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CD8⁺ T Regulatory Cells Use a Novel Genetic Program that Includes CD103 to Suppress Th1 Immunity in Eye-Derived Tolerance

¹From the Schepens Eye Research Institute, Department of Ophthalmology, Harvard Medical School, Boston, Massachusetts.

	Abstract

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PURPOSE. The peripheral tolerance that arises after injection of antigen into the anterior chamber (anterior chamber-associated immune deviation; ACAID) is associated in part with CD8⁺ T cells that suppress the expression of Th1 and Th2 immunity. The purpose of these studies was to determine the genes and molecules that are critical for CD8⁺ T regulatory cell (T reg) functions in ACAID.

METHODS. Ovalbumin (OVA)-specific CD8⁺ T cells from T-cell receptor (TCR) transgenic OT-1 mice acquire efferent regulatory properties similar to in vivo-generated CD8⁺ T regs after stimulation with OVA-pulsed TGF-ß2-treated APCs. Changes in the genetic program associated with acquisition of efferent regulatory function in OT-1 CD8⁺ T cells in vitro were determined by DNA microarray analyses and confirmed by RT-PCR analyses and biological assays.

RESULTS. T regulatory OT-1 T cells acquired a novel transcriptional pattern indicative of their function. Genes for molecules associated with TGF-ß function, resistance to TCR-triggered apoptosis, and localization of cells to antigen deposition in peripheral tissues were upregulated, and genes related to cytolytic function were downregulated. Further study showed that CD103, a cell-adhesion molecule that binds E-cadherin, was highly upregulated in in vivo-generated ACAID T regs and was necessary for their suppression of T-cell activation in vitro.

CONCLUSIONS. OT-1 CD8 T cells modulated in vitro by exposure to antigen-pulsed, TGF-ß2-treated APCs expressed genes related to immune suppression. Thus, the necessity for CD103 emerges in the efferent CD8⁺ T-cell regulatory mechanisms in eye-derived tolerance.

ACAID mice express two functionally distinct populations of regulatory T cells that suppress DH. ^{5 6 7 8 9 10} One population of regulatory T cells express CD4 and prevent the induction of immunity that leads to the generation of DH effectors (i.e., afferent regulators). Another population expresses CD8 and inhibits the expression of DH in vivo (i.e., efferent regulators). The molecular mechanisms by which these cells accomplish their regulatory functions are largely unknown. Unfortunately, the frequency of these putative regulator T cells in lymphoid organs of mice with ACAID has been too low for their collection and a detailed molecular analysis. To overcome this technical barrier, we turned to T-cell receptor (TCR) transgenic mice, which have lymphoid organs that contain a high frequency of T cells expressing T-cell receptors specific for defined peptides of ovalbumin (OVA) in the context of major histocompatibility complex (MHC) class I (K^b, OT-I) and class II (I-A^d, DO11.10). We recently reported that OVA-specific CD8⁺ OT-I T cells that are exposed in vitro to OVA-pulsed, TGF-ß2-pretreated APCs acquire the ability to suppress expression of DH when adoptively transferred into OVA-immune C57BL/6 mice.¹¹ Because this is a key property of CD8⁺ efferent T regulatory cells (T regs) in ACAID, study of in vitro-generated CD8⁺ OT-I T regs offered us the possibility of identifying relevant molecules and mechanisms of suppression.

Although TGF-ß is known to be involved in the DH-inhibitory activities of regulatory T cells in ACAID,^{11 12 13} there is little additional information that implicates other molecules that are involved in the generation of these T regulators or in enabling the regulators to mediate suppression. In this study, we used DNA microarray analysis to compare patterns of gene expression in regulatory OT-I CD8⁺ T cells generated in vitro with patterns from nonregulatory OT-I CD8⁺ T cells. Based on our results, we identified expected and, more importantly, unexpected genes with products that may influence the capacities of these T cells to perform their regulatory function in eye-derived tolerance. Several categories of differentially expressed genes were found that promote regulatory function, including genes that enable these T regs (1) to synthesize and secrete active TGF-ß, (2) to express signaling receptors for active TGF-ß, and (3) to resist antigen-triggered apoptosis. Several other categories of differentially expressed genes were found that prevent the generation of effector cells, including genes that rob the cells of their native capacity to lyse target cells and inhibit their secretion of proinflammatory Th1-type cytokines. The most strongly upregulated gene in CD8⁺ T regs generated in vitro encodes the cell surface integrin CD103. Using CD103 knockout (KO) mice, we found that expression of CD103 molecules by CD8⁺ T regs was absolutely essential to the capacity of these T regs to inhibit bystander OVA-primed T-cell activation in vitro and that expression of CD103 molecules by mice that received AC injections of OVA was essential in the induction of ACAID and in the generation of efferent CD8⁺ T regulators. Thus, CD103 expression is essential in both the inductive and effector stages of ACAID.

