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Combined IL-15/IL-15R Immunotherapy Maximizes IL-15 Activity In Vivo¹

Department of Immunology, University of Connecticut Health Center, Farmington, CT 06030

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
IL-15 has substantial potential as an immunotherapeutic agent for augmenting immune responses. However, the activity of IL-15 is mediated by a unique mechanism in which the cytokine is transpresented by cell-bound high-affinity IL-15R to target cells expressing the IL-15R and the common -chain. Thus, the efficacy of administered IL-15 alone may be limited by the availability of free IL-15R. We now show that administration of soluble IL-15/IL-15R complexes greatly enhanced IL-15 half-life and bioavailability in vivo. Treatment of mice with this complex, but not with IL-15 alone, resulted in robust proliferation of memory CD8 T cells, NK cells, and NK T cells. The activity of the complex required IL-15R, but not IL-15R, expression by the responding cells and was IL-7-independent. Interestingly, IL-15/IL-15R immunotherapy also caused naive CD8 T cell activation and development into effector cells and long-term memory T cells. Lastly, complexed IL-15, as compared with IL-15 alone, dramatically reduced tumor burden in a model of B16 melanoma. These findings hold significant importance for the use of IL-15 as a potential adjuvant/therapeutic and inducer of homeostatic proliferation, without the necessity for prior immunodepletion.

	Introduction

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Interleukin-15 is a member of the four helix bundle family of cytokines, and IL-15 mRNA can be detected in a wide variety of tissues of both nonhemopoietic and hemopoietic lineages, but is not thought to be produced by T cells (1, 2). In contrast, under normal circumstances, IL-15 is difficult to detect at the protein level in vivo, perhaps due to short protein half-life and tight transcriptional and translational control (1, 3, 4, 5). IL-15 was initially discovered in an adult T cell leukemia cell line and a simian kidney epithelial cell line as a 14- to 16-kDa protein able to stimulate CTLL and peripheral blood T cell proliferation and induce peripheral blood mononuclear cell effector function in vitro (1, 2, 6). The analysis of mutant mice lacking IL-15 or the IL-15R (7, 8) reveals that IL-15 plays a multifaceted role in the development and control of the immune system. Both IL-15^–/– and IL-15R^–/– mice lack peripheral NK and NK T cell populations, certain intestinal intraepithelial lymphocyte subsets, a portion of the naive CD8 T cell compartment, and most memory phenotype CD8 T cells. In addition, Ag-specific memory CD8 T cells can develop in both types of knockout mice; however, the resulting memory CD8 T cell pool undergoes dramatic erosion over time (9, 10, 11).

The IL-15R consists of three polypeptides, the type-specific IL-15R, the IL-2/IL-15R, and the common -chain (C),⁴ which is shared by multiple cytokine receptors (12, 13). Unlike the IL-2R-chain, which exhibits low-affinity for IL-2 in the absence of the IL-2R and C, the IL-15R-chain alone binds IL-15 with high-affinity (K_d 10^–11 M). IL-15R was originally believed to form a membrane-bound heterotrimeric complex with the shared IL-2R and the C (13), akin to the structure of the IL-2R. Although this may be the case in certain situations, IL-15R is expressed by a wide variety of cell types but not necessarily in conjunction with IL-2R and C. For example, the IL-15R-chain does not coprecipitate with the IL-2/IL-15R/C in the presence of IL-15, unlike the IL-2R bound by IL-2 (14). Moreover, unlike the IL-2R-chain, the IL-15R-chain mediates signal transduction (15, 16, 17). The functional reasons for these apparent discrepancies between the IL-15 and IL-2 systems became apparent when the mechanism of action of IL-15 was shown to occur via transpresentation by IL-15R. Thus, IL-15 produced by one cell type is bound to IL-15R expressed by the same cell and presented to apposing cells expressing the IL-15R/C complex (18, 19, 20, 21, 22, 23, 24, 25). In vitro experiments demonstrate that the effect is direct, because IL-15 bound to IL-15R-Fc supports the survival of IL-15R^–/– memory CD8 T cells (20), and soluble receptor/cytokine complexes exhibit hyperagonist activity on cell lines in vitro (26, 27). Overall, the results suggest that the stoichiometry of IL-15 production and IL-15R expression may serve to regulate IL-15 activity in vivo.

Given the known effects of IL-15 on the immune system, IL-15 has become an immunotherapeutic target. Although IL-15 administration is used to bolster immune responses or augment immune system reconstitution, blockade of IL-15 activity can inhibit immune responses in certain cases. For example, administration of IL-15-blocking agents such as mutant IL-15/Fc proteins or a soluble form of the IL-15R has therapeutic potential in mouse models of arthritis and allograft survival (28, 29, 30). Conversely, overexpression of IL-15 or administration of IL-15 (as protein or expressed by plasmid DNA) augments protection of mice from a variety of infections and enhances vaccination (31, 32, 33, 34, 35, 36, 37, 38, 39). Furthermore, IL-15 therapy stimulates anti-HIV immunity and increases survival of CD4 and CD8 lymphocytes from HIV-infected patients in vitro (40, 41, 42, 43, 44, 45, 46). IL-15 can also accelerate immune reconstitution after bone marrow transplantation (47). Lastly, several groups have found that IL-15 therapy, in conjunction with chemotherapy, TLR agonists, or adoptive transfer of tumor-reactive CD8 T cells, results in increased survival or complete tumor regression in mouse tumor models, in contrast to each therapy alone (48, 49, 50). Thus, manipulation of IL-15 activity has potential as a therapeutic modality in a number of clinical situations.

