Ablation of T cell–associated PD-1H enhances functionality and promotes adoptive immunotherapy
Li Hu, Ling Chen, Zexiu Xiao, Xu Zheng, Yuangui Chen, Na Xian, Christina Cho, Liqun Luo, Gangxiong Huang, Lieping Chen
Li Hu, Ling Chen, Zexiu Xiao, Xu Zheng, Yuangui Chen, Na Xian, Christina Cho, Liqun Luo, Gangxiong Huang, Lieping Chen
View: Text | PDF
Research Article Immunology Therapeutics

Ablation of T cell–associated PD-1H enhances functionality and promotes adoptive immunotherapy

Abstract

Programmed death-1 homolog (PD-1H) is a coinhibitory molecule that negatively regulates T cell–mediated immune responses. In this study, we determined whether ablation of T cell–associated PD-1H could enhance adoptive T cell therapy in experimental tumor models. The expression of PD-1H is upregulated in activated and tumor-infiltrating CD8+ T cells. Activated CD8+ T cells from PD-1H–deficient (PD-1H–KO) mice exhibited increased cell proliferation, cytokine production, and antitumor activity in vitro. Adoptive transfer of PD-1H–KO CD8+ T cells resulted in the regression of established syngeneic mouse tumors. Similar results were obtained when PD-1H was ablated in T cells by CRISPR/Cas9-mediated gene silencing. Furthermore, ablation of PD-1H in CAR-T cells significantly improved their antitumor activity against human xenografts in vivo. Our results indicate that T cell–associated PD-1H could suppress immunity in the tumor microenvironment and that targeting PD-1H may improve T cell adoptive immunotherapy.

Authors

Li Hu, Ling Chen, Zexiu Xiao, Xu Zheng, Yuangui Chen, Na Xian, Christina Cho, Liqun Luo, Gangxiong Huang, Lieping Chen

×

Figure 3

PD-1H suppresses the function of CD8+ T cells ex vivo.

Options: View larger image (or click on image) Download as PowerPoint
PD-1H suppresses the function of CD8+ T cells ex vivo. CFSE-labeled WT o...
CFSE-labeled WT or PK CD8+ T cells were stimulated by plate-bound anti-mCD3. (A) Cell proliferation was analyzed at the end of 72 hours of culture. (B) Supernatants were harvested from 96-well proliferation plates at 72 hours and analyzed for IFN-γ, IL-17A, and TNF. (C) Purified of PKO or WT OT-I cells were stimulated with 1 μM OVA peptide–pulsed irradiated PK splenocytes. Proliferation was analyzed at 48 and 72 hours. (D) Supernatants were harvested from proliferation assays at 48 hours and analyzed for cytokines at specific peptide concentrations. Duplicated wells were analyzed for all conditions. All data are mean ± SEM and represent 3 independent experiments. *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001 by 2-way ANOVA.