	Materials and Methods

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Mice
C57BL/6 (B6) mice, between 6 and 8 weeks of age, were purchased from Taconic Farms (Germantown, NY). Mice were used as a source of peritoneal exudate cells (PECs). BALB/cJ mice at 6 to 8 weeks of age were purchased from The Jackson Laboratory (Bar Harbor, ME). OT-I TCR transgenic mice (C57BL/6 background, obtained originally from The Jackson Laboratory) were maintained in our colony. T cells from OT-I mice recognize a peptide (residues 257-264) derived from OVA presented in the context of K^b. OT-I mice were used as the source of T cells. OVA-specific TCR transgenic T cells in OT-I mice were identified by surface flow cytometry for the expression of CD8 and Vß5. In general, 30% to 40% of CD3⁺ T cells in OT-I lymphoid cell suspensions expressed CD8 and TCR Vß5. CD103 (Itgae) gene knockout mice¹⁴ (backcrossed 10 generations to BALB/c) were provided by Gregg Hadley (University of Maryland Medical School, Baltimore, MD and maintained in our animal facility. Thrombospondin (TSP)-1 KO mice (C57BL/6 background)¹⁵ were provided by Jack Lawler (Beth Israel Deaconess Hospital, Boston, MA). All animals were treated according to NIH guidelines with approval by the Schepens Animal Care and Use Committee (ACUC) and the ARVO Statement for the Use of Animals in Ophthalmic and Vision Research.

Culture Medium
Serum-free medium was used for all cell cultures and was composed of RPMI 1640, 10 mM HEPES, 0.1 mM nonessential amino acids, 1 mM sodium pyruvate, 100 U/mL penicillin, and 100 µg/mL streptomycin, (all from BioWhittaker, Walkersville, MD), 1 x 10^–5 2-mercaptoethanol (ME; Sigma-Aldrich, St. Louis, MO), supplemented with 0.1% bovine serum albumin (Sigma-Aldrich), ITS⁺ culture supplement (1 µg/mL iron-free transferrin, 10 ng/mL linoleic acid, 0.3 ng/mL Na₂Se, and 0.2 µg/mL Fe(NO₃)₃; Collaborative Biochemical Products, Bedford, MA).

Regents: Antigens, Adjuvants, and Antibodies
OVA was purchased from Sigma-Aldrich and dissolved in Hanks’ balanced sale solution (HBSS) at a concentration of 25 mg/mL. Complete Freund’s adjuvant (CFA) containing heat-killed Mycobacterium tuberculosis strain H37 Ra was purchased from Difco Laboratories (Detroit, MI). Porcine TGF-ß2 and anti-pan TGF-ß neutralizing antibody were purchased from R&D Systems (Minneapolis, MN). The Abs used for flow cytometry analysis were: Fc block (anti-mouse Fcr II/III mAb, clone 2.4G2), phycoerythrin (PE)-conjugated anti-CD4 mAb (clone GK1.5), FITC- or PE-conjugated anti-CD8 mAb (clone 53-6.7), FITC-conjugated anti-TCR Vß5.1, 5.2 mAb (clone MR9-4), FITC-conjugated or purified anti-CD103 mAb (clone NM290), and purified or FITC- or PE-conjugated isotype controls (all purchased from BD-PharMingen; San Diego, CA). Purified anti-E-cadherin mAb (clone ECCD-2) was obtained from Zymed (South San Francisco, CA). FITC-conjugated anti-rat Ig polyclonal Ab was purchased from BD-PharMingen.

Preparation of Pure OT-I T Cells
Spleens were removed from OT-I mice and pressed through nylon mesh to produce a single cell suspension. Red blood cells were lysed with Tris-NH₄Cl. The remaining cells were washed three times with RPMI 1640 and passed through T-cell columns (Immulan; Biotecx Laboratory, Houston TX). After enrichment, the percentages of T cells were monitored by CD4 and CD8 staining and flow cytometric analyses. Together, CD4⁺ and CD8⁺ cells accounted for >90% of the cells in enriched suspensions.

Preparation of PECs Pretreated with TGF-ß2
PECs were harvested from normal C57BL/6 mice that received 2.5 mL of thioglycolate (Sigma-Aldrich) intraperitoneally 3 days earlier. In some experiments, PECs were harvested from TSP-1 KO mice. As described previously,^{11 16} the recovered cells were washed and resuspended, placed in 24-well culture plates (1 x 10⁶/well), and treated with or without 5 ng/mL porcine TGF-ß2 in serum-free medium at 37°C in an atmosphere of 5% CO₂. After overnight culture, plates were washed three times with culture medium to remove TGF-ß2 and nonadherent cells. Adherent cells were retained in the wells for use in all subsequent experiments. More than 92% of the adherent cells were F4/80⁺ and 99% of the cells were CD11b⁺.

