Verteporfin inhibits PD-L1 through autophagy and the STAT1-IRF1-TRIM28 signaling axis, exerting antitumor efficacy

Jiyong Liang; Lulu Wang; Chao Wang; Jianfeng Shen; Bojin Su; Anantha L. Marisetty; Dexing Fang; Cynthia Kassab; Kang Jin Jeong; Wei Zhao; Yiling Lu; Abhinav K. Jain; Zhicheng Zhou; Han Liang; Shao Cong Sun; Changming Lu; Zhi Xiang Xu; Qinghua Yu; Shan Shao; Xiao Hua Chen; Meng Gao; Francois X. Claret; Zhiyong Ding; Jian Chen; Pingsheng Chen; Michelle C. Barton; Guang Peng; Gordon B. Mills; Amy B. Heimberger

doi:10.1158/2326-6066.CIR-19-0159

Verteporfin inhibits PD-L1 through autophagy and the STAT1-IRF1-TRIM28 signaling axis, exerting antitumor efficacy

Jiyong Liang, Lulu Wang, Chao Wang, Jianfeng Shen, Bojin Su, Anantha L. Marisetty, Dexing Fang, Cynthia Kassab, Kang Jin Jeong, Wei Zhao, Yiling Lu, Abhinav K. Jain, Zhicheng Zhou, Han Liang, Shao Cong Sun, Changming Lu, Zhi Xiang Xu, Qinghua Yu, Shan Shao, Xiao Hua ChenMeng Gao, Francois X. Claret, Zhiyong Ding, Jian Chen, Pingsheng Chen, Michelle C. Barton, Guang Peng, Gordon B. Mills, Amy B. Heimberger^*

^*Corresponding author for this work

Research output: Contribution to journal › Article › peer-review

51 Scopus citations

Abstract

Programmed cell death 1 ligand 1 (PD-L1) is a key driver of tumor-mediated immune suppression, and targeting it with antibodies can induce therapeutic responses. Given the costs and associated toxicity of PD-L1 blockade, alternative therapeutic strategies are needed. Using reverse-phase protein arrays to assess drugs in use or likely to enter trials, we performed a candidate drug screen for inhibitors of PD-L1 expression and identified verteporfin as a possible small-molecule inhibitor. Verteporfin suppressed basal and IFN-induced PD-L1 expression in vitro and in vivo through Golgi-related autophagy and disruption of the STAT1-IRF1-TRIM28 signaling cascade, but did not affect the proinflammatory CIITA-MHC II cascade. Within the tumor microenvironment, verteporfin inhibited PD-L1 expression, which associated with enhanced T-lymphocyte infiltration. Inhibition of chromatin-associated enzyme PARP1 induced PD-L1 expression in high endothelial venules (HEV) in tumors and, when combined with verteporfin, enhanced therapeutic efficacy. Thus, verteporfin effectively targets PD-L1 through transcriptional and posttranslational mechanisms, representing an alternative therapeutic strategy for targeting PD-L1.

Original language	English (US)
Pages (from-to)	952-965
Number of pages	14
Journal	Cancer Immunology Research
Volume	8
Issue number	7
DOIs	https://doi.org/10.1158/2326-6066.CIR-19-0159
State	Published - Jul 1 2020
Externally published	Yes

ASJC Scopus subject areas

Immunology
Cancer Research

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

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10.1158/2326-6066.CIR-19-0159

Cite this

Liang, J., Wang, L., Wang, C., Shen, J., Su, B., Marisetty, A. L., Fang, D., Kassab, C., Jeong, K. J., Zhao, W., Lu, Y., Jain, A. K., Zhou, Z., Liang, H., Sun, S. C., Lu, C., Xu, Z. X., Yu, Q., Shao, S., ... Heimberger, A. B. (2020). Verteporfin inhibits PD-L1 through autophagy and the STAT1-IRF1-TRIM28 signaling axis, exerting antitumor efficacy. Cancer Immunology Research, 8(7), 952-965. https://doi.org/10.1158/2326-6066.CIR-19-0159

