| Literature DB >> 28096513 |
Heather Torrey1, John Butterworth1, Toshiyuki Mera1, Yoshiaki Okubo1, Limei Wang1, Danielle Baum1, Audrey Defusco1, Sara Plager1, Sarah Warden1, Daniel Huang1, Eva Vanamee1, Rosemary Foster2, Denise L Faustman3.
Abstract
Major barriers to cancer therapy include the lack of selective inhibitors of regulatory T cells (Tregs) and the lack of broadly applicable ways to directly target tumors through frequently expressed surface oncogenes. Tumor necrosis factor receptor 2 (TNFR2) is an attractive target protein because of its restricted abundance to highly immunosuppressive Tregs and oncogenic presence on human tumors. We characterized the effect of TNFR2 inhibition using antagonistic antibodies. In culture-based assays, we found that two TNFR2 antagonists inhibited Treg proliferation, reduced soluble TNFR2 secretion from normal cells, and enabled T effector cell expansion. The antagonistic activity occurred in the presence of added TNF, a natural TNFR2 agonist. These TNFR2 antibodies killed Tregs isolated from ovarian cancer ascites more potently than it killed Tregs from healthy donor samples, suggesting that these antibodies may have specificity for the tumor microenvironment. The TNFR2 antagonists also killed OVCAR3 ovarian cancer cells, which have abundant surface TNFR2. The antibodies stabilized antiparallel dimers in cell surface TNFR2 that rendered the receptor unable to activate the nuclear factor κB pathway and trigger cell proliferation. Our data suggest that, by targeting tumor cells and immunosuppressive tumor-associated Tregs, antagonistic TNFR2 antibodies may be an effective treatment for cancers positive for TNFR2.Entities:
Mesh:
Substances:
Year: 2017 PMID: 28096513 DOI: 10.1126/scisignal.aaf8608
Source DB: PubMed Journal: Sci Signal ISSN: 1945-0877 Impact factor: 8.192