Preparation of Regulatory T Cells and RNA Isolation
OT-I T cells (4 x 10⁵) were cultured in 24-well plates containing TGF-ß2-treated or untreated PECs, and 400 µg/mL OVA. In some experiments, OT-I T cells were cultured in the presence of pan anti-TGF-ß antibody for neutralization (1 µg/mL). After 72 hours, nonadherent OT-I T cells were harvested and purified by immunomagnetic depletion with anti-CD4, anti-CD11b, anti-B220, anti-DX5, and anti-Ter-119 (Miltenyi Biotec, Auburn, CA). The negatively selected cells were collected as CD8⁺ T cells. Cell purity, as examined by flow cytometry, showed that >95% were CD8⁺. Total RNA was extracted from these cells (RNA Stat-60 Kit; Tel-Test, Friendswood, TX and purified (RNeasy columns; Qiagen, Valencia, CA), according to the manufacturers’ instructions.

DNA Microarray Hybridization and Analysis
Preparation of the biotinylated RNA probe was performed as described (GeneChip Expression Analysis Manual; Affymetrix, Santa Clara, CA). In brief, 10 µg of total RNA was converted to double-stranded cDNA, by using oligo dT primers. Biotinylated RNA was generated with high-yield reagents (BioArray; Enzo Diagnostics, Farmingdale, NY), according to the manufacturers’ protocol. Samples were hybridized to murine genome U74Av2 chips (Affymetrix) and read, using a microarray chip scanner (GeneChip scanner; Affymetrix) and accompanying gene expression software, at the Bauer Center for Genomics Research at Harvard University.

Semiquantitative Reverse Transcription-Polymerase Chain Reaction
Real-Time PCR Assay.
A real-time PCR assay (SYBR Green; Applied Biosystems, Inc. [ABI] Foster City, CA) was used to determine the relative quantitative expression of selected genes. Sequences of the primers used for these genes are as follows : IL-12Rb1, forward (F), 5'-CAG TTC TGG GAA CAG GAC GGT ATC, reverse (R), 5'-GGG GTC GTC TTG GTC CAG TTG TA; granzyme B, F, 5'-GAC AGG TGG CAG GAT CTG AAT AAA, R, 5'-AGG AAG ATG TCA GTT GGG TTG TCA; CD103, F, 5'-GCC GTG ATC CAG ACT GAG TTT GAT, R, 5'-ATG GCT GAG GCG GTC TTA GTG ACT; RAR-, F-5'-GGG CAA GTA CAC TAC GAA CAA CAG; R, 5'-GGC GAA CTC CAC AGT CTT AAT GAT; MMP9, F, 5'-AAG GTG CTA GCT GGC CAG GTA CAG, R, 5'-GAA AAG GTT GGG GAT CCG TGT TTA; and CCR8, F, 5'-GGT GTT TGG GAC TGC GAT GTG TAA, R, 5'-GAT GGC ATA GAC AGC GTG GAC AAT. Amplification reactions were set up with mastermix (SurePRIME-&GO; QBiogene, Carlsbad, CA). Briefly, each reaction contained 1x mastermix, 100 µM each dNTP, 10 mM Tris-HCl (pH 8.3), 50 mM KCl, 2.5 mM MgCl₂, 0.02 U/µL DNA polymerase (SurePRIME; QBiogene), 200 nM forward and 200 nM reverse primers; 1:20,000 nucleic acid gel stain (SYBR green I dye; Molecular Probes Inc., Eugene, OR), and a 1:50 dilution of cDNA. The reactions were performed in 96-well plates (MicroAmp; ABI) capped with optical caps (MicroAmp; ABI) and amplified for 40 cycles (Prism 7900HT; ABI) with the standard PCR parameters (thermal profile: 50°C for 2 minutes; 1 cycle, 95°C for 15 minutes; 1 cycle, 52 to 55°C for 1 minute; 40 cycles, 72°C for 30 seconds). Dissociation curves were analyzed to ensure product specificity and amplicon identification based on Tm (melting temperature) values. The data generated from reactions was analyzed by plotting Rn (normalized) fluorescence signal versus the cycle number. An arbitrary threshold was set at the midpoint of the log Rn versus cycle number plot. The Ct values (thresholds) calculated from this plot were used to determine relative quantitation of gene expression by applying comparative Ct method (Ct). Ct was calculated by subtracting the Ct of the reference gene from the Ct (target gene). The reference gene was GAPDH. Comparative expression level was then calculated by converting Ct from a logarithmic to a linear value. Fold change, 2^–Ct.