Considering these findings and the transpresentation model, we hypothesized that IL-15 action in vivo could be augmented by the administration of soluble IL (sIL)-15R and IL-15 complexes. Our results show that forced transpresentation of IL-15 in vivo profoundly enhanced IL-15 activity and drove proliferation and differentiation of IL-15-responsive immune cells. Importantly, complexed IL-15, in contrast to IL-15 alone, reduced B16 tumor burden in a systemic tumor model. These findings hold important ramifications for the future of IL-15-targeted therapy.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Mice and cells

C57BL/6-Ly 5.1 mice were purchased from The Jackson Laboratory. C57BL/6-Ly 5.2 mice were purchased from Charles River Laboratories. The OT-I mouse line was provided by Dr. W. R. Heath (Walter and Eliza Hall Institute, Parkville, Australia) and Dr. F. Carbone (University of Melbourne, Parkville, Australia) and was maintained as a C57BL/6-Ly5.2 line on a RAG^–/– background. IL-15R^–/– mice (8) were provided by Dr. A. Ma (University of California San Francisco, CA). Spleen cells from IL-2R^–/– mice were provided by Dr. M. Farrar (University of Minnesota, Minneapolis, Minnesota). IL-7^–/– mice (51) were originally obtained from DNAX Research Institute and were maintained on a C57BL/6 background. All procedures were conducted under National Institutes of Health guidelines and were approved by the institutional animal care committee. Memory CD8 T cells were generated by adoptive transfer of CD45.1 OT-I-RAG^–/– cells to CD45.2 C57BL/6 (B6) mice that were then infected with vesicular stomatitis virus (VSV)-OVA. Alternatively, to produce VSV nucleoprotein-specific memory cells, CD45.1 B6 mice were infected i.v. with 1 x 10⁵ PFU VSV-Indiana. In either case, at least 60 days after infection, enriched CD8 T cells containing OT-I or VSV-specific memory cells were used in adoptive transfer studies.

CFSE labeling of cells and adoptive transfer

Single-cell suspensions were created in HBSS by homogenizing spleens or lymph nodes using frosted glass slides. RBC were lysed, and splenocytes were filtered through Nitex. Cells were incubated for 10 min at 37°C with CFSE (2 µM; Molecular Probes), the reaction was squelched with HBSS with 5% FCS (52), and the cells were washed twice. CFSE-labeled cells were resuspended in PBS and injected i.v. into congenic mice.

IL-15 treatment

Human IL-15 was generously provided by Amgen. Recombinant mouse IL-15R-Fc chimeric molecule was purchased from R&D Systems. Human IL (hIL)-15 and recombinant murine (rm)IL-15R-Fc, both suspended in PBS, were mixed and incubated for 30 min at 37°C. Each mouse, unless specifically noted, received 2.5 µg of IL-15 either alone or precomplexed with 15 µg of rmIL-15R-Fc in 200 µl of PBS i.p.

Flow cytometric analysis

Cells were isolated at the indicated times and analyzed for the presence of donor cells using CD45 allele status and their expression of surface markers and CFSE intensity. The percentage of cells of the original population that had divided (the "responding" population, R) was calculated as described previously (53). VSV nucleoprotein-specific donor cells were detected using H-2K^b tetramers prepared as described previously (54, 55). For staining, lymphocytes were suspended in PBS/0.2% BSA/0.1% NaN₃ (FACS buffer) at a concentration of 3–15 x 10⁶/200 µl. For tetramer staining, cells were incubated at room temperature for 1 h with tetramer-APC plus the appropriate dilution of anti-CD8 PerCP. Cells were washed with FACS buffer and stained with Abs specific for either CD44, CD122, NK1.1, CD3, or CD4 (all mAbs from BD Pharmingen) at 4°C for 20 min, washed, and then fixed in PBS with 3% paraformaldehyde. Relative fluorescence intensities were measured with a FACSCalibur (BD Biosciences). Data were analyzed using FlowJo Software (Tree Star).