@article{4ae51e69b16348a7bb0c4750418b8022,

title = "Verteporfin inhibits PD-L1 through autophagy and the STAT1-IRF1-TRIM28 signaling axis, exerting antitumor efficacy",

abstract = "Programmed cell death 1 ligand 1 (PD-L1) is a key driver of tumor-mediated immune suppression, and targeting it with antibodies can induce therapeutic responses. Given the costs and associated toxicity of PD-L1 blockade, alternative therapeutic strategies are needed. Using reverse-phase protein arrays to assess drugs in use or likely to enter trials, we performed a candidate drug screen for inhibitors of PD-L1 expression and identified verteporfin as a possible small-molecule inhibitor. Verteporfin suppressed basal and IFN-induced PD-L1 expression in vitro and in vivo through Golgi-related autophagy and disruption of the STAT1-IRF1-TRIM28 signaling cascade, but did not affect the proinflammatory CIITA-MHC II cascade. Within the tumor microenvironment, verteporfin inhibited PD-L1 expression, which associated with enhanced T-lymphocyte infiltration. Inhibition of chromatin-associated enzyme PARP1 induced PD-L1 expression in high endothelial venules (HEV) in tumors and, when combined with verteporfin, enhanced therapeutic efficacy. Thus, verteporfin effectively targets PD-L1 through transcriptional and posttranslational mechanisms, representing an alternative therapeutic strategy for targeting PD-L1.",

author = "Jiyong Liang and Lulu Wang and Chao Wang and Jianfeng Shen and Bojin Su and Marisetty, {Anantha L.} and Dexing Fang and Cynthia Kassab and Jeong, {Kang Jin} and Wei Zhao and Yiling Lu and Jain, {Abhinav K.} and Zhicheng Zhou and Han Liang and Sun, {Shao Cong} and Changming Lu and Xu, {Zhi Xiang} and Qinghua Yu and Shan Shao and Chen, {Xiao Hua} and Meng Gao and Claret, {Francois X.} and Zhiyong Ding and Jian Chen and Pingsheng Chen and Barton, {Michelle C.} and Guang Peng and Mills, {Gordon B.} and Heimberger, {Amy B.}",

note = "Funding Information: The authors thank Kenneth Dunner Jr at the High Resolution Electron Microscopy Facility for assistance in performing electron microscopy; David M. Wildrick, PhD, for editorial assistance; and Audria Patrick for assisting in manuscript preparation. This project was supported by the Gynecologic SPORE (5P50CA098258, NIH/NCI; to G.B. Mills), the Provost Retention Fund and the Brockman Foundation (to A.B. Heimberger), and the Shanghai Pujiang Program (17PJ1401400; to C. Wang). This research was performed in the Flow Cytometry & Cellular Imaging Facility, which is supported in part by the NIH through MD Anderson's Cancer Center Support Grant CA016672. Funding Information: The authors thank Kenneth Dunner Jr at the High Resolution Electron Microscopy Facility for assistance in performing electron microscopy; David M. Wildrick, PhD, for editorial assistance; and Audria Patrick for assisting in manuscript preparation. This project was supported by the Gynecologic SPORE (5P50CA098258, NIH/NCI; to G.B. Mills), the Provost Retention Fund and the Publisher Copyright: {\textcopyright} 2020 American Association for Cancer Research.",

year = "2020",

month = jul,

day = "1",

doi = "10.1158/2326-6066.CIR-19-0159",

language = "English (US)",

volume = "8",

pages = "952--965",

journal = "Cancer immunology research",

issn = "2326-6066",

publisher = "American Association for Cancer Research Inc.",

number = "7",

}

Liang, J, Wang, L, Wang, C, Shen, J, Su, B, Marisetty, AL, Fang, D, Kassab, C, Jeong, KJ, Zhao, W, Lu, Y, Jain, AK, Zhou, Z, Liang, H, Sun, SC, Lu, C, Xu, ZX, Yu, Q, Shao, S, Chen, XH, Gao, M, Claret, FX, Ding, Z, Chen, J, Chen, P, Barton, MC, Peng, G, Mills, GB & Heimberger, AB 2020, 'Verteporfin inhibits PD-L1 through autophagy and the STAT1-IRF1-TRIM28 signaling axis, exerting antitumor efficacy', Cancer Immunology Research, vol. 8, no. 7, pp. 952-965. https://doi.org/10.1158/2326-6066.CIR-19-0159

TY - JOUR

T1 - Verteporfin inhibits PD-L1 through autophagy and the STAT1-IRF1-TRIM28 signaling axis, exerting antitumor efficacy

AU - Liang, Jiyong

AU - Wang, Lulu

AU - Wang, Chao

AU - Shen, Jianfeng

AU - Su, Bojin

AU - Marisetty, Anantha L.

AU - Fang, Dexing

AU - Kassab, Cynthia

AU - Jeong, Kang Jin

AU - Zhao, Wei

AU - Lu, Yiling

AU - Jain, Abhinav K.

AU - Zhou, Zhicheng

AU - Liang, Han

AU - Sun, Shao Cong

AU - Lu, Changming

AU - Xu, Zhi Xiang

AU - Yu, Qinghua

AU - Shao, Shan

AU - Chen, Xiao Hua

AU - Gao, Meng

AU - Claret, Francois X.

