Address correspondence to Paul M. Allen, Department of Pathology and Immunology, Washington University School of Medicine, Campus Box 8118, 660 South Euclid Avenue, St. Louis, MO 63110. Phone: (314) 362-8758; Fax: (314) 362-8888; email: allen{at}wustl.edu
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Abstract |
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Key Words: autoimmunity thymic deletion arthritis T regulatory cells TCR transgenic
B.T. Wipke's present address is Elan Pharmaceuticals, Inc., 800 Gateway Boulevard, Building 800, Room 154B, South San Francisco, CA 94080.
Abbreviations used in this paper: ANA, antinuclear antibodies; d3Ntx, day 3 neonatally thymectomized; GI, gastrointestinal; GPI, glucose-6-phosphate-isomerase; HEL, hen egg lysozyme; mHEL, membrane form of HEL; NOD, nonobese diabetic; SP, single positive; Tg, transgenic; Treg, regulatory T cell.
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Introduction |
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To investigate the role of antigen presentation in the failure in T cell selection, we have generated a Tg mouse expressing a peptide mimic of GPI(281293) termed G7m under the control of the MHC II promoter. Accordingly, we showed G7mTg splenocytes to be potent stimulators of KRN T cells, signifying effective presentation of the transgene-encoded agonist. As expected, KRN/G7mTg double Tg mice exhibited a greatly attenuated arthritis course with concomitant loss of anti-GPI T and B cell responses. Surprisingly, KRN/G7mTg mice succumbed to a systemic autoimmunity with multiorgan inflammation and autoantibody production. Expression of the TCR ligand resulted in severe deletion of T cells bearing transgene-encoded TCR, leaving behind autoreactive CD4+ T cells using endogenous TCRs. CD4+ CD25+ regulatory T cells (Tregs) were reduced in the double Tg mice, suggesting loss of Tregs as a mechanism of disease. Significantly, cotransfer of CD4+ CD25+ Tregs prevented induction of disease achieved via transfer of splenocytes from double Tg mice. Taken together, our studies demonstrated that central tolerance can paradoxically result in systemic autoimmunity through differential susceptibility of Tregs and autoreactive T cells to thymic deletion.
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Materials and Methods |
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KRN TCR Tg mice on a C57BL/6 background have been described (1). KRN Tg mice were bred to congenic B6.AKR (H-2k background) to generate KRNk mice, which are homozygous for H-2k. KRNk mice were crossed to G7mTgk mice to generate KRN/G7mTgk mice, which are then bred to NOD mice to generate KRNk/g7 and KRN/G7mTgk/g7 mice on an H-2k/g7 heterozygous background. B6.G7 denotes congenic C57BL/6 mice expressing I-Ag7. These were crossed to KRN/G7mTgk to generate congenic KRN/B6.G7 and KRN/G7mTg/B6.G7 mice expressing H-2k/g7 with pure B6 genetic background. NOD mice were purchased from Taconic. All mice were bred and housed under specific pathogen-free conditions in the animal facility at the Washington University Medical Center.
Primary T Cell Proliferation.
Proliferation assays were performed in triplicate with unfractionated T cells (5 x 105 cells/well) from the spleen and LNs in Iscove's medium containing 10% heat-inactivated fetal calf serum, 2 mM Glutamax (GIBCO BRL), 2 x 10-5 M ß-mercaptoethanol, and 50 µg/ml gentamicin (ISC-10) in round-bottom 96-well plates (Costar). Splenic APCs received 2,000 rad irradiation before use. Cultures were pulsed at 72 h with 0.2 µCi [3H]thymidine/well and harvested 1824 h later. Proliferation was measured as counts per minute incorporated.
In Vitro Suppression Assay.
T cell proliferation was assayed as described above with sorted CD4+ CD25+ and CD4+ CD25- T cells (at 5 x 104 cells/well) from KRNk/g7 mice being cultured separately or mixed at 1:1 in 96-well round-bottom plates with 5 x 105 irradiated T celldepleted H-2k/g7 splenic APCs.
Arthritis and Wasting Incidence.