ELISA for detection of IL-15

Anti-hIL-15 (MAB647; R&D Systems) in PBS (5 µg/ml, 100 µl/well) was added to 96-well high binding plates (3590; Corning) at 37°C for 1 h. The plates were washed and then blocked using PBS/1% BSA/0.2% Tween 20 (200 µl/well) for 1 h at 37°C. Dilutions of serum (in blocking buffer) were incubated for 1 h at 37°C, followed by washing with PBS/0.05% Tween 20 and the addition of biotinylated anti-hIL-15 Ab (BAM247; R&D Systems; 0.2 µg/ml, 100 µl/well) for 1 h at 37°C. Finally, Avidin-HRP (BD Pharmingen) (1/1000 dilution) was added for 1 h at 37°C. After washing, TMB substrate (34021; Pierce) was added, and 1 M phosphoric acid was used to stop the reaction. ODs at 450–570 nm were measured using a microplate reader (Bio-Rad; model 680). The serum half-life of IL-15 was calculated using the medical calculator provided by Cornell University per the given instructions (http://www-users.med.cornell.edu/spon/picu/calc/halfcalc.htm).

In vivo cytotoxicity assay

This assay was performed essentially as described previously (56). Normal spleen cells were labeled to low (0.25 µm) or high (2.5 µm) CFSE levels, and CFSE^low cells were incubated with 1 µg/ml SIINFEKL peptide for 45 min at 37°C. Equal numbers (10 x 10⁶) of each population were mixed and injected i.v. into OT-I-transferred mice that were either untreated or treated with IL-15/IL-15R or were infected with 1 x 10⁵ PFU of VSV-expressing chicken OVA (57) 4 days earlier. Four hours later, spleen cells were analyzed for the presence of CFSE^high and CFSE^low populations. Percentage of lysis = [1 – (ratio unprimed:ratio primed)] x 100. Ratio = percentage of CFSE^low:percentage of CFSE^high.

Intracellular detection of IFN-

Lymphocytes were isolated from the spleen and cultured for 5 h with 1 µg/ml Golgistop (BD Pharmingen), with or without 1 µg/ml of the OVA-derived peptide SIINFEKL. After culture, cells were stained for surface molecules then fixed, and cell membranes were permeabilized in Cytofix/Cytoperm solution (BD Pharmingen) and stained with anti-IFN- PE or control rat IgG1 PE. Cells were then washed, and the fluorescence intensity was measured on a FACSCalibur (BD Biosciences).

Tumor challenge and treatment

B16-F1 cells were maintained in Advanced DMEM (Invitrogen Life Technologies) supplemented with 10% FCS/100 U/ml penicillin/100 µg/ml streptomycin/430 µg/ml Glut-Max. Cells were harvested using 0.25% trypsin/EDTA (Invitrogen Life Technologies) when 50–80% confluent, and 1 x 10⁵ cells (in PBS) were injected via the lateral tail vein. On day 1 and day 10 post-B16 injection, mice began receiving treatment i.p.: PBS, IL-15 (2.5 µg), or IL-15/R-Fc (2.5 µg/15 µg). Mice were sacrificed on day 21. For tumor examination, mice were randomized and scored in a blinded fashion.

	Results

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Coadministration of IL-15 and IL-15R drives CD8 memory T cell and NK cell proliferation in vivo

To determine whether precomplexed cytokine and soluble receptor would augment IL-15 activity in vivo, IL-15 and IL-15R-Fc (IL-15R) were incubated at a 1:1 molar ratio before injection. At this ratio, because rmIL-15R-Fc is dimeric, one binding site per rmIL-15R-Fc is theoretically filled. Increasing by 2-fold the amount of IL-15 added to the receptor did not increase activity (data not shown). Human and mouse IL-15 provoked similar responses in our model, although hIL-15 exhibited somewhat higher activity than mouse IL-15 (data not shown). To measure IL-15-mediated activity in vivo, we used an adoptive transfer model to gauge the effect of IL-15 on the proliferation of CD8 T cells. CD45.1 CFSE-labeled CD8-enriched splenocytes were transferred to normal CD45.2 mice that were then treated with PBS, IL-15 alone (2.5 µg), IL-15R (15 µg), or a mixture of IL-15 (2.5 µg) and IL-15R (15 µg). Four days after treatment with IL-15 alone, 8.4% of the donor CD8 T cell population had divided (Fig. 1A, top panels), in agreement with our previous results (23). In dramatic contrast, the coadministration of the same amount of IL-15 bound to IL-15R resulted in the proliferation of 64.3% of the donor CD8 T cells (Fig. 1A, top panels). Furthermore, whereas the majority of CD8 T cells responding to IL-15 alone divided once, the cells responding to combination treatment underwent 5–7 divisions, resulting in a substantial increase in donor cell numbers (data not shown). Importantly, administration of IL-15R alone did not induce proliferation of CD8 T cells (Fig. 1A, top panels). The bulk of the dividing cells expressed high levels of CD44, suggesting that the responding cells were primarily memory CD8 T cells or that CD44 had been up-regulated (Fig. 1A, bottom panels). To test the action of combined therapy on bona-fide memory CD8 T cells, we adoptively transferred CFSE-labeled nucleoprotein-specific memory CD8 T cells that had been generated by infection with VSV. Similar to the above results, Ag-specific memory CD8 T cells responding to combined IL-15/IL-15R treatment proliferated to a much greater extent than those provided IL-15 alone (Fig. 1B) and increased in number (data not shown).