Flow Cytometry
Cells in staining buffer (PBS, 1% fetal calf serum, 0.1% sodium azide) were incubated with blocking reagent (Fc blocker, 2 µg/10⁶ cells). All cells were incubated on ice for 20 to 30 minutes and washed twice before the next reagents were added. In some experiments with PECs, aliquots of 2 x 10⁵ PECs were incubated with ECCD-2 which recognizes the extracellular domains of E-cadherin in a buffer containing PBS, 1 mM CaCl₂, and 1% bovine serum albumin (PBS-Ca-BSA) for 30 minutes at 4°C.¹⁷ Cells were washed three times in PBS followed by incubation with FITC-conjugated goat anti-rat Ig antibody for E-cadherin in PBS-Ca-BSA for 30 minutes at 4°C. Flow cytometry analysis of E-cadherin was performed in the absence of the blocking agent of Fc receptors on PECs, because FITC-conjugated anti-Ig antibody yielded high-background fluorescence in cells treated with antibodies for Fc blocking. Negative controls included direct staining with secondary antibody in the absence of the first antibody. Stained cells were analyzed on a flow cytometer (EPICS XL; Beckman Coulter, Miami, FL).

Administration of Antigens
For intraocular injection, mice received an injection of OVA (50 µg/2 µL HBSS) into the AC of the right eye, as described previously.^{7 18} For conventional sensitization, 100 µL of an emulsion produced from a 1:1 mixture of OVA (2 mg/mL), and CFA was injected subcutaneously (SC) into the nape of the neck.

DH Assay
Induction and assessment of DH were performed as previously described.^{7 18} Seven days after immunization, mice received an intradermal inoculation of 200 µg/10 µL HBSS of OVA into the right ear pinna. In some experiments, OVA-pulsed PECs (prepared as described earlier, 5 x 10⁵/10 µL HBSS) were used as the antigen,¹⁹ even though background is higher when OVA-pulsed PECs were used than when antigen alone was used. There was swelling in both cases when primed T cells were added. Ear-swelling was expressed as follows: specific ear-swelling = (24 hours measurement of right ear – 0 hour measurement of right ear) – (24 hours measurement of left ear – 0 hour measurement of left ear) in micrometers. Ear-swelling responses of groups of mice are presented as the mean ± SEM. At 24 and 48 hours, ear-swelling was measured with a micrometer (Mitsutoyo, Paramus, NJ).

Preparation of T-Cell-Reconstituted Mice
CD103 KO mice were reconstituted with CD103-expressing T cells by a modification of an original method previously described.¹² In brief, unfractionated, purified T cells and purified CD8⁺ T cells were prepared from spleens and lymph nodes of normal BALB/c mice, as described earlier. Recipient CD103 KO mice received naïve unfractionated (3–4 x 10⁷/mouse) or purified CD8⁺ (5–8 x 10⁶/mouse) BALB/c T cells, intravenously (IV) 24 hours before use.

Adoptive Transfer of Regulatory T Cells
T cells were enriched from spleens of mice that had received an AC injection of OVA 7 days earlier. Some of the T cells were depleted of CD103⁺ cells by incubation with biotin anti-CD103 mAb (M290) for 20 minutes, washed and incubated with streptavidin microbeads for 15 minutes, and purified by column-negative selection in a magnetic field (Miltenyi Biotec). CD103-depleted T cells (enrichment was 99.9% for both CD4⁺CD103^– and CD8⁺CD103^– T cells) or undepleted T cells from mice with ACAID (10⁷) and T cells from naïve BALB/c mice (10⁷) were inoculated IV into BALB/c recipients that had been immunized 7 days earlier with OVA plus CFA. Immediately after IV infusion, recipients received an ear pinna challenge with OVA (200 µg/10 µL) or OVA-pulsed PECs (5 x 10⁵/10 µL HBSS). Positive control mice received only OVA/CFA immunization 7 days earlier. Negative controls were injected into the right ear pinna only, with OVA or OVA-pulsed PECs. Ear-swelling responses were measured 24 hours after intradermal injections.

Local Adoptive Transfer of Regulatory T Cells
To test for the efferent regulator cells of ACAID, a modified local adoptive transfer (LAT) assay was performed, as described elsewhere.^{7 19 20} OVA-primed T cells (responder cells) were generated in BALB/c mice by immunization with OVA and CFA, and 7 days later the primed T cells were dissociated from the draining lymph nodes by removing B cells and macrophages (Immulan; Biotecx Laboratory) column. Regulator cells were enriched on the column from spleen cells of mice that had received an AC injection with OVA 7 days earlier. Some of the regulator T cells were depleted of their CD103⁺ cells by incubation with biotin anti-CD103 mAb, washed and incubated with streptavidin microbeads for 15 minutes, and purified by column-negative selection in a magnetic field (Miltenyi Biotec). Stimulator cells were OVA-pulsed PECs as described earlier. Responder cells (5 x 10⁵), stimulator cells (5 x 10⁵), and regulator cells (5 x 10⁵) were mixed and resuspended in 10 µL HBSS for inoculation into the right ear pinna of naïve mice. Ear-swelling was measured at 24 and 48 hours. As a negative control, naïve T cells from unmanipulated mice were used as responder cells and regulator cells. Primed T cells were used as responder cells, and naïve T cells from unmanipulated mice were used as regulator cells for a positive control.

