M & von Boehmer H. Tolerance in T cell receptor transgenic mice involves deletion of nonmature CD4+CD8+ thymocytes, Nature (Lond), 1988, 333, 742–746.[Medline]

39 Berg LJ, Fazekas de St B, Groth, Pullen AM & Davis MM. Phenotypic differences between ${alpha}$ β vs β T-cell receptor transgenic mice undergoing negative selection, Nature (Lond), 1989, 340, 559–562.[Medline]

40 Berg LJ, Pullen AM, Fazekas de St B, Groth, Mathis D, Benoist C & Davis MM. Antigen/MHC-specific T-cells are preferentially exported from the thymus in the presence of their MHC ligand, Cell, 1989, 58, 1035–1046.[Medline]

41 Pircher H, Burki K, Lang R, Hengartner H & Zinkernagel RM. Tolerance induction in double specific T-cell receptor transgenic mice varies with antigen, Nature (Lond), 1989, 342, 559–561.[Medline]

42 Ohashi PS, Pircher H, Bürki K, Zinkernagel RM & Hengartner H. Distinct sequence of negative or positive selection implied by thymocyte T-cell receptor densities, Nature (Lond), 1990, 346, 861–863.[Medline]

43 Sha W, Nelson C, Newberry R, Kranz D, Russell J & Loh D. Positive and negative selection of an antigen receptor on T-cells in transgenic mice, Nature (Lond), 1988, 336, 73–76.[Medline]

44 Wicker LS, Appel MC, Dotta F, Pressey A, Miller BJ, DeLarato NH, Fischer PA, Boltz RC Jr & Peterson LB. Autoimmune syndromes in major histocompatibility complex (MHC) congenic strains of non-obese diabetic (NOD) mice. The NOD MHC is dominant for insulitis and cyclophosphamide-induced diabetes, J Exp Med, 1992, 176, 67–77.[Abstract/Free Full Text]

45 Benoist C & Mathis D. Cell death mediators in autoimmune diabetes: no shortage of suspects, Cell, 1997, 89, 1–3.[Medline]

46 Grusby MJ, Johnson RS, Papaioannou VE & Glimcher LH. Depletion of CD4⁺cells in major histocompatibility complex class-II–deficient mice, Science (Wash DC), 1991, 253, 1417–1420.[Abstract/Free Full Text]

47 Rahemtulla A, Fung-Leung WP, Schillam MW, Kundig TM, Sambhara SR, Narendran A, Arabian A, Wakeham A, Paige CJ, Zinkernagel RM et al.. Normal development and function of CD8+ cells but markedly decreased helper cell activity in mice lacking CD4, Nature (Lond), 1991, 353, 180–184.[Medline]

48 Mackay CR. Chemokine receptors and T cell chemotaxis, J Exp Med, 1996, 184, 799–802.[Free Full Text]

49 Butcher EC & Picker LJ. Lymphocyte homing and homeostasis, Science (Wash DC), 1996, 272, 60–66.[Abstract]

50 Germain R. MHC-dependent antigen processing and peptide presentation: providing ligands for T lymphocyte activation, Cell, 1994, 76, 287–299.[Medline]

51 Chervonsky AV, Wang Y, Wong FS, Visintin I, Flavell RA, Janeway CA Jr & Matis LA. The role of Fas in autoimmune diabetes, Cell, 1997, 89, 17–24.[Medline]

