OX40 ligand expressed by DCs costimulates NKT and CD4+ Th cell antitumor immunity in mice
Jamal Zaini, … , Toshihiro Nukiwa, Toshiaki Kikuchi
Jamal Zaini, … , Toshihiro Nukiwa, Toshiaki Kikuchi
Published November 1, 2007
Citation Information: J Clin Invest. 2007;117(11):3330-3338. https://doi.org/10.1172/JCI32693.
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Research Article

OX40 ligand expressed by DCs costimulates NKT and CD4+ Th cell antitumor immunity in mice

Abstract

The exceptional immunostimulatory capacity of DCs makes them potential targets for investigation of cancer immunotherapeutics. We show here in mice that TNF-α–stimulated DC maturation was accompanied by increased expression of OX40 ligand (OX40L), the lack of which resulted in an inability of mature DCs to generate cellular antitumor immunity. Furthermore, intratumoral administration of DCs modified to express OX40L suppressed tumor growth through the generation of tumor-specific cytolytic T cell responses, which were mediated by CD4+ T cells and NKT cells. In the tumors treated with OX40L-expressing DCs, the NKT cell population significantly increased and exhibited a substantial level of IFN-γ production essential for antitumor immunity. Additional studies evaluating NKT cell activation status, in terms of IFN-γ production and CD69 expression, indicated that NKT cell activation by DCs presenting α-galactosylceramide in the context of CD1d was potentiated by OX40 expression on NKT cells. These results show a critical role for OX40L on DCs, via binding to OX40 on NKT cells and CD4+ T cells, in the induction of antitumor immunity in tumor-bearing mice.

Authors

Jamal Zaini, Sita Andarini, Minoru Tahara, Yasuo Saijo, Naoto Ishii, Kazuyoshi Kawakami, Masaru Taniguchi, Kazuo Sugamura, Toshihiro Nukiwa, Toshiaki Kikuchi

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Figure 5

NKT cell activation in an OX40-dependent manner.

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NKT cell activation in an OX40-dependent manner. (A) IFN-γ in serum. Wil...
(A) IFN-γ in serum. Wild-type, OX40–/–, or NKT cell–/– mice were injected intravenously with α-GalCer or vehicle. The levels of IFN-γ were determined in serum by ELISA. (B) IFN-γ in splenocyte culture. Splenocytes were isolated from wild-type, OX40–/–, or NKT cell–/– mice and cultured with α-GalCer or vehicle. The levels of IFN-γ in the culture medium were assayed by ELISA. (C) IFN-γ in splenocyte coculture. Splenocytes from NKT cell–/– mice were cocultured with NKT cells isolated from wild-type or OX40–/– mice in the presence of α-GalCer. Where indicated, anti-CD1d antibody or control IgG was added at the initiation of the coculture. The levels of IFN-γ were assayed by ELISA. (D) CD69 on NKT cells in splenocyte coculture. The study was similar to that in C, but at the end of coculture, NKT cells were analyzed for the surface expression of CD69 by flow cytometry. Overlay (filled) histograms depict NKT cells cocultured in the absence of α-GalCer as a control. The percentages of stained cells above isotype control staining are shown in each panel.