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Introduction
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During development, T cells whose antigen receptors are devoid of self-reactivity exit the thymus and participate in immune surveillance, whereas those bearing receptors endowed with self-reactivity are negatively selected and deleted by programmed cell death 1. This process of T cell screening and selection, known as central tolerance, requires the antigen to be available in the thymus in sufficient quantities and in a form presentable by MHC molecules 2345. Although central tolerance exerts a tight control on the shaping of the T cell repertoire, some self-reactive T cells still escape the thymus and migrate to the periphery 678. If the antigen is available in the periphery, a second round of T cell screening, known as peripheral tolerance, will follow to further minimize autoreactivity 3910111213. Presumably, peripheral tolerance develops as a consequence of presentation of autoantigen by nonactivated APCs expressing minimal or no costimulatory molecules 314.
For sequestered autoantigens that are not available for presentation in either the thymus or the periphery, the corresponding T cells will circulate harmlessly. However, events that trigger exposure of those autoantigens, which are usually accompanied by conditions favorable for activation of local APCs, lead to an optimal presentation to and activation of the circulating T cells 15161718. The results of this T cell activation may be the escalation of inflammatory reactions and injury of specific tissues and organs 192021.
Supply of antigen in an adjuvant free form might not stimulate the expression of costimulatory molecules on APCs and thereby drive an antigen presentation inadequate for T cell activation 32223. Prior studies have in fact indicated that this approach modulates autoreactive T cells and promotes recovery from illness 242526. However, the usefulness of this approach for modulation of autoimmunity is hampered by the unlimited availability of autoantigen at the injury site and the consequent continuous activation of the self-reactive T cells. In addition, as bystander suppression is unlikely to occur, the approach holds little promise for modulation of T cell–mediated autoimmunity involving multiple antigens. To overcome these issues, an in vitro approach that uses plasmid 27 and viral 2829 vector-driven modulatory cytokines was adopted. Indeed, autoreactive T cell clones or hybridomas expressing the cytokine IL-4 or IL-10, as a consequence of transfection or infection, induced recovery from disease when injected into animals with ongoing experimental autoimmune encephalomyelitis (EAE) 2728. This is a promising approach and bodes well for the development of practical strategies that could combine both peripheral tolerance and cytokine antagonism to combat autoimmunity.
It has previously been shown that peptide delivery on Igs increases presentation by 100–1,000-fold relative to free peptide 3031. It is also known that cross-linking of Fc receptors (FcRs) on target cells by antigen–antibody complexes can trigger the production of cytokines 323334. Moreover, aggregation of Igs confers the effector functions associated with the Fc fragment without the need for complex formation 3536. Here, the encephalitogenic proteolipid protein (PLP)1 was genetically engineered into an Ig molecule 30, and the resulting Ig-PLP1 chimera was aggregated and assayed for modulation of autoreactive T cells and amelioration of active EAE. The results show that aggregated (agg) Ig-PLP1 induced IL-10 secretion by both macrophages and dendritic cells (DCs) but not B cells. In vitro, APCs incubated with agg Ig-PLP1 presented PLP1 to specific T cells. However, because of the IL-10 secreted by the presenting APCs, IFN-
production by the T cells was impaired. In vivo, when soluble (sol) Ig-PLP1 was injected into mice with ongoing EAE, the severity of disease was slightly reduced. However, when mice were given agg Ig-PLP1, full recovery was achieved. Moreover, agg Ig-PLP1 was able to modulate disease induced by either an encephalitogenic peptide other than PLP1 or by a central nervous system (CNS) homogenate. Neutralization of endogenous IL-10 by injection of anti–IL-10 antibody during administration of agg Ig-PLP1 restored disease severity. Therefore, agg Ig-PLP1 triggers IL-10 production by APCs, drives inadequate peripheral presentation of PLP1, and couples both events to modulate autoimmunity involving diverse T cell specificities.
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Materials and Methods
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Animals.
SJL/J (H-2S) mice were purchased from Harlan, bred, and maintained in our animal care facility for the duration of the experiments.
Antigens
Peptides.
The peptides used in this study were purchased from Research Genetics, and were HPLC purified to >90% purity. PLP1 peptide (HSLGKWLGHPDKF) encompasses amino acid (aa) residues 139–151 of PLP and is encephalitogenic in SJL/J mice 37. PLP2 peptide (NTWTTCQSIAFPSK), encompassing aa 178–191 of PLP, is likewise encephalitogenic in SJL/J 38. Myelin basic protein (MBP)-3 peptide (VHFFKNIVTPRTP) corresponding to aa residues 87–99 of MBP is also I-AS restricted, and induces EAE in SJL/J mice 39. Hemagglutinin (HA) peptide, an I-Ed–restricted epitope 31, corresponding to aa residues 110–120 of HA, was used for negative control purposes.
CNS Homogenate.
50 frozen unstripped rat brains (Pelfreez Biologicals) were homogenized in PBS using a Waring blender and adjusted to 300 mg/ml with PBS. CNS homogenate was stored at –20°C.
