Ty to suppress T cell responses, and differentiated into mature macrophages and DCs [23]. In addition, ex vivo generation of human MDSCs from normal donor PBMCs by exposure to cytokines and tumor cell lines was associated with increased expression of NADPH oxidase constituent proteins [24,25].Taken together, these observations point to NADPH oxidase potentially favoring tumor progression by augmenting MDSC accumulation and immunosuppression in the tumor microenvironment. EOC is characterized by peritoneal implants, ascites, and accumulation of tumor-associated macrophages and MDSCs [26,27]. The effect of NADPH oxidase in these myeloid cells on tumor progression and local immune responses is unclear. Our major goals were to delineate the role of NADPH oxidase in ovarian tumor progression and in modulating MDSC accumulation and function in murine EOC. We found that tumor progression was similar between WT and engineered 16574785 NADPH oxidase-deficient mice. Granulocytic and monocytic MDSC accumulation in the peritoneum and spleen was similar between genotypes. Although MDSCs from tumor-bearing WT mice had functional NADPH oxidase, the suppressive effect of MDSCs on ex vivo stimulated T cell proliferation was NADPH oxidase-independent. We therefore conclude that in murine EOC, NADPH oxidase is dispensable for MDSC accumulation and immunosuppressive function. Understanding how the oxidative milieu modulates MDSC function, including NADPH oxidase-dependent and –101043-37-2 site independent pathways, may lead to novel ways to target these cells to enhance durable anti-tumor immunity.Park Cancer Institute Institutional Animal Care and Use Committee.MiceMice with a targeted disruption of the p47phox gene (p47phox2/2) have a defective phagocyte NADPH oxidase (NOX2), rendering phagocytes incapable of generating measurable superoxide [28]. p47phox2/2 mice are backcrossed 14 generations in the C57BL/ 6Ncr. A p47phox2/2 mouse breeding colony is established at Roswell Park Cancer Institute (Buffalo, NY) and gp91phox2/2 female mice were purchased from Jackson Labs (Bar Harbor, ME). Female mice (age 6? weeks) were used in all experiments. All mice were maintained under specific pathogen free conditions at the animal care facility at Roswell Park Cancer Institute and used in compliance with all relevant laws and institutional guidelines under a protocol approved by the Roswell Park Cancer Institute Institutional Animal Care and Use Committee.Mouse ovarian surface epithelial cancer (MOSEC) cellsThe ID8 MOSEC line was derived from epithelial ovarian cells harvested from female C57BL/6 (H-2b) mice that were passaged in vitro [29]. Intraperitoneal injection of clonal lines established from late passage epithelial cells from syngeneic tumors in C57BL/6 mice results in ascites and peritoneal implants that mimic the human disease [29]. ID8 MOSEC cells (a kind gift from Dr. P. Terranova, University of Kansas Medical Center, Kansas City, USA) were cultured in RPMI 1640 media with heat-inactivated FBS (10 ), L-glutamine (2 mM), HEPES (25 mM), 58-49-1 cost Sodium Pyruvate (1 mM), 2-Mercaptoethanol (50 mM), Penicillin-Streptomycin (100 U/ml), and non-essential amino acids.Tumor 23977191 administrationMice were administered intraperitoneal ID8 MOSEC cells (56106 cells in 200 mL PBS/mouse). For survival experiments, mice were monitored up to 150 days, and euthanized based on abdominal distention, ruffled fur, lethargy or inability to ambulate. In separate experiments, mice were sacrificed on day 42 or 90 after tu.Ty to suppress T cell responses, and differentiated into mature macrophages and DCs [23]. In addition, ex vivo generation of human MDSCs from normal donor PBMCs by exposure to cytokines and tumor cell lines was associated with increased expression of NADPH oxidase constituent proteins [24,25].Taken together, these observations point to NADPH oxidase potentially favoring tumor progression by augmenting MDSC accumulation and immunosuppression in the tumor microenvironment. EOC is characterized by peritoneal implants, ascites, and accumulation of tumor-associated macrophages and MDSCs [26,27]. The effect of NADPH oxidase in these myeloid cells on tumor progression and local immune responses is unclear. Our major goals were to delineate the role of NADPH oxidase in ovarian tumor progression and in modulating MDSC accumulation and function in murine EOC. We found that tumor progression was similar between WT and engineered 16574785 NADPH oxidase-deficient mice. Granulocytic and monocytic MDSC accumulation in the peritoneum and spleen was similar between genotypes. Although MDSCs from tumor-bearing WT mice had functional NADPH oxidase, the suppressive effect of MDSCs on ex vivo stimulated T cell proliferation was NADPH oxidase-independent. We therefore conclude that in murine EOC, NADPH oxidase is dispensable for MDSC accumulation and immunosuppressive function. Understanding how the oxidative milieu modulates MDSC function, including NADPH oxidase-dependent and -independent pathways, may lead to novel ways to target these cells to enhance durable anti-tumor immunity.Park Cancer Institute Institutional Animal Care and Use Committee.MiceMice with a targeted disruption of the p47phox gene (p47phox2/2) have a defective phagocyte NADPH oxidase (NOX2), rendering phagocytes incapable of generating measurable superoxide [28]. p47phox2/2 mice are backcrossed 14 generations in the C57BL/ 6Ncr. A p47phox2/2 mouse breeding colony is established at Roswell Park Cancer Institute (Buffalo, NY) and gp91phox2/2 female mice were purchased from Jackson Labs (Bar Harbor, ME). Female mice (age 6? weeks) were used in all experiments. All mice were maintained under specific pathogen free conditions at the animal care facility at Roswell Park Cancer Institute and used in compliance with all relevant laws and institutional guidelines under a protocol approved by the Roswell Park Cancer Institute Institutional Animal Care and Use Committee.Mouse ovarian surface epithelial cancer (MOSEC) cellsThe ID8 MOSEC line was derived from epithelial ovarian cells harvested from female C57BL/6 (H-2b) mice that were passaged in vitro [29]. Intraperitoneal injection of clonal lines established from late passage epithelial cells from syngeneic tumors in C57BL/6 mice results in ascites and peritoneal implants that mimic the human disease [29]. ID8 MOSEC cells (a kind gift from Dr. P. Terranova, University of Kansas Medical Center, Kansas City, USA) were cultured in RPMI 1640 media with heat-inactivated FBS (10 ), L-glutamine (2 mM), HEPES (25 mM), Sodium Pyruvate (1 mM), 2-Mercaptoethanol (50 mM), Penicillin-Streptomycin (100 U/ml), and non-essential amino acids.Tumor 23977191 administrationMice were administered intraperitoneal ID8 MOSEC cells (56106 cells in 200 mL PBS/mouse). For survival experiments, mice were monitored up to 150 days, and euthanized based on abdominal distention, ruffled fur, lethargy or inability to ambulate. In separate experiments, mice were sacrificed on day 42 or 90 after tu.
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