Shi Zhemin, Liu Qi, Zhang Mengxia, Du Xiaoxiao, He Yifan, Zheng Lina, Hong Wei, Han Tao, Zhang Kun
Department of Histology and Developmental Biology, School of Basic Medical Sciences, Tianjin Medical University, No. 22 Qixiangtai Road, Tianjin, 300070, China.
Department of Hepatology and Gastroenterology, Tianjin Union Medical Center, Tianjin Medical University, Tianjin Union Medical Center Affiliated to Nankai University, No. 190 Jieyuan Road, Tianjin, 300121, China.
J Transl Med. 2025 Jun 6;23(1):632. doi: 10.1186/s12967-025-06619-8.
Given the rising prevalence of liver fibrosis, there is an urgent need to improve the effective diagnostic methods and treatment of liver fibrosis. Although GPCRs are involved in various physiological and pathological processes, however, the hepatic functions of GPR56 have rarely been explored. This study aims to investigate the role and underlying mechanisms of GPR56 in liver fibrosis.
The expression of GPR56 in carbon tetrachloride (CCl) and bile duct ligation (BDL) induced mouse liver fibrosis, as well as human fibrotic liver tissues, was assessed by western blot, qRT-PCR and immunohistochemistry. Then, WGCNA combined with GO enrichment analysis were employed to predict the functions of GPR56. Additionally, Gain- and loss-of-function models (in vitro and in vivo) were established to explore GPR56's function and the signaling pathways involved in liver fibrosis and hepatocyte pyroptosis.
GPR56 was upregulated in both human and mouse fibrotic liver tissues, as well as hepatocytes from CCl-induced liver fibrosis mice. ROC analysis showed high diagnostic accuracy for cirrhosis (AUC = 0.895, 95% CI: 0.783-1.000). Moreover, WGCNA and GO enrichment analysis speculated that GPR56 was involved in the inflammatory response and extracellular matrix (ECM) synthesis. In vivo assays revealed that hepatocyte-specific overexpression of GPR56 attenuated, while knockdown of GPR56 exacerbated NLRP3 inflammasome-mediated pyroptosis and liver fibrosis. In vitro experiments confirmed that GPR56 inhibited hepatocyte pyroptosis, leading to the inactivation of hepatic stellate cells (HSC). Mechanistic experiments further revealed that GPR56 attenuated hepatocyte pyroptosis via inhibiting the activation of NF-κB pathway.
Our study identify GPR56 as a suppressor of hepatocyte pyroptosis and liver fibrosis, underscoring its potential as a therapeutic and diagnostic target.
鉴于肝纤维化的患病率不断上升,迫切需要改进肝纤维化的有效诊断方法和治疗手段。尽管G蛋白偶联受体(GPCRs)参与各种生理和病理过程,然而,GPR56的肝脏功能却鲜有研究。本研究旨在探讨GPR56在肝纤维化中的作用及潜在机制。
通过蛋白质免疫印迹法、定量逆转录聚合酶链反应(qRT-PCR)和免疫组织化学法评估GPR56在四氯化碳(CCl)和胆管结扎(BDL)诱导的小鼠肝纤维化以及人纤维化肝组织中的表达。然后,采用加权基因共表达网络分析(WGCNA)结合基因本体(GO)富集分析来预测GPR56的功能。此外,建立功能获得和功能缺失模型(体外和体内)以探索GPR56在肝纤维化和肝细胞焦亡中的功能及相关信号通路。
GPR56在人和小鼠的纤维化肝组织以及CCl诱导的肝纤维化小鼠的肝细胞中均上调。受试者工作特征(ROC)分析显示其对肝硬化具有较高的诊断准确性(曲线下面积[AUC]=0.895,95%置信区间[CI]:0.783 - 1.000)。此外,WGCNA和GO富集分析推测GPR56参与炎症反应和细胞外基质(ECM)合成。体内实验表明,肝细胞特异性过表达GPR56可减轻肝纤维化,而敲低GPR56则会加剧NLRP3炎性小体介导的焦亡和肝纤维化。体外实验证实,GPR56抑制肝细胞焦亡,导致肝星状细胞(HSC)失活。机制实验进一步表明,GPR56通过抑制核因子κB(NF-κB)通路的激活来减轻肝细胞焦亡。
我们的研究确定GPR56为肝细胞焦亡和肝纤维化的抑制因子,突显了其作为治疗和诊断靶点的潜力。
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