View larger version (29K): [in this window] [in a new window]   FIGURE 1. Coadministration of IL-15 and IL-15R-Fc enhances CD8 T cell proliferative response to exogenous IL-15. A, On day –1, mice received 1.5 x 107 congenic CFSE-labeled, CD8-enriched lymphocytes i.v. and were treated i.p. on day 0 with PBS, IL-15 (2.5 µg), IL-15R-Fc (15 µg), or IL-15R-Fc (15 µg) with IL-15 (2.5 µg). CD8+ splenocytes were analyzed on day 4 by flow cytometry for CFSE fluorescence and CD45.1 expression (top panels), or CD45.1+CD8+ cells were analyzed for CFSE fluorescence and CD44 expression (bottom panels) (n = 4). Data are representative of three similar experiments. B, On day –1, mice received CFSE-labeled CD8 T cell-enriched splenocytes containing 6.5 x 105 tetramer+ VSV nucleoprotein-specific memory CD8 T cells and were treated on day 0 with PBS, IL-15 (2.5 µg), or IL-15R-Fc (15 µg) with IL-15 (2.5 µg). Donor tetramer+ splenocytes were analyzed by flow cytometry on day 4 for CFSE fluorescence. R = the percentage of responding cells.

View larger version (18K): [in this window] [in a new window]   FIGURE 2. NK and NK T cells are highly responsive to IL-15/IL-15R-Fc. On day –1, mice received 1.5 x 107 congenic CFSE-labeled lymphocytes i.v. and on day 0 were treated with PBS, IL-15 (2.5 µg), or IL-15R-Fc (15 µg) with IL-15 (2.5 µg). Spleen cells were analyzed by flow cytometry on day 4 (n = 3). Samples were gated on the indicated donor population (NK = NK1.1+CD3–; NK T cell = NK1.1+CD3+; CD4 = CD4+ lymphocytes). Data are representative of three similar experiments.

Complexed IL-15/IL-15R greatly enhances IL-15 activity in vivo

We next examined the early kinetics of the CD8 T cell-proliferative response to the coadministration of IL-15R with IL-15. CFSE dilution was negligible 1 day after treatment, but by day 2 33% of the donor CD8 T cell population had divided (Fig. 3). By day 3, 66% of donor CD8 T cells had divided with many cells in divisions 5–6, whereas 74% had divided by day 4 with some cells in their 7th round of division. By day 20 after treatment, many of the cells had completely diluted their CFSE, although cells at intermediate stages of division remained. These results showed that the maximum effect of a single dose of IL-15/IL-15R was achieved by 4 days posttreatment.

View larger version (14K): [in this window] [in a new window]   FIGURE 3. CD8 T cells rapidly divide in response to IL-15/IL-15R-Fc treatment. On day –1, mice received 1 x 107 congenic CFSE-labeled, CD8-enriched lymphocytes i.v. and were treated with PBS or IL-15R-Fc (15 µg) with IL-15 (2.5 µg) on day 0. Peripheral blood lymphocytes were analyzed by flow cytometry on days 1–4 and day 20. Samples shown are gated on live donor CD8 T cells. Data are representative of two similar experiments. R = the percentage of responding cells.

View larger version (20K): [in this window] [in a new window]   FIGURE 4. Coadministration of IL-15R-Fc with IL-15 greatly enhances IL-15 potency. A, On day –1, mice received 1.5 x 106 congenic CFSE-labeled, CD8-enriched lymphocytes i.v. and on day 0 received either PBS (data not shown), IL-15 (5 µg), or varying doses of IL-15/IL-15R-Fc (0.5 µg + 3 µg) i.p. (n = 3). Data are representative of two similar experiments. B and C, On day –1, each mouse received 4.5 x 106 congenic CFSE-labeled, CD8-enriched lymphocytes i.v. and on day 0 received either PBS (data not shown), IL-15 (0.5 µg) + IL-15R-Fc (3 µg), or IL-15 (37.5 µg) i.p. CD8+ splenocytes were analyzed on day 4 for CFSE dilution by flow cytometry (n = 3). Data are representative of two similar experiments.

Complexing IL-15 to IL-15R greatly increases half-life and serum levels of IL-15

The effect seen by complexing IL-15 and soluble receptor may operate in part by increasing the half-life and bioavailability of exogenously administered IL-15. To test this possibility, we developed an ELISA to detect hIL-15 in mouse serum. Preliminary experiments indicated that complexing hIL-15 with IL-15R did not interfere with Ab binding (data not shown). Mice were treated i.p. with hIL-15 (2.5 µg) alone or a mixture of hIL-15 (2.5 µg) and IL-15R (15 µg), and serum was obtained at various times after treatment, as well as just before treatment. We noted that the half-life of hIL-15 alone was 1 h, whereas when complexed to the receptor, IL-15 half-life was extended to 20 h (Fig. 5A). With regard to maximum serum levels obtained, IL-15 alone peaked at a concentration of 70 ng/ml 30 min after administration, whereas complexed IL-15 peaked 2 h after administration at a concentration of 600 ng/ml. Similar results were noted with administration via the i.v. route, indicating that the differences noted were not due to differences in absorption from the peritoneal cavity (data not shown). Using this assay, we also determined that the presence or absence of endogenous IL-15R did not affect the serum levels or kinetics of administered hIL-15 (data not shown), suggesting that IL-15 binding to endogenous IL-15R did not contribute significantly to the short half-life of IL-15. The serum levels of IL-15 when administered as a receptor complex also correlated with functional activity as measured by CFSE dilution of transferred cells (Fig. 5B). By 24 h after administration, activity had declined substantially and by day 4 after treatment, no activity was detected by this assay.

