雷公藤红素通过靶向SHP2并上调MHC-I增强黑色素瘤中的CD8+T细胞免疫。
Celastrol enhanced CD8+T cell immunity in melanoma by targeting SHP2 and upregulating MHC-I.
作者信息
Kong Qing, Liu Suqing, He Shan, Luo Zhuyu, Lei Rui, Wang Ruilong, Liu Xiao, Wu Jinfeng
机构信息
Department of Dermatology, Huashan Hospital, Fudan University, Shanghai, China.
Department of Dermatology, Huashan Hospital, Fudan University, Shanghai, China.
出版信息
Phytomedicine. 2025 Jul;142:156731. doi: 10.1016/j.phymed.2025.156731. Epub 2025 Apr 14.
BACKGROUND
Celastrol (CEL) has demonstrated promising anti-cancer properties, yet its specific mechanisms against melanoma remain insufficient. This study investigated the CEL's anti-tumor effects and determined its potential mechanisms in the regulation of MHC-I expression in melanoma. In addition, we also tested its efficacy in sensitizing immune checkpoint inhibitors (ICIs) to melanoma.
METHODS
CEL's anti-tumor activity was evaluated in B16F10 melanoma-bearing C57BL/6 mice across five groups (control, CEL 0.5 mg/kg, CEL 1 mg/kg, CEL 2 mg/kg, and ICIs), the tumor volume, histopathology, and body weight were assessed. Mechanistic insights were obtained through network pharmacology and RNA sequencing in B16F10 cells. Differential gene and pathway analysis were validated using qRT-PCR, Western blotting, and flow cytometry. CD8+T cell activation and cytotoxicity were analyzed in co-culture with CEL-pretreated B16F10 cells using flow cytometry and ELISA. CEL's interaction with potential targets was determined by molecular docking, surface plasmon resonance (SPR), and siRNA. The synergistic effect of CEL combined with ICIs was confirmed in B16F10-bearing C57BL/6 mice, and tumor-infiltrating T cells were assessed by flow cytometry across four groups (control, CEL, ICIs, CEL+ICIs).
RESULTS
CEL exhibited a significant anti-tumor effect in B16F10 melanoma-bearing mice. Mechanistically, CEL-pretreated B16F10 cells notably enhanced CD8+T cell activation and promoted IFNγ and TNFα secretion, leading to B16F10 cell death. CEL upregulated MHC-I expression through activation of the JAK/STAT1 pathway in B16F10 cells. The binding assay revealed that CEL interacted with SHP2, with an affinity of 37.93 μM. When SHP2 was silenced in B16F10 cells by siRNA, CEL failed to induce MHC-I upregulation. Moreover, CEL combined with ICIs produced superior antitumor efficacy compared to ICIs alone, which was accompanied by increased CD8+T cell infiltration in melanoma.
CONCLUSION
CEL enhanced CD8+T cell immunity by upregulating MHC-I expression in melanoma cells, these effects were at least partially through targeting SHP2 and activating JAK/STAT1 pathway. CEL might be a novel sensitizer for ICIs in melanoma.
背景
雷公藤红素(CEL)已显示出有前景的抗癌特性,但其针对黑色素瘤的具体机制仍不充分。本研究调查了CEL的抗肿瘤作用,并确定其在调节黑色素瘤中MHC-I表达的潜在机制。此外,我们还测试了其使免疫检查点抑制剂(ICI)对黑色素瘤敏感的功效。
方法
在携带B16F10黑色素瘤的C57BL/6小鼠中评估CEL的抗肿瘤活性,分为五组(对照组、0.5mg/kg CEL组、1mg/kg CEL组、2mg/kg CEL组和ICI组),评估肿瘤体积、组织病理学和体重。通过网络药理学和对B16F10细胞进行RNA测序获得机制方面的见解。使用qRT-PCR、蛋白质印迹法和流式细胞术验证差异基因和通路分析。使用流式细胞术和酶联免疫吸附测定法分析与经CEL预处理的B16F10细胞共培养时CD8+T细胞的活化和细胞毒性。通过分子对接、表面等离子体共振(SPR)和小干扰RNA(siRNA)确定CEL与潜在靶点的相互作用。在携带B16F10的C57BL/6小鼠中证实了CEL与ICI联合使用的协同效应,并通过流式细胞术对四组(对照组、CEL组、ICI组、CEL+ICI组)的肿瘤浸润T细胞进行评估。
结果
CEL在携带B16F10黑色素瘤的小鼠中表现出显著的抗肿瘤作用。机制上,经CEL预处理的B16F10细胞显著增强了CD8+T细胞的活化,并促进了IFNγ和TNFα的分泌,导致B16F10细胞死亡。CEL通过激活B16F10细胞中的JAK/STAT1通路上调MHC-I的表达。结合试验表明CEL与SHP2相互作用,亲和力为37.93μM。当通过siRNA使B16F10细胞中的SHP-2沉默时,CEL未能诱导MHC-I上调。此外,与单独使用ICI相比,CEL与ICI联合使用产生了更好的抗肿瘤效果,同时黑色素瘤中CD8+T细胞浸润增加。
结论
CEL通过上调黑色素瘤细胞中MHC-I的表达增强CD8+T细胞免疫,这些作用至少部分是通过靶向SHP2并激活JAK/STAT1通路实现的。CEL可能是黑色素瘤中ICI的一种新型增敏剂。
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