Single-cell atlas of diverse immune populations in the advanced biliary tract cancer microenvironment

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作者
Xuebing Shi
Zhixuan Li
Renqi Yao
Qingbao Cheng
Wei Li
Rui Wu
Zhihua Xie
Yanjing Zhu
Xinyao Qiu
Shuai Yang
Tao Zhou
Ji Hu
Yangqianwen Zhang
Tong Wu
Yan Zhao
Yani Zhang
Jianmin Wu
Hongyang Wang
Xiaoqing Jiang
Lei Chen
机构
[1] Naval Medical University,Department I of Biliary Tract, Eastern Hepatobiliary Surgery Hospital
[2] Eastern Hepatobiliary Surgery Hospital,The International Cooperation Laboratory on Signal Transduction
[3] Medical Innovation Research Division and Fourth Medical Center of the Chinese PLA General Hospital,Translational Medicine Research Center
[4] the First Affiliated Hospital of Naval Medical University,Department of Burn Surgery
[5] Fudan University Shanghai Cancer Center,Department of Oncology
[6] Shanghai Medical College,Institute of Metabolism and Integrative Biology and School of Life Sciences
[7] Fudan University,undefined
[8] Fudan University,undefined
[9] National Center for Liver Cancer,undefined
[10] Key Laboratory on Signaling Regulation and Targeting Therapy of Liver Cancer,undefined
[11] Ministry of Education,undefined
[12] Shanghai Key Laboratory on Hepatobiliary Tumor Biology,undefined
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摘要
Immunotherapies have been explored in treating solid tumors, albeit with disparate clinical effects in distinct cancer types. Systematic interrogation of immune cells in the tumor microenvironment (TME) is vital to the prediction of immunotherapy response and the development of innovative immunotherapeutics. To comprehensively characterize the immune microenvironment in advanced biliary tract cancer (BTC), we utilized single-cell RNA sequencing in unselected viable cells from 16 matched samples, and identified nineteen cell subsets from a total of 45,851 cells, in which exhausted CD8+ T cells, macrophages, and dendritic cells (DCs) in BTC were shown to augment and communicate within the TME. Transcriptional profiles coupled with T cell receptor (TCR) sequences revealed that exhausted CD8+ T cells retained clonal expansion and high proliferation in the TME, and some of them highly expressed the endoplasmic reticulum stress (ER) response gene, XBP1, indicating the role of ER stress in remodeling TME. Functional assays demonstrated that XBP1 and common immune checkpoints (PD1, TIGIT) were significantly upregulated in CD8+ T cells cocultured within the TME of BTC cells (GBC-SD, HCCC-9810). When treating the coculture groups with the specific inhibitor of IRE1α-XBP1 (4μ8C), the downregulation of TIGIT was observed in the treatment group. Collectively, comprehensive transcriptome profiling provides deep insights into the immune atlas in advanced BTC, which might be instrumental in exploring innovative immunotherapy strategies.
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