首页|期刊导航|陆军军医大学学报|E3泛素连接酶FBXL8通过泛素化降解p53促进肝内胆管细胞癌恶性进展

E3泛素连接酶FBXL8通过泛素化降解p53促进肝内胆管细胞癌恶性进展OA

E3 ubiquitin ligase FBXL8 promotes malignant progression of intrahepatic cholangiocarcinoma by ubiquitination-mediated degradation of p53

中文摘要英文摘要

目的 肝内胆管细胞癌(intrahepatic cholangiocarcinoma,ICC)侵袭性强、预后极差,现有靶向治疗靶点匮乏.泛素化修饰失调是肿瘤发生发展的重要机制,E3泛素连接酶FBXL8在肿瘤中呈组织特异性功能,但其在ICC中的表达特征、临床价值及分子机制尚未明确.本研究旨在系统探讨FBXL8在ICC中的表达特征,分析其与临床病理指标的相关性,明确FBXL8对ICC细胞生物学行为的影响并阐明其潜在分子机制,为ICC的预后评估及分子靶向治疗提供新的科学依据和潜在靶点.方法 采用生物信息学方法分析TCGA、GEO数据库中FBXL8在ICC组织及癌旁正常组织中的表达差异;收集79例ICC患者癌组织及配对癌旁正常组织芯片,通过免疫组织化学染色检测FBXL8蛋白表达,依据染色综合评分将患者分为高表达组(n=44)和低表达组(n=35),采用Pearson x2检验分析FBXL8表达与临床病理特征的相关性,Kaplan-Meier法联合Log-rank检验进行生存分析.在人ICC细胞系RBE和SNU-1079中,通过2条靶向Fbxl8的siRNA(siFbxl8#1组、siFbxl8#2组)下调其表达,CCK-8法检测细胞增殖活性,Transwell实验评估细胞迁移能力;通过UbiBrowser数据库预测FBXL8潜在底物蛋白,免疫共沉淀(Co-immunoprecipitation,Co-IP)实验验证FBXL8与候选底物的相互作用,Western blotting检测蛋白酶体抑制剂MG132干预后底物蛋白的表达变化,体内泛素化实验明确FBXL8对底物蛋白的泛素化修饰作用.结果 生物信息学分析显示,TCGA数据库中ICC组织(n=35)FBXL8表达水平显著高于癌旁正常组织(n=9,t=13.57,P<0.001);GEO数据库中GSE26566(ICC:n=104、癌旁:n=59)和GSE107943(ICC:n=30、癌旁:n=27)2个数据集也证实上述结果(t=3.47,P<0.001;t=8.74,P<0.001).免疫组织化学染色结果显示,ICC组织FBXL8蛋白阳性表达率及染色强度显著高于癌旁正常组织.临床病理分析显示,FBXL8高表达与ICC患者肿瘤体积≥ 3 cm(x2=16.528,P<0.001)、淋巴结转移(x2=4.090,P=0.043)、TNM Ⅲ~Ⅳ期(x2=11.446,P<0.001)、肿瘤低分化(x2=26.404,P<0.001)显著相关,与性别、年龄、血管和神经侵犯无显著相关性.生存分析结果显示,FBXL8高表达组患者总生存期显著短于低表达组(x2=19.47,P<0.001).细胞功能实验显示,siRNA有效沉默RBE细胞中FBXL8表达后,RBE细胞[OD(450)]值显著降低[吸光度值由对照组的(1.15±0.05)减少到siFbxl8#1组的(0.73±0.04,q=19.42,P<0.001)和siFbxl8#2组的(0.70±0.04,q=23.69,P<0.001)],RBE细胞迁移数量显著减少[穿孔数量从对照组的(899.67±85.13)减少到 siFbxl8#1 组的(344.00±67.02,q=7.46,P<0.05)和 siFbxl8#2 组的(355.00±51.00,q=27.49,P<0.01)],在SNU-1079细胞中沉默FBXL8的表达也发现同样的现象.机制研究显示,p53为FBXL8评分最高的潜在底物,Co-IP实验证实二者存在内源性相互作用;过表达FBXL8可降低p53蛋白水平,加入MG132后该降解作用被阻断,p53蛋白水平回升;体内泛素化实验证实,过表达FBXL8可增强p53的泛素化修饰水平.结论 FBXL8在ICC组织中呈高表达,其高表达与ICC患者肿瘤体积增大、淋巴结转移、高TNM分期、低分化等不良临床病理特征密切相关,是ICC患者不良预后的潜在标志物;FBXL8可通过泛素-蛋白酶体途径泛素化降解p53蛋白,进而促进ICC细胞的增殖与迁移,推动ICC恶性进展.因此,FBXL8可作为ICC分子靶向治疗的潜在靶点,为ICC的精准治疗提供新的方向.