View larger version (16K): [in this window] [in a new window]   FIGURE 5. Complexing IL-15 with IL-15R-Fc increases half-life and bioavailability of exogenous IL-15 in the serum. A, Mice were injected with hIL-15 (2.5 µg) i.p. with or without precomplexed IL-15R-Fc (15 µg). Mice were bled over time (0.25, 0.5, 1, 2, 4, 7, 16, 21, 44, 79, and 110 h after treatment), and hIL-15 presence in mouse serum was monitored using a hIL-15-specific ELISA. Data are representative of two similar experiments with three mice per group. B, Mice were injected with either PBS on day 0 or IL-15 (2.5 µg) and IL-15R-Fc (15 µg) complex on day –4, day –1, or day 0 i.p. On day 0, all mice received 1 x 106 CFSE-labeled CD45.1 CD8 T cells i.v. Splenocytes were examined on day 4 posttransfer for CFSE dilution. Experiment is representative of two similar experiments with three mice each.

Receptor-complexed IL-15 functions through IL-15R

The effects of complexed IL-15/IL-15R could either be mediated by direct or indirect effects on the responding cell types. If direct, then it might be expected that the target cells would be required to express IL-15R component(s). To test this, we transferred CFSE-labeled CD45.1 IL-15R^–/– CD8 T cells into CD45.2 IL-15R^–/– hosts and treated the mice with either IL-15 or complexed IL-15/IL-15R. IL-15 alone could not be transpresented in the absence of endogenous IL-15R, and did not induce proliferation (Fig. 6A) (23). In contrast, donor CD8 T cells from IL-15/rmIL-15R-treated mice proliferated extensively. Furthermore, the IL-15R^–/– donor cells, which primarily consisted of naive phenotype CD8 T cells, progressively increased their expression of CD44 and CD122 with division (Fig. 6A).

View larger version (19K): [in this window] [in a new window]   FIGURE 6. Activity of complexed IL-15/IL-15R-Fc requires IL-2R but not IL-15R expression by responding cells. A, On day –1, CD45.2 IL-15R–/– mice received 2 x 106 CD45.1 CFSE-labeled, CD8-enriched IL-15R–/– lymphocytes i.v. and on day 0 were treated with PBS, IL-15 (2.5 µg), or IL-15R-Fc (15 µg) with IL-15 (2.5 µg) i.p. On day 4, CD8+ donor splenocytes were analyzed for CFSE fluorescence and CD44 and CD122 expression (n = 3). Data are representative of two similar experiments. B, On day –1, CD45.1 B6 mice received 1.7 x 107 CD45.2 CFSE-labeled wild-type or IL-2/IL-15R–/– splenocytes i.v. and on day 0 were treated with either PBS or IL-15R-Fc (15 µg) with IL-15 (2.5 µg) i.p. CD45.2 CD8+ donor splenocytes were analyzed for CFSE dilution on day 4 by flow cytometry.

Proliferation induced by forced IL-15 transpresentation does not require IL-7

Because IL-7 is essential for the homeostatic proliferation of CD8 T cells in immunodeficient hosts (64), we wished to test the role of IL-7 in proliferation induced by receptor-bound IL-15. Congenic CFSE-labeled CD8 T cells were transferred to control or IL-7^–/– mice, and combined IL-15/IL-15R was administered. The absence of IL-7 had no effect on CD8 T cell proliferation in response to IL-15 with IL-15R (Fig. 7), indicating that IL-7 was not involved in IL-15-mediated proliferation in our system.

View larger version (15K): [in this window] [in a new window]   FIGURE 7. IL-15/IL-15R-Fc-driven proliferation of CD8 T cells does not require host IL-7 expression. On day –1, CD45.1 IL-7+/– or IL-7–/– mice received 6 x 106 CD45.2 B6 CFSE-labeled CD8-enriched lymphocytes. On day 0, mice received PBS or IL-15R-Fc (15 µg) with IL-15 (2.5 µg) i.p. On day 4, CD45.2 CD8+ splenocytes were examined for CFSE dilution (n = 3). Data are representative of two similar experiments.