Mice were assessed weekly for synovitis of the rear and front paws for 4 mo. Ankle thickness was measure axially across the malleoli using a Fowler Metric Pocket Thickness Gauge (Ralmikes Tool-A-Rama). Ankle thickness was rounded off to the nearest 0.05 mm. Mice were weighed weekly using a miniscale. Wasting is defined clinically as fur ruffling, hunched posture, and weight loss >20%. Mice were killed when moribund or weight fell below 12 g (<50% mean weight of control).
Anti-GPI ELISA.
Mice were bled weekly and sera were stored at -20°C before analysis. Sera were diluted at 1:100 in PBS, 1% BSA, and 0.1% Tween 20 and plated in Immunlon II plates (Fisher Biotech) coated with 2 µg/ml GPI-GST as previously described (9). Donkey antimouse horseradish peroxidase (Jackson ImmunoResearch Laboratories) was used as a secondary antibody. The assay was detected using 2,2'-Azino-di-(3-ethylbenathiazoline sulfonate) diammonium salt (ABTS substrate; Roche Molecular Biochemicals). Absorbance was measured at 414 nm.
Antinuclear Antibodies (ANA).
Sera was diluted at 1:100 in PBS. 50 µl diluted serum sample was applied to immobilized Hep2 cells (Antibodies Inc.) and Crithidia luciliae (Antibodies Inc.). Antimouse IgG-FITC and antimouse IgM-FITC were used as secondary antibodies. ANA and Crithidia staining were read independently by two readers. Positive controls were sera from MRL/lpr mice.
Anti-RBC Antibody.
Sera was diluted at 1:50 in FACS® buffer (PBS, 1% BSA, and 0.1% NaN3). 50 µl diluted sera was used to stain B6.AKR RBCs and was detected with antimouse IgG-FITC and antimouse IgM-FITC for flow cytometric analysis. Positives were defined as staining >3x background.
RF ELISA.
This RF ELISA made use of allotypic difference between the capture Ig (a allotype) and sample IgG of b allotype. Sera were diluted at 1:100 in PBS, 1% BSA, and 0.1% Tween 20 and plated in Immunlon II plates (Fisher Biotech) coated with 2 µg/ml IgG2aa (HOPC-1). A cocktail of biotinylated antibodies comprising of anti-IgM (11/41), anti-IgG2ab (5.7), and anti-IgG1b (B68-2; 2 µg/ml each), followed by SAVhorseradish peroxidase, was used for detection. HOPC-1, 11/41, 5.7, and B68-2 were purchased from Southern Biotechnology Associates, Inc. As b allotypespecific antibodies were available for only the IgG2a and IgG1 isotypes, RFs of the IgG2b or IgG3 isotypes were not detected. Hence, the RF measurement was likely to be an underestimate. The assay was developed using ABTS substrate. Positive was defined as OD > 3x background.
Flow Cytometry.
Single cell suspensions of thymocytes, splenocytes, and LN cells (12 x 106) were surface stained according to standard protocols. The following antibodies/reagents were used: GK1.5-PE, GK1.5-FITC (anti-CD4), 53-6.7FITC (anti-CD8), RR4-7biotin (anti-Vß6), 14.4.4-FITC (anti-I-Ek), PC61-PE (anti-CD25), MEL-14PE (antiCD62-L), PgP-1FITC (anti-CD44), H1.2F3-FITC (anti-CD69), streptavidin-PerCP (BD Biosciences), F10.6.6-biotin (HEL specific), 1G12-biotin (3A9 clonotype specific), and streptavidin-PE (Caltag). TCR Vß usage was determined by flow cytometry using a panel of 15 FITC-conjugated TCR Vß-specific antibodies from BD Biosciences. All samples were analyzed on a FACScaliburTM flow cytometer (BD Biosciences) with CELLQuestTM software. Gating on live lymphocytes was based on forward and side scatter and/or exclusion of propidium iodide. 50500,000 gated events were collected per sample.
Quantitative PCR.
