The lck-DPP kd mice were analyzed for the level and specificity of DPP2 kd. dpp2 transcript levels were measured, because an antibody against murine DPP2 is currently unavailable. dpp2 mRNA was reduced by about 50% in whole splenocytes (Fig. 1C) and by over 90% in isolated peripheral T cells (Fig. 1D) from lck-DPP2 kd mice compared with littermate controls.
Thymic development was indistinguishable in lck-DPP2-kd and control mice, as evidenced by normal absolute numbers (data not shown) and percentages of thymocyte subsets (Fig. 2). Similarly, the absolute numbers of lymphocytes in the peripheral lymphoid organs were identical to those of littermate controls; however, the proportions of CD4+ and CD8+ T cells were increased about 40% in the spleen and, to a lesser extent, in the lymph nodes of the lck-DPP kd mice, and the proportion Everolimus order of B cells was decreased (Fig. 2). No difference in activation marker expression, CD4+CD44hiCD62L, GPCR Compound Library CD8+CD33hiCD122+, CD25+ and CD69+, was observed in the peripheral T cells of lck-DPP kd compared with control mice (Supporting Information Fig. 2 and data not shown). DPP2 has been shown to maintain cells in a quiescent state, and its inhibition in vitro results in cells drifting into G1 of the cell cycle 5. Thus, we reasoned that the loss of DPP2 may cause T cells to proliferate faster
than normal cells. To test this hypothesis, splenocytes and lymph node cells from lck-DPP kd mice and littermate controls were stimulated with various concentrations of anti-CD3 alone or in combination with anti-CD28, followed by an 8 h [3H]-thymidine pulse at various time points. As shown in Fig. 3A, more T cells from lck-DPP kd mice entered S-phase compared with those of control mice. Even after just two days of stimulation, lck-DPP kd T cells incorporated more [3H]-thymidine into newly synthesized DNA than control T cells, suggesting that DPP2 inhibition causes T cells to proliferate faster. To analyze the proliferative phenotypes of the individual
T-cell subpopulations, CD4+ and CD8+ T cells were isolated from the spleen and lymph nodes by negative selection. Similarly to what we had observed in unseparated selleck antibody lymphocytes, both CD4+ and CD8+ T cells from lck-DPP kd mice proliferated more than those of littermate controls (Fig. 3B and C), thus confirming our initial results. The hyper-proliferative phenotype of the activated T cells from lck-DPP kd mice prompted the analysis of the cytokines secreted by these cells. Whole splenocytes and lymph node cells or isolated CD4+ and CD8+ T cells were simulated with anti-CD3 plus anti-CD28, and supernatants were collected 24, 48 and 72 h later and tested by ELISA for the level of IL-2, IFN-γ, IL-4 and IL-17 cytokines. Very little IL-2 was observed in the supernatant of unseparated lymphocytes (Fig. 4A), probably due to the rapid use of this cytokine by the activated CD8+ T cells.