MFG-E8–mediated uptake of apoptotic cells by APCs links the pro- and antiinflammatory activities of GM-CSF
Masahisa Jinushi, Yukoh Nakazaki, Michael Dougan, Daniel R. Carrasco, Martin Mihm, Glenn Dranoff
Masahisa Jinushi, Yukoh Nakazaki, Michael Dougan, Daniel R. Carrasco, Martin Mihm, Glenn Dranoff
View: Text | PDF
Research Article Oncology

MFG-E8–mediated uptake of apoptotic cells by APCs links the pro- and antiinflammatory activities of GM-CSF

Abstract

Granulocyte-macrophage colony-stimulating factor (GM-CSF) enhances protection against tumors and infections, but GM-CSF–deficient mice develop inflammatory disease. Here we show that GM-CSF is required for the expression of milk fat globule EGF 8 (MFG-E8) in antigen-presenting cells, and that MFG-E8–mediated uptake of apoptotic cells is a key determinant of GM-CSF–triggered tolerance and immunity. Upon exposure to apoptotic cells, GM-CSF–deficient antigen-presenting cells (APCs) produce an altered cytokine profile that results in decreased Tregs and increased Th1 cells, whereas concurrent ablation of IFN-γ promotes Th17 cells. In wild-type mice, MFG-E8 attenuates the vaccination activity of GM-CSF–secreting tumor cells through Treg induction, whereas a dominant-negative MFG-E8 mutant potentiates GM-CSF–stimulated tumor destruction through Treg inhibition. These findings clarify the immunoregulatory effects of apoptotic cells and suggest new therapeutic strategies to modulate CD4+ T cell subsets in cancer and autoimmunity.

Authors

Masahisa Jinushi, Yukoh Nakazaki, Michael Dougan, Daniel R. Carrasco, Martin Mihm, Glenn Dranoff

×

Figure 6

MFG-E8 reconstitution restores CD4+ T cell homeostasis in vivo.

Options: View larger image (or click on image) Download as PowerPoint
MFG-E8 reconstitution restores CD4+ T cell homeostasis in vivo. ...
(A) Peritoneal macrophages recovered 2 months following transplantation (5 mice per group) were assayed for phagocytosis of labeled apoptotic thymocytes. Numbers refer to the percentage of cells within an indicated gate. (B) Serum cytokine levels measured by ELISA 2 months after transplant (n = 4). (C) Splenocytes (n = 4) were harvested 2 months after transplant and assayed for FoxP3 expression and (D) IL-17 and IFN-γ expression (CD3+CD4+ gated cells). (E) Peritoneal macrophages from mice that received transplants were loaded with apoptotic cells and used to stimulate allogeneic Balb/c splenocytes. Proliferation was determined by 3H-thymidine uptake. Similar results were obtained with 2 independent transplant experiments.