Ig-PLP Chimeras.
The Ig-PLP1 and Ig-PLP2 chimeras harbor, within the heavy chain CDR3 region, PLP1 and PLP2, respectively, and have been described previously 304041. Ig-W is the parental IgG2b antiarsonate antibody, 91A3, not encompassing any PLP peptide, and has been described elsewhere 30. Large-scale cultures of Ig-W, Ig-PLP1, and Ig-PLP2 transfectants were performed in DMEM containing 10% serum supreme (BioWhittaker) and purified on separate rat anti–mouse 
chain sepharose columns to avoid cross-contamination. Subsequently, the Ig chimeras were dialyzed against PBS and concentrated on collodion membranes (Schleicher & Schuell). The chimeras were aggregated by precipitation with 50% saturated (NH4)2SO4 as described 42. In brief, filtered 100% saturated (NH4)2SO4 was added at an equal volume to the sol Ig chimera preparation. The mixture was incubated at 24°C for 1 h with gentle agitation every 20 min. Subsequently, the samples were spun down at 10,000 rpm, and the pellet was resuspended at 1 mg/ml in PBS. Electrophoresis on a 10% acrylamide gel indicated that the sol Ig chimera entered the gel and migrated 
160 kD. However, the agg Ig chimera did not enter the gel. Knowing that we applied the equivalent of 2 µg of agg Ig chimera, and that the sensitivity of the technology is 0.1 µg, we concluded that at least 95% of the agg Ig chimera preparation is in an aggregate form.
Induction of EAE
6–8-wk-old mice were induced for EAE by subcutaneous injection in the footpads, and at the base of the limbs and tail with a 200 µl IFA/PBS (vol/vol) solution containing the autoantigen and 200 µg Mycobacterium tuberculosis H37Ra. 6 h later, the mice were given intravenous 5 x 109 inactivated Bordetella pertussis (Bioport). A second injection of B. pertussis was given after 48 h. Subsequently, the mice were scored daily for clinical signs of EAE as follows: 0, no clinical score; 1, loss of tail tone; 2, hindlimb weakness; 3, hindlimb paralysis; 4, forelimb paralysis; and 5, moribund or death. In some experiments, purified pertussis toxin (List Biological Laboratories, Inc.) was used instead of whole B. pertussis organism.
Treatment of EAE with Ig-PLP1
Mice induced for EAE with PLP1, PLP2, a mixture of PLP1 plus PLP2, or CNS homogenate began receiving treatment with Ig-PLP1 after loss of tail tone, which occurs regularly between days 6 and 8 after disease induction. Treatment injections were given intraperitoneally in PBS on days 9, 13, and 17.
Histopathology
Mice treated with agg Ig-PLP1 or agg Ig-W were killed at the peak of the initial phase of disease (day 28 after disease induction), and the brain and spinal cord were removed, fixed with formalin, and embedded in paraffin. Serial cross-sections (6 µm) from the cerebellum, cerebrum, and lumbar cord were cut and stained with hematoxylin and eosin. Perivascular clusters containing at least 20 mononuclear cells were counted as inflammatory foci.
T Cells
TCC-PLP1-1B10.
Adult SJL mice were immunized subcutaneously with 100 µg PLP1 peptide in CFA, and 10 d later the draining LNs were removed and the cells (5 x 106 cells/ml) were stimulated with PLP1 (15 µg/ml). After 5 d, the blasts were separated on a Histopaque gradient (Sigma-Aldrich), and then restimulated with peptide and fresh irradiated (3,000 rads) syngeneic APCs. 10 d later, the cells were washed, resuspended in media containing 10% T-Stim (Collaborative Research), and rested for 7 d. After three cycles of stimulation/resting, the cells were cloned by limiting dilution (1 cell/3 wells) and positives were subjected to a second round of limiting dilution cloning. Subsequently, one clone, designated TCC-PLP1-1B10, was selected for these studies.
Isolation of Macrophages, DCs, and B Cells
Macrophages.
Macrophages were obtained from the peritoneal cells of mice injected with thioglycollate broth as described previously 43. In brief, 2 ml of thioglycollate broth was injected intraperitoneally, and after 5 d the macrophages were removed by washing the peritoneal cavity with 8 ml of HBSS, 4 µM EDTA. Macrophage purity was 
93% as determined by FACS® analysis using antibody to F4/80 marker.
DCs.
DCs were purified from SJL/J spleen according to the standard collagenase/differential adherence method 44. Cell purity was 94% as determined by FACS® analysis using antibody to the 33D1 marker.
B Cells.
SJL/J splenocytes were panned on plates coated with rat anti–mouse (1 mg/ml) for 15 min at 25°C. Nonadherent cells were washed out with PBS. B cells were then dissociated from the plate by incubation with lidocaine HCl (0.8 mg/ml), followed by vigorous pipetting. Cell purity was 90% as determined by FACS® analysis for expression of B220 marker.
Proliferation Assays.
