HO-1 impairs the efficacy of radiotherapy by redistributing cGAS and STING in tumors
Chuqing Zhang, Zhenji Deng, Jiawei Wu, Cong Ding, Zhe Li, Zhimin Xu, Weipeng Chen, Kaibin Yang, Hanmiao Wei, Tingxiang He, Liufen Long, Jun Ma, Cheng Xu, Xiaoyu Liang
Chuqing Zhang, Zhenji Deng, Jiawei Wu, Cong Ding, Zhe Li, Zhimin Xu, Weipeng Chen, Kaibin Yang, Hanmiao Wei, Tingxiang He, Liufen Long, Jun Ma, Cheng Xu, Xiaoyu Liang
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Research Article Immunology Oncology

HO-1 impairs the efficacy of radiotherapy by redistributing cGAS and STING in tumors

Abstract

Type I IFNs (IFN-Is) induced by radiotherapy (RT) are critical for its efficacy, while the mechanism by which tumor cells inhibit IFN-I production remains largely unsolved. By an unbiased CRISPR screen, we identified hemeoxygenase 1 (HO-1) as an RT-related regulator of IFN-I production. Mechanistically, the ER-anchored, full-length HO-1 disrupted stimulator of IFN genes (STING) polymerization and subsequent coat protein complex II–mediated (COPII-mediated) ER-Golgi transportation, leading to hampered activation of downstream signaling. This process was exacerbated by the upregulation of HO-1 expression under RT. Importantly, RT also induced HO-1 cleavage. Cleaved HO-1 underwent nuclear translocation, interacted with cyclic GMP-AMP synthase (cGAS), and inhibited its nuclear export upon irradiation, leading to suppressed 2′3′-cyclic GMP-AMP (cGAMP) production. Furthermore, we revealed that HO-1 inhibitors could enhance local and distant tumor control of RT in vivo. Clinically, higher HO-1 expression was associated with a poorer prognosis and earlier tumor relapse after RT in multiple types of patient tumors. Collectively, through comprehensive inhibition of the cGAS/STING pathway, HO-1 strongly inhibited RT-induced IFN-I production, and targeting HO-1 was shown to be a promising RT-sensitizing therapeutic strategy.

Authors

Chuqing Zhang, Zhenji Deng, Jiawei Wu, Cong Ding, Zhe Li, Zhimin Xu, Weipeng Chen, Kaibin Yang, Hanmiao Wei, Tingxiang He, Liufen Long, Jun Ma, Cheng Xu, Xiaoyu Liang

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Figure 8

Molecular docking of HO-1 and STING.

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Molecular docking of HO-1 and STING. (A and B) The interaction of MYC-ta...
(A and B) The interaction of MYC-tagged full-length STING (aa 1–379), N-terminus of STING (aa 1–139), C-terminus of STING (aa 140–379) and Flag-tagged HO-1 in HEK293T cells was analyzed by immunoprecipitation. (C) View of binding modes between the STING dimer and the HO-1 dimer based on MD simulations. (D) The interaction of MYC-tagged full-length STING and Flag-tagged WT HO-1 or its mutants in HEK293T cells was analyzed by immunoprecipitation. (E) HEK293T cells were cotransfected with plasmids expressing STING and HO-1, or its mutants and stimulated or not with cGAMP, followed by native PAGE and SDS-PAGE. (B, D, and E) All representative data from 1 experiment are shown (n = 3 biologically independent experiments).