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Pauza, M. E., Dobbs, C. M., He, J., Patterson, T., Wagner, S., Anobile, B. S., Bradley, B. J., Lo, D., Haskins, K. (2004). T-Cell Receptor Transgenic Response to an Endogenous Polymorphic Autoantigen Determines Susceptibility to Diabetes. Diabetes 53: 978-988 [Abstract] [Full Text]
Lee, I-F., Qin, H., Trudeau, J., Dutz, J., Tan, R. (2004). Regulation of Autoimmune Diabetes by Complete Freund's Adjuvant Is Mediated by NK Cells. J. Immunol. 172: 937-942 [Abstract] [Full Text]
Thomas, H. E., Irawaty, W., Darwiche, R., Brodnicki, T. C., Santamaria, P., Allison, J., Kay, T. W.H. (2004). IL-1 Receptor Deficiency Slows Progression to Diabetes in the NOD Mouse. Diabetes 53: 113-121 [Abstract] [Full Text]
Yamanouchi, J., Verdaguer, J., Han, B., Amrani, A., Serra, P., Santamaria, P. (2003). Cross-Priming of Diabetogenic T Cells Dissociated from CTL-Induced Shedding of {beta} Cell Autoantigens. J. Immunol. 171: 6900-6909 [Abstract] [Full Text]
Hutton, J. C., Eisenbarth, G. S. (2003). A pancreatic {beta}-cell-specific homolog of glucose-6-phosphatase emerges as a major target of cell-mediated autoimmunity in diabetes. Proc. Natl. Acad. Sci. USA 100: 8626-8628 [Full Text]
Lieberman, S. M., Evans, A. M., Han, B., Takaki, T., Vinnitskaya, Y., Caldwell, J. A., Serreze, D. V., Shabanowitz, J., Hunt, D. F., Nathenson, S. G., Santamaria, P., DiLorenzo, T. P. (2003). Identification of the {beta} cell antigen targeted by a prevalent population of pathogenic CD8+ T cells in autoimmune diabetes. Proc. Natl. Acad. Sci. USA 100: 8384-8388 [Abstract] [Full Text]
Suri, A., Walters, J. J., Kanagawa, O., Gross, M. L., Unanue, E. R. (2003). Specificity of peptide selection by antigen-presenting cells homozygous or heterozygous for expression of class II MHC molecules: The lack of competition. Proc. Natl. Acad. Sci. USA 100: 5330-5335 [Abstract] [Full Text]
Serra, P., Amrani, A., Han, B., Yamanouchi, J., Thiessen, S. J., Santamaria, P. (2002). RAG-dependent peripheral T cell receptor diversification in CD8+ T lymphocytes. Proc. Natl. Acad. Sci. USA 99: 15566-15571 [Abstract] [Full Text]
Lesage, S., Hartley, S. B., Akkaraju, S., Wilson, J., Townsend, M., Goodnow, C. C. (2002). Failure to Censor Forbidden Clones of CD4 T Cells in Autoimmune Diabetes. JEM 196: 1175-1188 [Abstract] [Full Text]
McGargill, M. A., Mayerova, D., Stefanski, H. E., Koehn, B., Parke, E. A., Jameson, S. C., Panoskaltsis-Mortari, A., Hogquist, K. A. (2002). A Spontaneous CD8 T Cell-Dependent Autoimmune Disease to an Antigen Expressed Under the Human Keratin 14 Promoter. J. Immunol. 169: 2141-2147 [Abstract] [Full Text]
Nakayama, M., Nagata, M., Yasuda, H., Arisawa, K., Kotani, R., Yamada, K., Chowdhury, S. A., Chakrabarty, S., Jin, Z. Z., Yagita, H., Yokono, K., Kasuga, M. (2002). Fas/Fas Ligand Interactions Play an Essential Role in the Initiation of Murine Autoimmune Diabetes. Diabetes 51: 1391-1397 [Abstract] [Full Text]
Wen, L., Wong, F. S., Sherwin, R., Mora, C. (2002). Human DQ8 Can Substitute for Murine I-Ag7 in the Selection of Diabetogenic T Cells Restricted to I-Ag71. J. Immunol. 168: 3635-3640 [Abstract] [Full Text]