CD4+ T cells were enriched from the spleen and LN cells from three to five 4-wk-old KRNk/k or KRNk/g7 mice using anti-CD4 microbeads (Miltenyi Biotec) according to the manufacturer's directions. CD4+ single positive (SP) thymocytes were isolated by complement-mediated depletion of CD8+ thymocytes using anti-CD8 antibody 3.166. CD4+ CD25+ and CD4+ CD25- T cells were sorted using the FACS VantageTM after labeling with antiGK1.5-FITC and PC61-PE. Typically, 0.5 x 106 CD4+ CD25+ T cells and 0.2 x 106 CD4+ CD25+ thymocytes were isolated from three to five mice. mRNA was isolated using TRIzol (Invitrogen) extraction and was treated with DNase I for 15 min at 25°C. First strand cDNA was generated using oligo-dT primers via TaqMan Reverse Transcription kit (Applied Biosystems) according to the manufacturer's directions. Real-time PCR for FoxP3 was measured as previously described (10) using TaqMan Universal Master Mix (Applied Biosystems). CD25 and HPRT PCR were performed as previously described (11) using SYBR Master Mix (Applied Biosystems). PCR was performed in 25 µl with cycling conditions as previously described (10). Data were collected using ABI Prism 7700 Sequence Detection System Software. A standard curve was generated with a dilution series (1:1, 1:10, 1:100, 1:1,000, 1:10,000, and 1:100,000) of a reference cDNA sample that was run at the same time as the unknown samples. CD25 and FoxP3 expression were normalized to HPRT mRNA.
Transfer Studies.
Spleens were harvested from 512-wk-old 3A9 or 3A9/G7mTg mice. Single cell suspension was generated by RBC lysis. Unfractionated splenocytes (3040 x 106) from one spleen were injected intravenously into each 46-wk-old B6.AKR or congenic RAG1-/- mouse. Equivalent numbers of T cells from 3A9 or 3A9/G7mTg mice were transferred. CD4+ CD25+ T cells comprised 1.5% (4.56 x 105) and <0.2% (<7 x 104) of total transferred cells from 3A9 and 3A9/G7mTg mice. Mice were followed weekly for weight loss and clinical evidence of disease.
For the cotransfer experiments, 5 x 105 CD4+ CD25+ or CD4+ CD25- T cells were purified from 3A9 mice via MACS (Miltenyi Biotec) separation according to the manufacturer's directions and injected intravenously into each RAG1-/- mouse 24 h before transfer of 3A9/G7m splenocytes. Some mice received 20 x 106 CD4+ CD25- T cells purified from 3A9 mice.
Online Supplemental Material.
Fig. S1 demonstrates the expression of the mHEL/G7m transgene on I-Ekexpressing cells in the thymic medulla of mHEL/G7mTg7 mice. Fig. S2 depicts the time course of wasting of representative KRN/G7mTg (Fig. S2 A) and 3A9/mHELTg (Fig. S2 B) mice. Fig. S3 illustrates the splenomegaly and disrupted splenic architecture seen in KRN/G7mTg7 mice. Figs. S1S3 are available at http://www.jem.org/cgi/content/full/jem.20031137/DC1.
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Results |
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The transgene was expressed in the majority of MHC II+ cells in the spleen, LN, and thymus. In the thymus, mHEL/G7m chimeric molecules were expressed most highly in the medulla, coinciding with MHC II+ cells (Fig. S1, top, available at http://www.jem.org/cgi/content/full/jem.20031137/DC1). Hence, we showed that the transgene was appropriately targeted to thymic medullary cells, which have previously been shown to be exquisitely effective at mediating thymic negative selection (12).
Moreover, when we bred G7mTg7 mice to NOD mice to introduce the I-Ag7 molecule, the resultant G7mTg7k/g7 splenocytes provoked vigorous proliferation of KRNk T cells in comparison to the modest response elicited by transgene-negative and NOD splenocytes (Fig. 1). Indeed, expression of the mHEL/G7m transgene augmented T cell stimulation by 1,000-fold relative to that achieved with endogenous GPI, highlighting the enhanced presentation of the KRN TCR ligand through our targeted transgene approach.
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Next, we assessed T cell response to GPI(281293) in KRN/G7mTg7k/g7 mice relative to their KRNk/g7 littermate. In contrast to the residual but significant GPI reactivity exhibited by KRNk/g7 splenocytes, no proliferation was elicited from splenocytes isolated from KRN/G7mTg7k/g7 mice (Fig. 2 C). Hence, GPI-specific T cells were functionally eliminated. Taken together, overexpression of the KRN TCR agonist abrogated arthritis and anti-GPI B and T cell responses, demonstrating effective T cell tolerance of KRN T cells in KRN/ G7mTg7k/g7 mice.