Statistical Analysis
Data were subjected to analysis by ANOVA and the Scheffé test. Means were considered to be significantly different when P 0.05.

	Results

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Comparison of Gene Expression Profiles in Regulatory and Nonregulatory CD8⁺ T Cells by DNA Microarray Analysis
To determine the molecules that might be involved in the generation of as well as the regulatory properties of the regulatory CD8⁺ T cells of ACAID that suppress expression of Th1 and Th2 effector cells, we compared RNA isolated from CD8⁺ OT-I T cells exposed to OVA-pulsed, TGF-ß2-treated APCs (T regs) or those exposed to OVA-pulsed, untreated APCs T effector cells (non-T regs). We used DNA microarrays that analyze 12,000 murine genes and expressed sequence tags (ESTs). Summaries of genes differentially expressed between the two cell populations are shown in Table 1 . The signal ratio (T regs/non-T regs) of each of the 12,000 genes was calculated. Genes with a threefold increase in this ratio were defined arbitrarily as upregulated in T regs, whereas those with a threefold decrease in this ratio were defined as downregulated. Using these criteria, 45 genes were found to be upregulated, and 16 genes were found to be downregulated in T regs compared with non-T regs.

Confirmation of Differentially Expressed Genes
To confirm that the observed differences in DNA microarray analysis correlated with differences in steady state levels of the corresponding mRNAs, the expression patterns of selected genes were determined by real-time RT-PCR, using primers specific for the genes shown in the Materials and Methods section. Levels of selected genes relative to that of a housekeeping gene (GAPDH) were compared between T reg- and non-T reg-derived RNA. This method confirmed the differential expression of each of the selected genes in the expected manner (Fig. 1) . mRNA expression of CD103, MMP-9, CCR8, and RAR- was upregulated in T regs, whereas expression of granzyme B and IL-12 receptor ß1 was downregulated. Furthermore, CD94 protein expression on T regs and non-T regs was examined by flow cytometry. Increased cell surface levels of CD94 were detectable on T regs compared with non-T regs (data not shown).

View larger version (31K): [in this window] [in a new window]   FIGURE 1. Confirmation of genes differentially expressed in T regs and non-T regs. Total RNA isolated from OT-I T cells stimulated, in vitro, with OVA-pulsed TGF-ß-treated or untreated APCs was subjected to real-time PCR analysis, with gene-specific primers for selected genes. GAPDH served as the reference gene. PCR products were analyzed by a nucleic acid gel stain assay. Relative expression of each gene was determined from the Ct. (A) PCR reaction curves for GAPDH and CD103. Reactions were performed in triplicate. The GAPDH curve represents six reactions (three per sample). (B) Change in expression (x-fold) of selected up- and downregulated genes in T regs compared with that in non-T regs.

View larger version (34K): [in this window] [in a new window]   FIGURE 2. Cell surface expression of CD103 on T regs and non-T regs. OT-I T cells stimulated with TGF-ß-treated or untreated APCs in the presence of OVA were harvested at 72-hour intervals. These cells were stained with FITC-conjugated anti-CD103 and PE-conjugated anti-CD8 mAbs for subsequent analysis by flow cytometry. The percentages represent the amount of CD103-expressing CD8+ cells detected within the lymphocyte gate. The experiments were repeated three times with similar results.

Development of Eye-Derived Tolerance in CD103 KO Mice
The lack of T reg activity in AC-inoculated CD103 mice suggests that eye-derived tolerance (ACAID) may not develop in CD103 KO mice. To examine this possibility, we treated groups of CD103 KO and WT mice with an AC injection of OVA. Seven days later, these mice were immunized SC with OVA and CFA, and 1 week later their ear pinnae were injected intradermally with a 200-µg OVA challenge. Ear-swelling responses were measured 24 hours after the challenge. As expected, groups of AC-injected WT mice displayed a reduced ear-swelling response compared with a positive control group, indicating suppressed OVA-specific DH (Fig. 3) . By contrast, a similarly treated group of CD103 KO mice displayed ear-swelling responses comparable to that in the positive control group. This lack of suppression of OVA-specific DH indicates absence of eye-derived tolerance. These results are consistent with our observations in in vitro experiments that indicate the absence of regulatory activity in splenic T cells of CD103 KO mice receiving an AC inoculation of OVA. Thus, both results suggest that expression of CD103 protein is necessary for the development of eye-derived tolerance (ACAID).