Zhang, Y., O'Brien, B., Trudeau, J., Tan, R., Santamaria, P., Dutz, J. P. (2002). In Situ {beta} Cell Death Promotes Priming of Diabetogenic CD8 T Lymphocytes. J. Immunol. 168: 1466-1472 [Abstract] [Full Text]
Serreze, D. V., Johnson, E. A., Chapman, H. D., Graser, R. T., Marron, M. P., DiLorenzo, T. P., Silveira, P., Yoshimura, Y., Nathenson, S. G., Joyce, S. (2001). Autoreactive Diabetogenic T-Cells in NOD Mice Can Efficiently Expand From a Greatly Reduced Precursor Pool. Diabetes 50: 1992-2000 [Abstract] [Full Text]
Amrani, A., Serra, P., Yamanouchi, J., Trudeau, J. D., Tan, R., Elliott, J. F., Santamaria, P. (2001). Expansion of the Antigenic Repertoire of a Single T Cell Receptor upon T Cell Activation. J. Immunol. 167: 655-666 [Abstract] [Full Text]
Bercovici, N., Heurtier, A., Vizler, C., Pardigon, N., Cambouris, C., Desreumaux, P., Liblau, R. (2000). Systemic Administration of Agonist Peptide Blocks the Progression of Spontaneous CD8-Mediated Autoimmune Diabetes in Transgenic Mice Without Bystander Damage. J. Immunol. 165: 202-210 [Abstract] [Full Text]
Kanagawa, O., Shimizu, J., Vaupel, B. A. (2000). Thymic and Postthymic Regulation of Diabetogenic CD8 T Cell Development in TCR Transgenic Nonobese Diabetic (NOD) Mice. J. Immunol. 164: 5466-5473 [Abstract] [Full Text]
Graser, R. T., DiLorenzo, T. P., Wang, F., Christianson, G. J., Chapman, H. D., Roopenian, D. C., Nathenson, S. G., Serreze, D. V. (2000). Identification of a CD8 T Cell That Can Independently Mediate Autoimmune Diabetes Development in the Complete Absence of CD4 T Cell Helper Functions. J. Immunol. 164: 3913-3918 [Abstract] [Full Text]
Anderson, B., Park, B.-J., Verdaguer, J., Amrani, A., Santamaria, P. (1999). Prevalent CD8+ T cell response against one peptide/MHC complex in autoimmune diabetes. Proc. Natl. Acad. Sci. USA 96: 9311-9316 [Abstract] [Full Text]
Kagi, D., Ho, A., Odermatt, B., Zakarian, A., Ohashi, P. S., Mak, T. W. (1999). TNF Receptor 1-Dependent {beta} Cell Toxicity as an Effector Pathway in Autoimmune Diabetes. J. Immunol. 162: 4598-4605 [Abstract] [Full Text]
Verdaguer2, J., Amrani2, A., Anderson, B., Schmidt, D., Santamaria, P. (1999). Two Mechanisms for the Non-MHC-Linked Resistance to Spontaneous Autoimmunity. J. Immunol. 162: 4614-4626 [Abstract] [Full Text]
Schmidt, D., Amrani, A., Verdaguer, J., Bou, S., Santamaria, P. (1999). Autoantigen-Independent Deletion of Diabetogenic CD4+ Thymocytes by Protective MHC Class II Molecules. J. Immunol. 162: 4627-4636 [Abstract] [Full Text]
Guerder, S., Eynon, E. E., Flavell, R. A. (1998). Autoimmunity Without Diabetes in Transgenic Mice Expressing {beta} Cell-Specific CD86, But Not CD80: Parameters that Trigger Progression to Diabetes. J. Immunol. 161: 2128-2140 [Abstract] [Full Text]
Geng, L., Solimena, M., Flavell, R. A., Sherwin, R. S., Hayday, A. C. (1998). Widespread expression of an autoantigen-GAD65 transgene does not tolerize non-obese diabetic mice and can exacerbate disease. Proc. Natl. Acad. Sci. USA 95: 10055-10060 [Abstract] [Full Text]
Susan Wong, F., Visintin, I., Wen, L., Granata, J., Flavell, R., Janeway, C. A. Jr. (1998). The Role of Lymphocyte Subsets in Accelerated Diabetes in Nonobese Diabetic-Rat Insulin Promoter-B7-1 (NOD-RIP-B7-1) Mice. JEM 187: 1985-1993 [Abstract] [Full Text]

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