KRN/G7mTg7k/g7 Mice Develop Multiorgan Inflammation.
Surprisingly, KRN/G7mTg7k/g7 mice developed multiorgan systemic autoimmunity. Starting at 1012 wk of age, the mice exhibited wasting, manifested as ruffled fur, scaly skin, hunched posture, colitis, and weight loss. By 100 d of age, 50% of the KRN/G7mTg7k/g7 (n = 16) mice had succumbed to wasting. A representative time course is presented in Fig. S2 A, available at http://www.jem.org/cgi/content/full/jem.20031137/DC1. The remaining mice became progressively affected, such that by 6 mo of age only 20% remained. With the exception of arthritis in KRNk/g7 mice, KRNk/g7 (n = 20) and G7mTg7k/g7 (n = 15) mice were otherwise healthy throughout this time course.
A survey of multiple organs from 420-wk-old KRN/G7mTg7k/g7 mice revealed involvement of the liver, kidneys, lungs, heart, pancreatic islets, salivary glands, thyroid, and gastrointestinal (GI) tract. No histologic inflammation was seen in the muscle, skin, brain, ovaries, and testes. Two patterns of inflammatory infiltrates were observed. The first was well-organized perivascular infiltrates comprised of T and B cells, as well as neutrophils, seen in the liver, kidneys, lungs, pancreatic islets, and salivary glands (Fig. 3, AC, and unpublished data). In the more affected organs, the infiltrates eroded through the vessel walls with resultant vasculitis occluding the lumen. The organ parenchyma was relatively spared as there was no hepatocellular necrosis or glomerulonephritis. These perivascular lesions were observed in all the KRN/G7mTg7k/g7 mice as early as 4 wk of age, albeit to a lesser degree.
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KRNk/g7 mice exhibited inflammatory infiltrates in the periarticular regions as previously reported (1). Of the multiple visceral organs surveyed in 8 KRNk/g7 mice, perivascular infiltrates in the lungs were seen in one 3-mo-old mouse. No other pathologic abnormality was evident (Fig. 3, DF, I, and J). Organs from control G7mTg7k/g7 mice were notably normal.
To exclude infection as the cause of the inflammation, KRN/ G7mTg7k/g7 mice were screened and were negative for respiratory and enteric pathogens including rodent Helicobacter spp. with the exception of lactose-negative Escherichia coli. Thus, by overexpressing the KRN TCR ligand in MHC II+ cells, the disease phenotype was diverted from a largely joint-centered disease to a lethal multiorgan systemic inflammation.
Splenomegaly with Extramedullary Hematopoiesis in KRN/G7mTg7k/g7 Mice.
KRN/G7mTg7k/g7 mice displayed significant splenomegaly, two- to fourfold greater than their KRNk/g7 littermates (Fig. S3 A, available at http://www.jem.org/cgi/content/full/jem.20031137/DC1). The anatomic distinction between red and white pulp in the spleen was obliterated by the presence of exuberant extramedullary hematopoiesis. No normal lymphoid follicles were discernible (Fig. S3, B and C, available at http://www.jem.org/cgi/content/full/jem.20031137/DC1). Correspondingly, complete blood counts and peripheral blood smears from KRN/G7mTg7k/g7 mice revealed autoimmune hemolytic anemia and compensatory reticulocytosis. There was also markedly enhanced granulocytosis with elevated numbers of neutrophils and immature band forms in the peripheral blood, indicative of acute inflammation (unpublished data).
Autoantibody Production in KRN/G7mTg7 Mice.
Given the disease involvement in multiple organ systems, we next assessed for the presence of autoantibodies commonly associated with systemic autoimmunity. Although KRN/G7mTg7k/g7 mice did not produce anti-GPI antibodies, they were hypergammaglobulinemic (unpublished data) and produced autoantibodies of multiple specificities. ANA were detected in the sera of all the KRN/G7mTg7k/g7 mice tested (n = 30), as early as 5 wk of age (before the onset of overt disease). The specificity of ANA was confirmed to be double stranded DNA by positive staining for the kinetoplast of C. luciliae. RF (anti-IgG antibodies) was detected in 67% of the KRN/G7mTg7k/g7 mice (n = 15) in contrast to their absence in KRNk/g7 mice. In addition, anti-RBC antibodies were detected in 50% of the KRN/G7mTg7k/g7 sera (n = 14). The production of disease-associated autoantibodies was not the result of indiscriminate polyclonal B cell activation as antibodies to GPI or neoself-antigen, HEL, were not produced (unpublished data).