View larger version (13K): [in this window] [in a new window]   FIGURE 3. Role of CD103 in the capacity of in vivo-generated CD8+ T regs to suppress bystander T cells in vitro. Lymph node cells (responder cells) were harvested from BALB/c mice immunized 1 week earlier with OVA/CFA. Purified T cells (regulator cells) were harvested from the spleens of CD103 KO mice (or from WT control subjects) 1 week after AC injection of OVA (50 µg/2 µL). These regulator T cells (2.5 x 105/well) were added to cultures containing OVA-primed T cells (responder cells: 2.5 x 105/well) and OVA-pulsed PECs (stimulator cells: 105/well). In negative controls for regulator activity, T cells were harvested from spleens of mice that had not received an injection of OVA in the AC, added to cultures of responders and stimulators. Supernatants were collected from these cultures after 72 hours and analyzed for content of IFN- by ELISA. Each data point represents the mean ± SEM. *Significant difference (P 0.05); n.d., not detected. The experiments were repeated twice with similar results.

Positive control CD103 KO mice were immunized (SC) with OVA/CFA. We observed that AC injection of OVA into CD103 KO mice reconstituted with purified WT T cells led to suppression of OVA-specific DH (Fig. 4) . Similarly, CD103 KO mice that received highly enriched CD8⁺ T cells from WT donors also showed suppressed ear-swelling responses after immunization with OVA. Together, these findings indicate that successful development of peripheral tolerance and ACAID requires the presence of CD103-expressing CD8⁺ T cells. The CD103 molecule may be essential for cellular interactions during induction or expression of ACAID.

View larger version (12K): [in this window] [in a new window]   FIGURE 4. Development of eye-derived tolerance in CD103-deficient mice. Groups (five mice each) of wild BALB/c and CD103 KO mice received an AC injection in one eye of OVA (50 µg/2 µL). Seven days later, the mice were immunized SC with 100 µL of a 1:1 mixture of OVA (2 mg/mL) and CFA. Positive control subjects received only the SC immunization. One week later, OVA (200 µg/10 µL) was injected intradermally into the right ear pinna of the mice and the negative control subjects. Ear-swelling responses were measured 24 hours after challenge. Mean ± SEM ear-swelling responses are shown. *Mean response significantly lower than that in positive control subjects (P < 0.05). The experiments were repeated twice with similar results.

A suppressed ear-swelling response was detected in the recipients of replete T cells (Fig. 5) . Similar results were obtained when the ears of adoptive transfer recipients were challenged with OVA only (data not shown). By contrast, ear-swelling responses were not suppressed in recipients of CD103-depleted T cells. Next, we used an LAT, in which regulatory cells derived from the spleens of AC-inoculated BALB/c mice were mixed with OVA-primed T cells (responders) and OVA-pulsed PECs (stimulators) and injected into the ear pinnae of naïve syngeneic mice. Ear-swelling was measured at 24-hour intervals (Fig. 6) . Whereas replete T cells from AC-injected donors suppressed ear-swelling responses, CD103-depleted T cells from similar donors did not (Fig. 7) . Together, the results of our systemic transfer and LAT assays support the postulate that CD103 expression on T regs is necessary for the suppression of the efferent phase of the DH response.

View larger version (15K): [in this window] [in a new window]   FIGURE 5. Capacity of CD103-bearing T cells to reconstitute ACAID in CD103 KO mice. T cells were isolated from naïve BALB/c spleens and lymph nodes, using T-cell enrichment columns. Enriched T cell suspensions (3–4 x 107 cells/mouse), or CD8+ T cells purified from enriched T-cell suspensions (5–8 x 106 cells/mouse), were injected intravenously into groups of CD103 KO mice. After 24 hours, each recipient received an injection of OVA into the AC of one eye. Seven days later, these mice and the positive control subjects, were immunized SC with OVA plus CFA. One week later, the ear pinnae were injected with an OVA challenge, and ear-swelling responses were measured after 24 hours Mean ± SEM ear-swelling responses are presented (n = 5). *Mean response significantly lower than those in positive control subjects (P < 0.05).

