Interaction between different leukocyte subsets and stromal cells in different organ microenvironments is critical for optimizing organ-specific immune responses that could limit metastasis formation and control disease-induced inflammation. IL-12 and IL-18 are potent immunoregulatory cytokines for natural killer (NK), NKT, and T cells, and have very distinctive effects on the NKT/NK subsets in different organs. The liver is a major target for the formation of metastases. We used a mouse model of liver metastasis to study the anti-tumor activity of IL-18 and/or IL-12 cytokines and the roles of NK and NKT cells to these responses. Treating mice with IL-18 plus IL-12 significantly reduced the number of tumor nodules in the liver to a greater degree than did either of the cytokines alone. As expected, IL-18 plus IL-12 stimulated a synergistic increase in systemic IFN-gamma in tumor bearing mice. The anti-tumor activity of IL-18 plus IL-12 therapy was abolished in IFN-gamma(-/-) mice. Using intracellular staining, NK and NKT cells were identified as the major producers of IFN-gamma in the livers of mice treated with IL-18 and/or IL-12. Liver NK cells were increased with daily treatment of mice with IL-18 plus IL-12 whereas liver NKT cells were diminished by this treatment. Preferential depletion of NK cells with anti-asGM1 resulted in a partial loss of the anti-tumor activity of IL-18 plus IL-12 therapy and revealed NK cells to be an important component of the mechanism for tumor regression. In contrast, the preferential depletion of NKT cells with betaGalCer decreased the number of liver tumor nodules in mice treated with vehicle control or IL-18 alone. Similarly, all treatment approaches showed increased anti-tumor activity in CD1d(-/-) mice, which lack NKT cells. Our data therefore shows that the IL-18 plus IL-12 induced anti-tumor activity in mice is NK and IFN-gamma dependent, and is able to overcome an endogenous immunosuppressive effect of NKT cells. These results thereby suggest that immunotherapeutic approaches that enhance NK cell numbers and function while preferentially depleting NKT cells could be effective in the treatment of cancer in the liver. Because IL-18 plus IL-12 treatment of tumor bearing mice elicited significant anti-tumor activity concurrent with a decrease in the detectable number of invariant NKT (iNKT) cells, we compared iNKT cell modulation mechanisms of alpha-GalCer, a glycolipid known to modulate iNKT cells, and IL-18 plus IL-12. We found acute treatment with IL-18 + IL-12 induced a loss of NK1.1(+) subset of iNKT cells, while acute treatment with aGalCer depleted all liver iNKT cells at 24hrs. However, other lymphoid tissues showed little to know loss of these cells suggesting the liver microenviroment is a critical regulator of iNKT cells. At 72hrs iNKT cells repopulated and expanded in the liver following aGalCer and IL-18 plus IL-12 treatment of mice. To study this expansion, we administered BrdU to mice 24hrs after acute treatment with IL-18 plus IL-12 or aGalCer and found a high percentage of proliferating iNKT cells. We further found the spleen was needed for iNKT repopulation and expansion following aGalCer, but not for IL-18 plus IL-12 treatment, as no expansion was observed in splenectomized mice. We next examined chronic treatment of mice with aGalCer or IL-18 plus IL-12 and found aGalCer induced a severe loss of liver iNKT cells, while only IL-18 plus IL-12 caused a systemic loss of iNKT cells. Long term ( greater than 60 days) thymic development was needed to repopulate the liver following both treatments. These data reveal an important role for the liver microenvironment in regulating iNKT cell response to inflammatory signals. Based on our data, our hypothesis for this project is that stimulation of NKT cells via cytokine receptors vs the TCR results in qualitatively different changes in NKT cell subsets and functions, and thereby alter their role in inflammation and/or anti-tumor immunity. To date, we have contrasted the effects of IL-12 and IL-18, two potent inducers of IFNgamma, which are known to dramatically influence functions of NKT cells with the biologically distinct effects induced by ligation of the invariant TCR expressed on these cells. Major findings include the demonstration that IL-12 and IL-18 synergize for the preferential depletion/absence of NKT cells, and the loss of NKT cells increases resistance to metastasis formation which has revealed a previously unappreciated regulatory role for NKT cells in the liver. Detailed examination of NKT cell populations following acute or chronic treatment with IL-12 + IL-18 or the NKT- specific antigen alpha-galactosylceramide (aGalCer) has also revealed different mechanisms for activation- induced depletion and recovery, and show that NKT cell phenotypes and functions can be profoundly and differentially reshaped by TCR vs cytokine signaling.

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Investigator-Initiated Intramural Research Projects (ZIA)
Project #
1ZIABC009322-22
Application #
8157232
Study Section
Project Start
Project End
Budget Start
Budget End
Support Year
22
Fiscal Year
2010
Total Cost
$370,298
Indirect Cost
Name
National Cancer Institute Division of Basic Sciences
Department
Type
DUNS #
City
State
Country
Zip Code
Chan, Tim; Back, Timothy C; Subleski, Jeffrey J et al. (2012) Systemic IL-12 administration alters hepatic dendritic cell stimulation capabilities. PLoS One 7:e33303
Subleski, Jeff J; Jiang, Qun; Weiss, Jonathan M et al. (2011) The split personality of NKT cells in malignancy, autoimmune and allergic disorders. Immunotherapy 3:1167-84
Subleski, Jeff J; Hall, Veronica L; Wolfe, Thomas B et al. (2011) TCR-dependent and -independent activation underlie liver-specific regulation of NKT cells. J Immunol 186:838-47
Chan, Tim; Wiltrout, Robert H; Weiss, Jonathan M (2011) Immunotherapeutic modulation of the suppressive liver and tumor microenvironments. Int Immunopharmacol 11:879-89
Subleski, Jeff J; Wiltrout, Robert H; Weiss, Jonathan M (2009) Application of tissue-specific NK and NKT cell activity for tumor immunotherapy. J Autoimmun 33:275-81