NOD Background Is Not Required for Disease Development.
To ascertain whether the NOD background was necessary for disease manifestation, KRN/G7mTg7k mice were bred to congenic B6.G7 mice to introduce I-Ag7 while maintaining a pure B6 genetic background. Similar to KRN/G7mTg7k/g7 mice, KRN/G7mTg7/B6G7k/g7 mice did not develop arthritis but succumbed to multiorgan inflammation, colitis, hematologic abnormalities, and autoantibodies (ANA and RF). The tempo of disease was accelerated. All KRN/G7mTg7/B6.G7k/g7 mice succumbed to wasting by 3 mo of age. Despite sharing some of the inflammatory changes of aged NOD mice, the systemic autoimmunity seen in KRN/G7mTg7k/g7 mice did not require the NOD genetic background. Indeed, the NOD background genes conferred a degree of protection, as the disease course was less severe in the KRN/G7mTg7k/g7 mice (B6xNOD background) compared with the KRN/G7mTg7/B6.G7k/g7 mice (homozygous B6 background).
To exclude a transgene founder effect, KRN mice were crossed to another G7mTg line, designated G7mTg5. KRN/G7mTg5k/g7 mice displayed a similar disease phenotype as KRN/G7mTg7k/g7 mice with an attenuated arthritis course (Table I). They did not produce anti-GPI antibodies but produced ANA in all the mice assayed. KRN/G7mTg5k/g7 mice also succumbed to the multiorgan disease seen in KRN/G7mTg7k/g7 mice (Table I and Fig. S2 A, which is available at http://www.jem.org/cgi/content/full/jem.20031137/DC1).
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Consistent with negative selection, there was graded reduction of thymocyte numbers in KRNk/g7 and KRN/G7mTg7k/g7 mice relative to KRNk mice (Fig. 4 A). Deletion of KRN T cells by endogenous GPI in KRNk/g7 mice was relatively inefficient as the thymocyte numbers were reduced only threefold with preservation of the CD4/CD8 profile. In contrast, thymocyte deletion in KRN/G7mTg7k/g7 mice was much more effective with a 100-fold reduction in total cellularity. Analysis of the CD4/CD8 compartments showed that the loss was primarily in the double positive thymocytes with preservation of CD4+ SP thymocytes compared with the CD8+ SP thymocytes.
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To determine the TCR usage in the remaining CD4+ T cells, we conducted flow cytometric analysis using a panel of 15 Vß-specific antibodies. There was a dramatic shift in the TCR repertoire such that >50% of the residual CD4+ T cells in the KRN/G7mTg7k/g7 mice used Vß2 in contrast to 6.5% in the KRNk/g7 mice (Fig. 4 B). There was no significant difference among the other endogenous Vß genes. Vß2+ T cells were not selectively elevated in either G7mTg7 or non-Tg mice on the H-2k/g7 background (unpublished data). It was plausible that the Vß2 expansion resulted from aberrant thymic selection for HEL-specific T cells in KRN/G7mTg7k/g7 mice. To address this possibility, we assayed for T cell proliferation in response to HEL protein and the five identified MHC II determinants of HEL. No HEL-specific T cell response was detected (unpublished data). Therefore, this oligoclonal expansion of Vß2+ T cells is likely a reflection of autoreactive T cells that had evaded deletion and expanded in response to self-antigen as had been seen in certain autoimmune disease such as experimental autoimmune encephalomyelitis (13).
CD4+ T cells from KRN/G7mTg7k/g7 and KRNk/g7 mice displayed activation markers consistent with previous antigen exposure. In KRNk/g7 mice, increased numbers of CD4+ T cells were CD44hi and CD62Llo compared with KRNk mice (Fig. 4 C). These data are consistent with the immune activation of KRN T cells by endogenous GPI. CD4+ T cells in KRN/G7mTg7k/g7 mice exhibited a further elevation in activation markers, such that 91% of the CD4+ T cells were CD44hi CD62Llo (Fig. 4 C). In addition, these activated T cells exhibited elevated CD69 levels as well as increased cell volume by forward and side scatter (unpublished data).