View larger version (14K): [in this window] [in a new window]   FIGURE 6. Capacity of T cells depleted of CD103+ cells to transfer ACAID adoptively. Groups of BALB/c mice were immunized SC with OVA plus CFA. One week later, enriched T cells were obtained from spleens of BALB/c mice that had received an AC injection of OVA 1 week earlier. One group of immunized BALB/c mice received an intravenous infusion of these splenic T cells (1 x 107/mouse), whereas another group of immunized mice received an intravenous infusion of splenic T cells that had been depleted of CD103-bearing cells (1 x 107/mouse). An additional group of BALB/c mice received an intravenous infusion of naïve splenic T cells (1 x 107/mouse), and a further group of BALB/c mice was simply immunized with OVA plus CFA (positive control). One week after OVA+CFA immunization, and (where relevant) within 2 hours of the T-cell infusion, the pinnae of the mice were injected intradermally with an OVA-pulsed PEC challenge (5 x 105/10 µL HBSS). Negative control subjects received only the intrapinna OVA-pulsed PEC challenge. Ear-swelling responses were measured at 24 hours. Mean ± SEM ear-swelling responses are presented (n = 5). *Mean response significantly lower than that in positive control subjects (P < 0.05). The experiments were repeated twice with similar results.

View larger version (17K): [in this window] [in a new window]   FIGURE 7. Capacity of T cells depleted of CD103+ cells in the LAT assay. Regulator cells, OVA-primed responder T cells, and stimulator cells pulsed with OVA were prepared. Mixtures containing regulator cells (5 x 105/injection), responder cells (5 x 105/injection), and stimulator cells (5 x 105/injection) were injected (10 µL) into the ear pinnae of naïve BALB/c mice. As a negative control, naïve T cells from untreated mice were used as responder cells and regulator cells. Primed T cells were used as responder cells, and naïve T cells from untreated mice were used as regulator cells for a positive control. Ear-swelling was measured at 24 hours. Ear-swelling responses are presented as the mean ± SEM. *Mean response significantly lower than that in positive control subjects (P < 0.05; n = 5). The experiments were repeated twice with similar results.

	Discussion

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In this communication, we report the results of experiments designed to determine genes that are differentially expressed in OT-I T cells exposed to OVA-pulsed, TGF-ß2-treated or untreated APCs. We assigned priority of interest to those genes with the greatest change (threefold or greater) in expression compared with genes in OT-I T cells exposed to OVA-pulsed, TGF-ß-untreated APCs and with the known ability of the gene products to influence the following parameters of T cell function: (1) capacity to synthesize, activate, secrete, and respond to TGF-ß, (2) capacity to perform effector functions such as lysis of target cells and secretion of proinflammatory cytokines, (3) ability to localize via vascular migration to selected peripheral tissues and to adhere to bystander immune and parenchymal cells, and (4) resistance to TCR-triggered apoptosis.

TGF-ß is known to be a crucial immunomodulatory factor within the eye,^{44 45 46} in the induction of ACAID by eye-derived APCs,^{37 47} and in the suppression of DH by ACAID T regulators.^{9 11 12 13} It was therefore gratifying to find several strongly up- and downregulated genes (14–23-fold increases) with the potential to influence TGF-ß production and responsiveness in OT-I T cells converted into T regs in vitro (Table 1 , category I). Although dramatic changes in gene expression profiles by OT-I T cells exposed to OVA-pulsed, TGF-ß2-treated APCs correlated with gain of function (regulation), there were also changes in gene expression that correlated with loss of function (effector). Downregulated genes that correlated with loss of effector function by OT-I T cells (Table 1 , category II) help explain why OT-I T cells that convert into T regulators in vitro no longer display effector functions. Presumably, these functions would be inimical to the inhibition of inflammation, which is the goal of their suppressor activities. Knowing that the efferent CD8⁺ T regulators of ACAID originate in the spleen and then disseminate peripherally^{2 4 7} implies that molecular factors governing migration and adhesion are likely to be important to expression of their regulatory function (Table 1 , category III). Our laboratory reported a few years ago that DO11.10 T cells stimulated in vitro with OVA-pulsed, TGF-ß2-treated APCs are spared from the apoptosis that is the fate of most of the DO11.10 T cells stimulated in vitro with OVA-pulsed, TGF-ß-untreated APCs. We suspect that prevention of apoptosis after antigen stimulation⁴⁸ of regulatory T cells may contribute to their stability. Thus, because TGF-ß2-treated APCs promote ACAID by rescuing antigen-activated T cells from apoptosis, it is not a surprise that antiapoptotic genes such as IGF-1 (Table 1 , category IV) are highly upregulated in OT-I T regs.