AU - Ding, Zhiyong

AU - Chen, Jian

AU - Chen, Pingsheng

AU - Barton, Michelle C.

AU - Peng, Guang

AU - Mills, Gordon B.

AU - Heimberger, Amy B.

N1 - Funding Information: The authors thank Kenneth Dunner Jr at the High Resolution Electron Microscopy Facility for assistance in performing electron microscopy; David M. Wildrick, PhD, for editorial assistance; and Audria Patrick for assisting in manuscript preparation. This project was supported by the Gynecologic SPORE (5P50CA098258, NIH/NCI; to G.B. Mills), the Provost Retention Fund and the Brockman Foundation (to A.B. Heimberger), and the Shanghai Pujiang Program (17PJ1401400; to C. Wang). This research was performed in the Flow Cytometry & Cellular Imaging Facility, which is supported in part by the NIH through MD Anderson's Cancer Center Support Grant CA016672. Funding Information: The authors thank Kenneth Dunner Jr at the High Resolution Electron Microscopy Facility for assistance in performing electron microscopy; David M. Wildrick, PhD, for editorial assistance; and Audria Patrick for assisting in manuscript preparation. This project was supported by the Gynecologic SPORE (5P50CA098258, NIH/NCI; to G.B. Mills), the Provost Retention Fund and the Publisher Copyright: © 2020 American Association for Cancer Research.

PY - 2020/7/1

Y1 - 2020/7/1

N2 - Programmed cell death 1 ligand 1 (PD-L1) is a key driver of tumor-mediated immune suppression, and targeting it with antibodies can induce therapeutic responses. Given the costs and associated toxicity of PD-L1 blockade, alternative therapeutic strategies are needed. Using reverse-phase protein arrays to assess drugs in use or likely to enter trials, we performed a candidate drug screen for inhibitors of PD-L1 expression and identified verteporfin as a possible small-molecule inhibitor. Verteporfin suppressed basal and IFN-induced PD-L1 expression in vitro and in vivo through Golgi-related autophagy and disruption of the STAT1-IRF1-TRIM28 signaling cascade, but did not affect the proinflammatory CIITA-MHC II cascade. Within the tumor microenvironment, verteporfin inhibited PD-L1 expression, which associated with enhanced T-lymphocyte infiltration. Inhibition of chromatin-associated enzyme PARP1 induced PD-L1 expression in high endothelial venules (HEV) in tumors and, when combined with verteporfin, enhanced therapeutic efficacy. Thus, verteporfin effectively targets PD-L1 through transcriptional and posttranslational mechanisms, representing an alternative therapeutic strategy for targeting PD-L1.

AB - Programmed cell death 1 ligand 1 (PD-L1) is a key driver of tumor-mediated immune suppression, and targeting it with antibodies can induce therapeutic responses. Given the costs and associated toxicity of PD-L1 blockade, alternative therapeutic strategies are needed. Using reverse-phase protein arrays to assess drugs in use or likely to enter trials, we performed a candidate drug screen for inhibitors of PD-L1 expression and identified verteporfin as a possible small-molecule inhibitor. Verteporfin suppressed basal and IFN-induced PD-L1 expression in vitro and in vivo through Golgi-related autophagy and disruption of the STAT1-IRF1-TRIM28 signaling cascade, but did not affect the proinflammatory CIITA-MHC II cascade. Within the tumor microenvironment, verteporfin inhibited PD-L1 expression, which associated with enhanced T-lymphocyte infiltration. Inhibition of chromatin-associated enzyme PARP1 induced PD-L1 expression in high endothelial venules (HEV) in tumors and, when combined with verteporfin, enhanced therapeutic efficacy. Thus, verteporfin effectively targets PD-L1 through transcriptional and posttranslational mechanisms, representing an alternative therapeutic strategy for targeting PD-L1.

UR - http://www.scopus.com/inward/record.url?scp=85087469654&partnerID=8YFLogxK

UR - http://www.scopus.com/inward/citedby.url?scp=85087469654&partnerID=8YFLogxK

U2 - 10.1158/2326-6066.CIR-19-0159

DO - 10.1158/2326-6066.CIR-19-0159

M3 - Article

C2 - 32265228

AN - SCOPUS:85087469654

SN - 2326-6066

VL - 8

SP - 952

EP - 965

JO - Cancer immunology research

JF - Cancer immunology research

IS - 7

ER -

Verteporfin inhibits PD-L1 through autophagy and the STAT1-IRF1-TRIM28 signaling axis, exerting antitumor efficacy

Abstract

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UN SDGs

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