Despite the activated phenotype of the CD4+ T cells derived from KRN/G7mTg7k/g7 mice, only 6% of these CD4+ T cells were CD25hi, whereas 20% of CD4+ T cells from KRNk/g7 mice were CD25hi (Fig. 4 C). As KRN T cells were activated by endogenous GPI in KRNk/g7 mice, the enhanced CD4+ CD25+ T cells may reflect peripherally activated T cells or CD4+ CD25+ Tregs. To distinguish between these two possibilities, we assessed the expression of the forkhead transcription factor, FoxP3, by quantitative PCR. FoxP3 had been identified as critical in the development of CD4+ CD25+ Tregs (10, 11). CD4+ CD25- and CD4+ CD25+ T cells were sorted from pooled LN cells and splenocytes from three to five KRNk/k and KRNk/g7 mice. Expression of CD25 and FoxP3 were analyzed by quantitative PCR and normalized to the housekeeping gene HPRT. FoxP3 was expressed in low abundance but correlated with CD25 expression in both KRNk/k and KRNk/g7 mice (Fig. 5 A). Moreover, to show that these are indeed Tregs, we assayed the ability of CD4+ CD25+ T cells from KRNk/g7 mice to suppress the proliferation of their CD4+ CD25- counterparts. CD4+ CD25+ T cells proliferated poorly in response to GPI compared to the response elicited in CD4+ CD25- T cells. The addition of CD4+ CD25+ Tregs at a 1:1 ratio reduced proliferation by 7085% (Fig. 5 B). Hence, CD4+ CD25+ T cells from KRNk/g7 mice expressed FoxP3 and functioned as Tregs.
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The paucity of CD4+ CD25+ T cells coupled with the severe thymic atrophy and lymphopenia in KRN/G7mTg7k/g7 mice precluded similar analyses in these mice. In day 3 neonatally thymectomized (d3Ntx) mice, loss of CD4+ CD25+ Tregs was shown to result in systemic autoreactivity (14, 15). In light of the regulatory function exhibited by CD4+ CD25+ T cells from KRNk/g7 mice and the similar disease manifestation seen in KRN/G7mTg7k/g7 and d3NTx mice, our data suggest loss of Tregs as a mechanism for the systemic autoreactivity.
Systemic Autoimmunity Is Generalizable to Settings of Extensive Thymic Deletion.
To determine if the disease phenotype was unique to KRN or was a generalizable phenomenon, we made use of 3A9 TCR Tg that recognizes HEL. Moreover, as HEL is a component of the mHEL/G7m transgene and clonotypic antibody to the 3A9 TCR is available, we could directly examine negative selection of 3A9 in mHEL/G7m. Accordingly, 3A9 TCR Tg mice were crossed to both G7mTg lineages. Consistent with efficient thymic deletion, clonotype+ 3A9 T cells were eliminated in 3A9/G7mTg mice (Fig. 6). As summarized in Table I and Fig. S2 B, which is available at http://www.jem.org/cgi/content/full/jem.20031137/DC1, both lineages of 3A9/G7mTg mice succumbed to disease with wasting, colitis, dermatitis, and autoantibody production starting at 910 wk of age. Compared with KRN/G7mTgk/g7 mice, 3A9/G7mTg mice displayed a higher frequency of wasting and colitis (8094 vs. 50%) and lower frequency of autoantibody production. ANA were produced in 4060% of 3A9/G7mTg mice and developed at a later time (812 wk). Histologically, 3A9/G7mTg mice also displayed multiorgan inflammation, albeit in only a subset of target organs (lungs, liver, and GI tract).
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Transfer of 3A9/G7m Splenocytes Recapitulates Disease Phenotype.