IL-15/IL-15R immunotherapy induces naive T cell activation and effector function

In previous experiments, we noted that CD44^low polyclonal CD8 T cells as well as naive TCR transgenic T cells responded to IL-15 when coadministered with IL-15R (Figs. 1 and 6). Considering that under homeostatic conditions CD8 memory T cells exhibit much greater responsiveness to IL-15 than do naive CD8 T cells, we wished to directly compare the responsiveness of these two subsets to complexed IL-15/rmIL-15R. To do so, CFSE-labeled memory OT-I and naive OT-I CD8 T cells were adoptively transferred into the same congenic C57BL/6 hosts, and proliferation was analyzed 4 days after treatment with IL-15/IL-15R. Surprisingly, naive OT-I CD8 T cells proliferated almost as well as memory OT-I CD8 T cells (Fig. 8A). The naive OT-I cells also expanded 10-fold in response to the complex as compared with controls and up-regulated CD44 (Fig. 8B). Similar results were seen with FACS-purified CD44^low OT-I cells (data not shown); thus, any contaminating CD44^high naive OT-I cells cannot account for the naive CD8 T cell proliferation seen. We also examined the activation status of naive OT-I cells 1 day after treatment by measuring the expression level of CD69, which is up-regulated after T cell activation, and IL-7R (CD127), which is down-regulated after T cell activation (64). Interestingly, CD69 was increased and CD127 was decreased on OT-I cells 1 day after treatment with IL-15/IL-15R (Fig. 8C).

View larger version (18K): [in this window] [in a new window]   FIGURE 8. Naive CD8 T cells acquire effector phenotype in response to IL-15/IL-15R-Fc treatment. A, On day –1, CD45.2 B6 mice received a mixture of CD45.1/2 naive and CD45.1 memory OT-I-RAG–/– cells and were treated with either PBS or rmIL-15R-Fc (15 µg) with IL-15 (2.5 µg) on day 0. Four days later, splenocytes were examined for CFSE intensity of each CD8 + donor population (n = 2). B, On day –1, CD45.2 B6 mice received 3 x 106 CD45.1 OT-I RAG–/– cells i.v. and were treated with either PBS or rmIL-15R-Fc (15 µg) with IL-15 (2.5 µg) on day 0. The donor OT-I population was examined for frequency and CD44 expression by flow cytometry (n = 3). Percentage shown is for percentage of OT-I per total splenocytes and is taken from one mouse representative of each population. Data are representative of two similar experiments. C, Mice received 6 x 106 naive CD45.1 OT-I-RAG–/– cells i.v. and either received PBS or IL-15 (2.5 µg) and IL-15R-Fc (15 µg) i.p. on day 0. Mice were sacrificed, and the expression of CD69 and CD127 by transferred OT-I population was examined by flow cytometry (n = 3).

View larger version (21K): [in this window] [in a new window]   FIGURE 9. Receptor-complexed IL-15 induces effector function in naive CD8 T cells. A, On day –1, mice received 2.5 x 106 naive OT-I-RAG–/– cells and were treated with PBS, IL-15 (2.5 µg), IL-15R-Fc (15 µg) with IL-15 (2.5 µg) i.p., or 1 x 105 PFU of VSV-OVA i.v. On day 4 posttreatment, each mouse received a mixture of CD45.1/2 CFSE-labeled (1.5 µM) nonpeptide-pulsed splenocytes and CFSE-labeled (0.0015 µM) SIINFEKL peptide-pulsed splenocytes. Four hours later, splenocytes were analyzed for the presence of the CFSE-labeled target populations (data shown) (n = 4). Data are representative of two experiments. Percentage shown is percentage of Ag-specific killing per group ± SD. B, On day –1, CD45.2 mice received 2 x 106 naive CD45.1 OT-I-RAG–/– cells and on day 0 were treated with PBS, IL-15 (2.5 µg), IL-15R-Fc (15 µg), and IL-15 (2.5 µg), or 1 x 105 PFU VSV-OVA i.v. On day 4, splenocytes were incubated in vitro with or without SIINFEKL peptide for 5 h, and the production of IFN- OT-I (gated on CD45.1 donor cells) was analyzed by intracellular staining (n = 3). Data are representative of two similar experiments. Percentage shown is percentage of the gated OT-I donor population staining for intracellular IFN-.

Treatment of naive T cells with complexed IL-15/IL-15R generates memory CD8 T cells

Although naive T cells developed into effector cells in response to transpresented IL-15, it remained to be seen whether this was a transient effect or resulted in memory T cell development. Therefore, we analyzed the number and phenotype of OT-I T cells 44 days after naive OT-I T cell transfer and IL-15/IL-15R treatment. At this time point, a 5-fold higher percentage of OT-I cells was present following IL-15/IL-15R administration as compared with untreated mice, as well as greater OT-I numbers (Fig. 10, top panels; data not shown). Moreover, nearly all of these cells expressed high levels of CD44 and CD122 (Fig. 10, middle and bottom panels). We have also noted that memory OT-I cells induced by receptor-complexed IL-15 were able to produce IFN- upon peptide restimulation to a similar extent as bona-fide Ag-experienced OT-I cells (data not shown). Thus, in the absence of Ag, IL-15/IL-15R treatment was able to induce the development of memory CD8 T cells.