SJL/J splenocytes (10 x 105 cells/well/100 µl) were pulsed with graded amounts of antigen on round-bottomed 96-well plates for 4 h, pelleted, fixed with 1% paraformaldehyde for 15 min, washed, and transferred to a fresh 96-well plate. TCC-PLP1-1B10 cells (0.5 x 105 cells/well/100 µl) were then added and incubated for 3 d. Subsequently, 1 µCi [3H]thymidine was added per well, and the incubation continued for an additional 14.5 h. The cells were then harvested on glass fiber filters, and incorporated [3H]thymidine was counted using an Innotech β counter (Wohlen).
Cytokine Detection
ELISA.
ELISA was done according to BD PharMingen's standard protocol. The capture antibodies were rat anti–mouse IL-2, JES6-1A12; rat anti–mouse IL-4, 11B11; rat anti–mouse IFN-, R4-6A2; rat anti–mouse IL-10, JES5-2A5; and rat anti–mouse IL-5, TRFK5. The biotinylated anticytokine antibodies were rat anti–mouse IL-2, JES6-5H4; rat anti–mouse IL-4, BVD6-24G2; rat anti–mouse IFN-, XMG1.2; rat anti–mouse IL-10, JES5-16E3; and rat anti–mouse IL-5, TRFK4. ELISA for the detection of active TGF-β was preformed using the human TGF-β1 DuoSet kit (Genzyme) according to the manufacturer's instructions. Bound ligand was revealed using the TMB microwell peroxidase substrate system (Kirkegaard & Perry Laboratories). Assays were read on a SpectraMAX 340 counter (Molecular Devices). Graded amounts of recombinant mouse IL-2, IL-4, IFN-, IL-10, IL-5, and TGF-β were included in all experiments for construction of standard curves. The cytokine concentration in culture supernatants was estimated by extrapolation from the linear portion of the standard curve.
Enzyme-linked Immunospot.
Enzyme-linked immunospot (ELISPOT) assays were used to measure the cytokines produced by LN T cells upon stimulation with antigen as described 41. In brief, LN cells (5 x 105 cells/100 µl/well) and the antigen (100 µl/well) were incubated in HA-multiscreen plates (Millipore) coated with capture antibody for 24 h. Bound cytokines were revealed with peroxidase and anticytokine antibodies. The anticytokine antibody pairs used here were those described for the ELISA technique. Spots were counted under a dissecting microscope.
Stimulation of Cytokine Production by TCC-PLP1-1B10
Stimulation was performed with both irradiated and fixed APCs. In one case, SJL/J splenocytes were irradiated (3,000 rads) and plated (at 5 x 105 cells/well/50 µl) with graded concentrations of antigens (100 µl/well). After 1 h, TCC-PLP1-1B10 cells (0.5 x 105 cells/well/50 µl) were added and the culture was incubated for 24 h. For fixed APCs, SJL/J splenocytes (10 x 105 cells/well/100 µl) were pulsed with graded amounts of antigen, fixed with 1% paraformaldehyde, and incubated with TCC-PLP1-1B10 cells (0.5 x 105 cells/well/100 µl) for 24 h. Detection and quantification of cytokines were then assessed by ELISA from 100 µl of culture supernatant.
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Results
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Soluble Ig-PLP1 Reduces Paralytic Severity and Suppresses Clinical Relapses in Mice with Ongoing EAE.
Prevention and treatment of active autoimmune disease have been achieved by injection of adjuvant-free autoantigens or peptides 2425264546474849. However, repetitive injections of the autoantigens are required, and the disease rebounds when the supply of antigen is discontinued 48. One approach that may overcome these setbacks and modulate active disease is the delivery of the self-peptide on Igs. Igs have long half-lives and grant the peptides access to newly synthesized MHC molecules 3150, which could lead to efficient peptide loading onto MHC molecules 50 over an extended period of time. To test the Ig delivery system for treatment of active autoimmunity, SJL/J mice were induced for EAE with free PLP1 peptide, and when the clinical signs of disease became apparent the animals were given three injections of sol Ig-PLP1 in saline at 4-d intervals and assessed for reduction in disease severity. Control mice were given sol Ig-W, the parental Ig without any PLP1 peptide. The results illustrated in Fig. 1 show that mice treated with the sol Ig-W had an initial severe phase of paralysis with a mean maximal score of 3.7 ± 0.5 and displayed relapses throughout the 120-d period of examination. The mice treated with sol Ig-PLP1, however, had a reduced severity of paralysis at the initial phase of disease with a mean maximal score of 2.5 ± 0.3 (P < 0.005) and fully recovered by day 42. Mice treated with 10-fold excess of free PLP1 peptide had a slight reduction in the severity of paralysis at the initial phase of disease (mean maximal clinical score 3.0 ± 0.2), but never recovered and underwent relapses throughout the entire 120-d observation period (Fig. 1).
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) for 1 h, after which TCC-PLP1-1B10 cells (0.5 x 105 cells/well) were added and the incubation continued for an additional 24 h. Cytokine production was measured by ELISA from 100 µl of culture supernatant. Each point represents the mean of triplicate wells.