Next, we ascertained whether the disease is transferable by splenocytes. We made use of the 3A9 system where the expression of the cognate antigen can be controlled. Accordingly, unfractionated splenocytes from 3A9/G7mTg mice were transferred into B6.AKR mice. Control mice received unfractionated 3A9 splenocytes. Mice were monitored weekly by clinical appearance and weight. Transfer of 3A9/G7mTg splenocytes into B6.AKR mice did not induce disease. Recipients remained healthy and continued to gain weight compared to control mice that received 3A9 splenocytes (Fig. 7 A). Failure to transfer disease may result from a requirement for mHEL/G7m expression in the host or active suppression by host lymphocytes. As the reduction of CD4+ CD25+ T cells in the KRN/G7mTg7k/g7 mice suggested the loss of Tregs as a mechanism accounting for the systemic autoimmunity seen in these double Tg mice, we repeated the experiment using immunodeficient RAG1-/- hosts. Transfer of 3A9/G7mTg splenocytes into RAG1-/- mice recapitulated the disease phenotype present in 3A9/G7mTg mice. RAG1-/- mice that received 3A9/G7mTg splenocytes displayed steady weight loss with >25% weight loss by 24 d (Fig. 7 B). These mice were moribund and were killed. Histologic examination showed inflammatory changes in the liver, colon, and cecum similar to that seen in double Tg mice (unpublished data). RAG1-/- mice that received 3A9 splenocytes remained healthy. Moreover, the ability to transfer disease into host mice that do not express the mHEL/G7m transgene indicated that anti-HEL T cell response was not required for disease induction consistent with the loss of clonotype+ T cells in 3A9/G7mTg mice. Therefore, the autoreactivity resulted from the specificity encoded by endogenously derived TCRs.
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Discussion |
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Thymic deletion is the major mechanism whereby autoreactive T cells are eliminated from the functional T cell repertoire. Incomplete thymic deletion allows autoreactive T cells to persist in the periphery where under certain conditions they are activated and cause disease. Mechanisms such as the induction of extrathymic deletion, anergy, and Tregs offer a buttress against the dangers of autoimmunity. In this study, we showed that the extremes of negative selection to a self-antigen can both result in autoimmunity and disease. In KRNk/g7 mice, presentation of endogenous GPI was insufficient to effect complete deletion of KRN T cells resulting in their activation and arthritis through provision of T cell help to anti-GPI B cells. Overexpression of its TCR ligand G7m in the thymus deleted >99% of T cells with elimination of CD4+ CD25+ Tregs. Residual effector T cells bearing endogenously encoded TCRs with likely low affinity recognition for peripheral self-peptides escape thymic deletion and expand in the periphery through homeostatic proliferation and release from Treg inhibition to cause systemic disease.
KRN/G7mTgk/g7 and 3A9/mHEL mice differed critically from the growing rank of systemic autoimmune disease models generated through targeted gene disruption, such as CTLA-4-/-, TGFdnR, and IL-10R-/- mice (for review see reference 17) in that multiorgan systemic autoreactivity arose paradoxically in the setting of tolerance induction. Instead of the generalized lymphadenopathy and an expanded T cell compartment seen in the majority of these autoimmune models, KRN/G7mTgk/g7 and 3A9/mHEL mice exhibited a paucity of T cells. The thymi and peripheral LNs were atrophic, an expected finding given the purposeful targeting of the antigen to sites mediating negative selection. As such, these mice more closely resembled autoreactivity associated with lymphopenia such as TCR C-/- and d3Ntx mice. Although KRN/G7mTg and 3A9/mHEL mice exhibited an ulcerative colitis-like disease as do the TCR C
-/- mice (18), the disease in the KRN/G7mTg mice was more extensive affecting multiple organs and involving autoantibody production. The disease phenotype of KRN/G7mTg and 3A9/mHEL mice resembled the wasting disease described in neonatally thymectomized mice (19, 20). The mechanism of this autoimmunity has yet to be defined. In the more extensively studied d3NTx model of autoimmunity, autoimmune gastritis and oophoritis were mediated by T cells with specificity for peripherally expressed antigens: gastric parietal H+/K+ ATPase (21) and ovarian antigen (22), respectively. Autoimmunity to these peripheral antigens was attributed to the absence of thymically derived CD4+ CD25+ Tregs, whose restoration abrogated disease (14). Similarly, we showed here that depletion of CD4+ CD25+ Tregs conferred disease phenotype and the addition of CD4+ CD25+ Tregs prevented disease induction. In contrast to the surgical thymectomy models, we achieved such overwhelming thymocyte depletion via the thymic expression of a highly potent TCR ligand.
