In addition, co-transfer of CD122-depleted spleen cells exhibited no effect on the tumor-growth and survival of melanoma-bearing mice after treatment with transfer of pmel-1 T cells and DC vaccination (Supporting Information Fig.
4), further supporting the notion that CD122+ cells were the major suppressor cells in naïve spleens. Since CD122+CD8+ T cells that functioned as Treg have been described in autoimmune disease models (see review 20), we will hereafter refer to these cells as the CD122+CD8+ Treg. The beneficial antitumor selleck screening library effects that follow depletion of CD4+CD25+ natural Treg have been well described 21. We sought to determine whether depletion of CD122+CD8+ Treg in addition to CD4+CD25+ natural Treg would further enhance the expansion and survival of pmel-1 T cells. Since NK cells and NK T cells were the other major CD122+ populations, their contribution to immune regulation was also investigated. Spleen cells from WT mice were subjected to depletion of CD25+ cells alone, CD25+ and NK1.1+ cells, and CD25+ and CD122+ T cells using magnetic beads. As expected, depletion with anti-CD25 or NK1.1 antibodies resulted in near-complete disappearance
of cells expressing CD25 or NK1.1, respectively. NK depletion resulted in elimination of both NK and NKT cells, while the CD122+ non-NK1.1 expressing cells remained. CD122− depletion resulted in near complete elimination of both NK1.1+ cells and CD8+CD122+ T cells (Fig. 2A). ZD1839 solubility dmso At wk 4 after vaccination, depletion of CD25+ cells from naïve spleen before adoptive transfer
had no effect on the number of pmel-1 T cells in blood (13% of CD8+ T cells) or spleen (400/106 spleen cells) (Fig. 2B and C). However, CD25- and CD122-depleted mice also exhibited a pronounced increase in the Erastin concentration number of endogenous peptide-specific T cells, identified by hgp9-Db tetramer staining (GFP-tetramer+) (Fig. 2B). In addition, 7% of total CD8+ T cells in the blood of mice with CD25 and CD122 depletion were positive for hgp9-tetramer+ GFP−, compared with 2 or 3% of CD8+ T cells in the control or CD25 only depletion group. Thus, the removal of CD122+ cells in addition to CD25+ cells led to expansion of both transgenic pmel-1 T cells and non-transgenic peptide-specific T cells. Four weeks after adoptive transfer the number of pmel-1 T cells in the spleen of mice from the CD25 and CD122 depletion group was threefold greater than in the control or CD25 depletion group (Fig. 2C). The function of pmel-1 T cells found in spleens among all three groups of mice was comparable as demonstrated by a similar production of IFN-γ upon ex vivo stimulation with peptide (Fig. 2D). Taken together, these experiments showed that lymphopenia-driven proliferation of CD4+CD25+ and CD122+CD8+ T cells negatively regulated proliferation of Ag-specific pmel-1 T cells and non-transgenic T cells in lymphodepleted mice.