View larger version (21K): [in this window] [in a new window]   FIGURE 10. IL-15/IL-15R-Fc treatment generates memory cells from naive CD8 T cells. On day –1, B6 mice received 6 x 106 CD45.1 CFSE-labeled naive OT-I-RAG–/– cells and on day 0 were treated i.p. with PBS or IL-15 (2.5 µg) and IL-15R-Fc (15 µg). Forty-four days later, splenocytes were analyzed for percentage of donor OT-I CD8 T cells (top panels) and OT-I expression of CD44 and CD122 (middle and bottom panels). Percentages shown are from individual mice (n = 2). Data are representative of two experiments.

IL-15/IL-15R acts as an antitumor immunotherapeutic agent

Because IL-15/IL-15R leads to the expansion and activation of CD8 T cells and NK cells, two populations known to be involved in tumor surveillance, we wished to compare the ability of IL-15 vs IL-15/IL-15R in enhancing tumor immunity. To this end, we injected 1 x 10⁵ B16-F₁ melanoma cells i.v. on day 0 and treated mice with either PBS, IL-15 (2.5 µg), or IL-15/IL-15R (2.5 µg/15 µg) i.p. on day 1 and day 10. This tumor protocol leads to the establishment of tumors in the lung and liver. Mice were examined and scored for the presence of tumor nodules. We found that 90% of the PBS and IL-15-treated mice (compiled from two separate experiments) were tumor positive (Fig. 11) and exhibited a similar tumor burden between groups (multiple tumors >5 mm in diameter), whereas only one of the IL-15/IL-15R-treated mice was tumor positive and contained only a single 2-mm lung tumor. These results indicated a potential therapeutic value of combining IL-15 and IL-15R to prevent tumor engraftment.

View larger version (9K): [in this window] [in a new window]   FIGURE 11. IL-15/IL-15R complex is an effective antitumor immunotherapy agent. Mice were given 1 x 105 B16-F1 cells i.v. (day 0), followed by two doses of either PBS, IL-15 (2.5 µg), or IL-15 (2.5 µg) with IL-15R-Fc (15 µg) i.p. on day 1 and day 10. On day 21 mice were sacrificed, and tumor (black nodules) burden in lung and liver were noted. Data shown are the compilation of two separate experiments (n = 10).

	Discussion

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Noteworthy, the level of proliferation obtained by treatment with the complex could not be achieved by high doses of IL-15 alone. Because the same cell producing IL-15 may also transpresent the cytokine (23, 24, 25, 75), the availability of free IL-15R may be limited thus restricting the effectiveness of treating with IL-15 alone. The fact that the serum half-life or level of exogenous IL-15 was not significantly altered by the presence or absence of endogenous IL-15R (data not shown) further supports the theory that free IL-15R is limiting in vivo. Our results demonstrated that IL-15/IL-15R recapitulated IL-15 responsiveness in an IL-15R^–/– host. This was illustrated by the proliferation of IL-15R^–/– donor CD8 T cells in an IL-15R^–/– host, as well as the induction of memory phenotype CD8 T cells and NK cells (data not shown), that are normally lacking in IL-15R^–/– mice. This effect highlighted the potential of receptor-complexed IL-15 to reestablish the cytolytic arm of the immune system during states of lymphopenia. In addition, our studies showed that the short half-life of IL-15 was extended 20-fold when complexed to the receptor. Equally impressive was the notable increase in the serum availability of IL-15 when administered bound to IL-15R. Indeed, when complex was delivered i.v., nearly all of the administered IL-15 was accounted for in the serum some 15 min later, whereas when uncomplexed, only 4% of the IL-15 dose could be detected in the serum (data not shown). Therefore, treatment with IL-15 alone is unlikely to achieve the full therapeutic potential of the cytokine. The combined administration of IL-15/IL-15R may provide improved efficacy by driving transpresentation through available IL-15R/C.

The activity of complexed IL-15/IL-15R appears to be mediated at multiple levels. Mortier et al. (26) recently demonstrated that IL-15 bound to sIL-15R has a higher affinity for IL-15R/C than does free IL-15. Thus, from our data and that of others, binding of IL-15 by IL-15R-chain can increase IL-15 potency by 1) increasing IL-15 half-life (Fig. 4), 2) increasing IL-15 affinity for IL-15R/C (26), and 3) providing a platform for transpresentation. Future work will examine the mechanisms of the IL-15R-mediated increase in IL-15 half-life. Possible mechanisms involve 1) protection of IL-15 from degradation by proteases, 2) inhibition of clearance via receptor binding or other mechanisms, or 3) FcR-mediated binding/recycling of complex. In regard to the latter, although the presence of the Ig Fc portion in the complex could augment activity through FcR-mediated signaling, IL-15 bound to monomeric sIL-15R lacking a Fc, retained function in vivo, although a quantitative comparison with the Fc-containing molecule was not performed (data not shown).