Numerous models of thymic tolerance had been described with diverse results. As allelic exclusion of transgene-encoded TCR was incomplete, coexpression of endogenously encoded TCRs allowed the generation of a repertoire of T cell specificities separate from those encoded by the transgenes. In some studies, coexpression of dual TCRs allowed autoreactive T cells to escape from negative selection and become activated upon recognition of their cognate antigen in the periphery to cause disease (2326). In those cases, the autoreactivity was confined to that of the transgene-encoded TCR. Our system differed critically from these models in that the transgene TCR specificity was not required for disease as pathology can be elicited in recipient mice that do not express the cognate antigen. In other TCR systems, deletion in response to antigens such as superantigens resulted in no pathology. In accordance with previous observation, we found superantigen (Mls-1a)-mediated deletion of KRN T cells to be delayed and less efficient. There was no ensuing disease (unpublished data). Yet other systems demonstrated the generation of Tregs through the recognition of self-peptide (2730). Interestingly, it is weak recognition of self-peptide that gave rise to Tregs. As such, it is intriguing that CD4+ CD25+ Tregs are increased in KRNk/g7 mice. One question that had been unanswered is why KRNk/g7 mice were not subjected to systemic autoimmunity given the ubiquitous presentation of GPI. As we have shown, thymic presentation of GPI is insufficient to induce complete deletion of KRN T cells but does induce the development of GPI-specific CD4+ CD25+ Tregs, which may provide a mechanism whereby the autoreactivity is limited to humorally mediated joint-specific disease. Precedents of such modulation of autoaggression by Tregs had previously been demonstrated in the IDDM and experimental autoimmune encephalomyelitis models (31, 32). In the face of overwhelming antigen dose due to overexpression of a strong TCR agonist, Tregs may indeed be deleted. This is consistent with our observation that HEL-specific 3A9 TCR Tg mice also developed systemic autoreactivity when crossed to mHEL Tg mice. 3A9 T cells are exquisitely sensitive to HEL(4661) and can be deleted by 10100 HEL(4661)I-Ak complexes on APC surfaces (33). Thus, overly efficient deletion of 3A9 may eliminate Tregs from the repertoire. It is, therefore, the convergence of high ligand density and/or TCR binding affinity that results in T cell overstimulation and deletion. The requirement for these two factors to coexist may explain the lack of systemic autoreactivity seen in some but not all TCR systems (3436). It is also possible that the TCR Tg mice were not followed for sufficient time for disease to manifest, as we had demonstrated with 3A9/JB5 mice.
What could account for the differential susceptibility of Tregs and pathologic effector T cells to deletion? Although the mechanism of Tregs differentiation is yet unclear, selective loss of Tregs from the repertoire in B7.1/B7.2- (37) and Foxp3-deficient (10, 11) mice suggests that Tregs and effector T cells arise from different maturation programs. As Tregs required cognate interaction with their ligand for differentiation, they may exhibit higher affinity for self-peptideMHC complex and thus be more susceptible to deletion compared with those expressing other autoimmune specificities to peripherally derived antigens. The preferential outgrowth of effector CD4+ T cells using endogenously encoded Vßs provides support to this hypothesis. An alternative possibility is that Tregs and autoimmune T cells arise at a distinct time course in ontogeny as shown by d3Ntx models and represent different lineages. Therefore, they might be subjected to different selection pressures.
In addition to the loss of Tregs from the T cell repertoire, a critical component to the disease phenotype is the requirement for homeostatic proliferation as lymphopenia was a shared feature in both TCR/antigen models and d3NTx mice. However, the homeostatic proliferation is not indiscriminate as only Vß2+ T cells were selectively expanded in KRN/G7mTg7k/g7 mice, suggesting that this expansion is antigen driven. Stimulation of Vß2+ T cells by BALB/cV virus in H-2d and H-2a had been previously reported correlating with deletion of Vß2+ T cells (38). No known endogenous Vß2-specific superantigens had been found in B6 nor NOD mice, hence this expansion is unlikely to be superantigen related. Therefore, these cells represent endogenous autoreactive T cells that escape negative selection and in the setting of lymphopenia and absence of Tregs, cause systemic autoimmunity.
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Acknowledgments |
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This work is supported by grants from the National Institutes of Health. F.F. Shih is supported by a grant from the Pediatric Scientist Development Program (National Institute of Child Health and Human Development).
Submitted: 10 July 2003
Accepted: 2 December 2003
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