Interestingly, several pieces
of evidence support the idea that the cytokine milieu greatly affects Treg-cell response to OX40 triggering. We have previously shown that OX86 reverses Treg-cell suppression in graft versus host disease (GVHD) 54 and in tumors 3, while others have reported that OX86 administration to naïve mice promotes Treg-cell expansion, thus reinforcing suppression 55. Therefore, the outcome of OX40 stimulation may vary depending on microenvironmental cues. Conversely, OX40 may affect Treg-cell response to cytokine stimulation. Indeed, OX40 signal Opaganib supplier supports Treg-cell susceptibility to IL-2 by sustaining miR155 expression and restraining SOCS1 availability 56. These data highlight the importance of understanding how different microenvironments influence
Treg-cell behavior and how to take advantage of Treg-cell plasticity for the development of efficient cancer immunotherapies. The strictly Treg-cell-intrinsic modifications CH5424802 detected in the transcriptome of sorted Treg cells, treated or not with OX40 agonist Ab, were relatively few and of limited extent (all modulations were below 1.8-fold). However, according to the above considerations about OX40 tuning cytokine susceptibility, far wider effects may be elicited by OX40 stimulation in Treg cells embedded in a complex microenvironment and exposed to a panoply of signals. Among downregulated genes, beside Irf1, attention should be paid to Igtp and Iigp2 (also called Irgm2), belonging to p47-GTPase family that, like Irf1, are downstream IFN-γ
during the immune responses to pathogens 57. Again, the expression levels of both Igtp and Irgm2 were particularly high in Treg cells derived from lamina propria 45. Other modifications induced in Treg-cell transcriptome by OX40 triggering seemed to affect Treg-cell homing or Treg-cell ability to recruit other cells: Ccr8 and Itgae (encoding for CD103) were increased, Ccl4 and Xcl1 were decreased. A general interpretation of these changes is complex. CD103 is an integrin dictating gut homing, and OX40 is required for Treg-cell accumulation in the colon 58. However, in a model of PJ34 HCl T-cell transfer-induced colitis, OX40-deficient Treg cells expressed normal levels of CD103 and properly accumulated in the lamina propria 56. Contrary to Treg cells, effector T cells express OX40 only upon activation 11, 59. We found that Tem cells, representing the most abundant TIL subset, highly expressed OX40. This class of memory lymphocytes was reported to constitutively express CD40L at sufficient levels to induce DC activation 17. We hypothesized that, at the tumor site, the presence of immune-suppressive elements could render the basal CD40/CD40L-mediated interaction insufficient for optimal DC stimulation by Tem cells, and that OX40 triggering may supply to Tem cells the adequate boost.