Because CD103 (a cell-adhesion molecule that binds E-cadherin) was recently shown to be upregulated in natural CD4⁺ CD25⁺ T regulators, and because it was the most highly upregulated in OT-I T cells, we chose to study the role of CD103 in eye-derived tolerance. Our results indicate that expression of CD103 was upregulated on nearly all in vitro-generated OT-I T reg cells and that this expression was dependent, at least in part, on active TGF-ß, presumably produced by the APCs and the T cells themselves.¹⁶ Moreover, we found that CD103 expression was necessary in vivo for induction of ACAID, and this resulted in the generation of splenic T cells that suppressed T cell activation in vitro. Finally, CD8⁺ T regs from spleens of mice with ACAID proved to be unable to transfer suppression of DH to OVA-primed mice if the splenic cells were first depleted of CD103-bearing cells. Thus, CD103 expression by regulatory T cells appears to be absolutely essential for these cells to suppress antigen-specific Th1-type immunity in vivo—that is, eye derived tolerance (ACAID). There are at least two ways in which CD103 interactions with E-cadherin could be necessary to achieve this outcome. First, it can be expressed by APCs,^{49 50} and our own results indicate that PECs treated with OVA and TGF-ß2 upregulate their expression of E-cadherin (Keino H, unpublished observations, 2004). Thus, the conversion of naïve OT-I T cells into T regs on exposure to OVA-pulsed, TGF-ß-treated APCs may be facilitated by interactions between CD103 on the T cells and E-cadherin on the APC, thus implicating CD103 in the induction of CD8⁺ T regs in ACAID. Alternatively, local APCs participate in activating primed Th1 cells at the site of antigen deposition in DH reactions. Thus, E-cadherin expression by APCs within the stroma of OVA-injected ear pinnae may be necessary for efferent CD103⁺ CD8⁺ T regs to effect suppression of the inflammatory response. It is worth pointing out that CD103/E-cadherin-adhesive interactions are enhanced by signaling via the T cell receptor complex,⁵¹ which makes it possible that CD103 stabilizes and retains CD8⁺ T regulators at the site of antigen deposition.⁵² We are attracted to this possibility, because CD103-depleted ACAID T regulators failed to suppress DH expression in the LAT assay.

A second way in which CD103 interactions with E-cadherin could be important relates to the expression of E-cadherin on vascular endothelial cells.⁵³ CD103 binding to E-cadherin on vascular endothelial cells is an attractive possibility, because it has been shown that CD103 functions to promote the entry or retention of CD8⁺ cytotoxic T cells into the epithelial compartment of allografts.^{54 55} One way to interpret our finding that CD103-depleted T regulators from mice with ACAID failed to suppress DH in an adoptive transfer experiment is that CD103 expression is necessary for the cells to localize first to the local vessels then into the stroma at the site of antigen injection. This is supported by Huehn et al.⁵² who showed a correlation of suppressive capacity of CD103^– expressing T regs subsides with their preferential migration to inflamed sites. A very recent paper by Schwarz et al.⁵⁶ provides evidence that the reason regulatory T cells generated after ultraviolet B radiation of the skin fail to suppress the expression of hapten-specific contact hypersensitivity is that the regulatory cells lack the requisite adhesion molecules that enable T cells to migrate into the skin. Together, these considerations lead us to propose that upregulation of CD103 creates a novel functional program that promotes migration of efferent T regulators to the nonlymphoid sites where antigen is deposited—that is, ear pinnae where OVA is injected to elicit DH.

Our immediate goal is to identify key up- and downregulated genes in OT-I T regulatory cells and to determine whether these genes are essential in the generation of these cells or in their capacity to effect suppression. Our near-term goal is to use molecular strategies to interrupt expression or to induce selective expression of individual genes within these OT-I T cells and then within nontransgenic CD8⁺ T cells obtained from naïve or primed donors. Our ultimate goal is to use these strategies to create regulatory T cells at will with the capacity to suppress immunogenic inflammation in experimental animal model systems as a preamble to attempting these strategies in humans with immunopathogenic diseases and to promote allograft acceptance.

	Acknowledgements

 
The authors thank Jacqueline Doherty for expert management of the laboratory; Marie Ortega and Stephanie Carroll for excellent animal husbandry in the vivarium; Bruce Turpie for expert technical assistance, and Dom Sanethong for excellent administrative assistance.

	Footnotes

 
² Current address: Department of Ophthalmology, Tokyo Medical University, Tokyo, Japan.

³ Deceased March 15, 2004.

Supported in part by National Eye Institute Grants EY05678 and EY11983.

Submitted for publication December 10, 2004; revised August 24, 2005; accepted February 17, 2006.

Disclosure: H. Keino, None; S. Masli, None; S. Sasaki, None; J.W. Streilein, None; J. Stein-Streilein, None

The publication costs of this article were defrayed in part by page charge payment. This article must therefore be marked "advertisement" in accordance with 18 U.S.C. 1734 solely to indicate this fact.

Corresponding author: Joan Stein-Streilein, Schepens Eye Research Institute, 20 Staniford Street, Boston, MA, 02114; jstein{at}vision.eri.harvard.edu.

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Top Abstract Materials and Methods Results Discussion References

 

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