The ability of IL-15/IL-15R to drive T cell activation was of particular interest given the current paradigm regarding the requirements for naive and memory T cell homeostatic survival and proliferation. Under normal conditions, survival of both naive and memory CD8 T cells requires IL-7 (64), whereas IL-15 is essential for homeostatic proliferation of memory CD8 T cells (9) and NK cell survival (24, 76) in normal hosts. In a lymphopenic environment, IL-7 is required for homeostatic proliferation of naive CD8 and CD4 T cells (64), and plays a role, along with IL-15, in mediating CD8 memory T cell homeostatic proliferation (62). Thus, it was unexpected that naive CD8 T cells responded vigorously to the IL-15/IL-15R complex. It should be noted, however, that in IL-15^–/– mice, the naive CD8 T cell pool is decreased 50%, suggesting that either naive CD8 T cell development and/or survival requires IL-15 (7). In any case, proliferation of naive, as well as memory phenotype, CD8 T cells driven by receptor-bound IL-15 was IL-7 independent and required IL-15R signaling. This result indicated that naive CD8 T cells expressed sufficient levels of IL-15R to respond to IL-15/IL-15R but not to sIL-15 alone. Previous reports also show that IL-15 activates naive human CD8 T cells in vitro (77, 78). Interestingly, the naive CD8 T cell response to cytokine paralleled that of an Ag-specific response, although the response was driven by unphysiological levels of IL-15 activity. Nevertheless, clonal expansion occurred, and effector function was induced, followed by contraction of the responding population and generation of memory CD8 T cells. Phenotypic changes similar to those observed following TCR triggering also accompanied activation via receptor-complexed IL-15, with CD69 levels up-regulated and IL-7R down-regulated early after treatment. This process occurred in the absence of Ag, although whether MHC is necessary for these events is currently under investigation. A previous in vitro study showed that IL-15 induced a similar activation and genetic profile in human CD8 memory T cells as did TCR cross-linking (79), suggesting some overlap in the signaling pathways activated by these receptors. Additional experimentation will be needed to decipher the underlying mechanisms of naive CD8 T cell activation mediated by IL-15.

Our findings also highlight the potential of receptor-complexed IL-15 as a cancer therapeutic. Two doses of complexed IL-15 were able to lead to the rejection (or prevent the establishment) of B16 melanoma tumors, whereas IL-15 alone was not able to diminish tumor burden. Future studies will examine the effect of IL-15/IL-15R on more established tumors using a variety of doses and treatment schedules, as well as determining the mechanism and cell types involved in tumor rejection.

These findings present a conundrum, considering that sIL-15R has been used to inhibit collagen-induced arthritis (29), cardiac allograft rejection (30), delayed type hypersensitivity (75), and allergic airway disease (80). Interestingly, initiation of all of these conditions is dependent, either solely or in part, on CD4 T cells, suggesting that CD4 T cells may respond to IL-15 indirectly. Thus, IL-15 may activate dendritic cells during certain immune responses (75) leading to CD4 T cell activation, and this event could hypothetically occur via direct IL-15 action through IL-15R in the absence of IL-15R, rather than through transpresentation. In this scenario, activation of CD4 T cells, and in some cases CD8 T cells, could be inhibited by administration of sIL-15R if levels of free IL-15 are elevated, as is known to occur in inflammatory diseases. Recent data (81) also show that a cell surface form of IL-15 exists whose function in vivo remains obscure, but binding of sIL-15R to such a molecule could also exert potential inhibitory effects. Some diversion of the response toward CD8 and NK/NK T cell activation through treatment with sIL-15R may also result in inhibition of certain immune responses. Further studies are needed to determine the parameters that determine whether inhibition or augmentation of immune responses is the outcome of manipulation of the IL-15 system.

During the course of our studies, we became aware of the work of Rubinstein et al. (82), whose study also shows that complexing sIL-15R to IL-15 results in hyperagonist activity toward CD8 memory T cells and NK cells in vivo, although the mechanisms of action based on transpresentation and increasing half-life and bioavailability were not examined in detail in that study. Our studies also go beyond their findings by showing that naive CD8 T cells respond to IL-15/IL-15R, resulting in effector cell induction and memory T cell generation. In addition, our B16 tumor findings highlight the potential of complexed IL-15 as a tumor immunotherapy agent. Together, these findings illustrate the potential power of IL-15 in driving robust NK/NK T and CD8 T cell expansion and effector differentiation in intact hosts, which may have important immunotherapeutic applications.

	Disclosures

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The authors have no financial conflict of interest.

	Footnotes

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

¹ This work was supported by National Institutes of Health Grants AI51583 and P01 AI56172 (to L.L.) and U.S. Public Health Service Training Grant T32 AI07080 (to T.A.S.).

² Current address: Department of Immunology, University of Texas MD Anderson Cancer Center, Houston, TX 77030.

³ Address correspondence and reprint requests to Dr. Leo Lefrançois, Department of Immunology, University of Connecticut Health Center, 263 Farmington Avenue, Farmington, CT 06030-1319. E-mail address: llefranc{at}neuron.uchc.edu

⁴ Abbreviations used in this paper: C, common -chain; sIL, soluble IL; VSV, vesicular stomatitis virus; hIL, human IL; rm, recombinant murine.

Received for publication June 12, 2006. Accepted for publication August 3, 2006.

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