Objective Intrahepatic cholangiocarcinoma(ICC)is characterized by high invasiveness and extremely poor prognosis,and till now,its effective molecular targets for targeted therapy remain scarce.Dysregulation of ubiquitination modification is a crucial mechanism underlying tumorigenesis and progression.E3 ubiquitin ligase FBXL8 exerts tissue-specific functions in tumors,yet its expression profile,clinical value and molecular mechanisms in ICC remain unclear.This study aims to systematically investigate the expression characteristics of FBXL8 in ICC,analyze its correlation with clinicopathological parameters,clarify its regulatory effects on the biological behaviors of ICC cells and elucidate its potential molecular mechanisms,thereby providing novel scientific evidence and potential targets for prognostic evaluation and molecular targeted therapy of ICC.Methods Bioinformatic analysis was performed to examine the differential expression of FBXL8 in ICC tissues and adjacent normal tissues based on the TCGA and GEO databases.Tissue microarrays containing cancerous tissues and paired adjacent normal tissues from 79 ICC patients were collected,and immunohistochemical staining was applied to detect the protein expression of FBXL8.According to the results,the patients were divided into a high-expression group(n=44)and a low-expression group(n=35).Pearson x2 test was used to analyze the correlation between FBXL8 expression and clinicopathological features,and Kaplan-Meier test and Log-rank test were employed for survival analysis.In human ICC cell lines RBE and SNU-1079,2 Fbxl8-targeted siRNAs(siFbxl8#1 and siFbxl8#2)were transfected to downregulate FBXL8 expression.CCK-8 assay was conducted to measure cell proliferative activity,and Transwell assay was carried out to evaluate cell migratory ability.The UbiBrowser database was used to predict potential substrate proteins of FBXL8.Co-immunoprecipitation(Co-IP)was conducted to verify the interaction between FBXL8 and candidate substrates.Western blotting was used to detect the changes in substrate protein expression after intervention with the proteasome inhibitor MG 132,and in vivo ubiquitination assay was performed to confirm the regulatory effect of FBXL8 on the ubiquitination modification of substrate proteins.Results Bioinformatic analysis showed that the expression level of FBXL8 was significantly higher in ICC tissues(n=35)than in adjacent normal tissues(n=9)in the TCGA database(t=13.57,P<0.001).Two datasets from the GEO database,GSE26566(ICC:n=104,adjacent:n=59)and GSE107943(ICC:n=30,adjacent:n=27),further validated the above results(t=3.47,P<0.001;t=8.74,P<0.001).Immunohistochemical staining revealed that both the positive expression rate and staining intensity of FBXL8 protein were markedly elevated in ICC tissues compared with adjacent normal tissues.Clinicopathological analysis indicated that high FBXL8 expression was significantly correlated with tumor diameter ≥ 3 cm(x2=16.528,P<0.001),lymph node metastasis(x2=4.090,P=0.043),TNM stage Ⅲ-Ⅳ(x2=11.446,P<0.001)and poor tumor differentiation(x2=26.404,P<0.001),whereas no significant correlation was observed with gender,age,or vascular and perineural invasion.Survival analysis demonstrated that the patients with high FBXL8 expression had a significantly shorter overall survival than those with low expression(x2=19.47,P<0.001).Cell functional experiments showed that effective silencing of FBXL8 expression in RBE cells by siRNA significantly reduced the[OD(450)]value,and the absorbance value was decreased from 1.15±0.05 in the control group to 0.73±0.04 in the siFbxl8#1 group(q=19.42,P<0.001)and 0.70±0.04 in the siFbxl8#2 group(q=23.69,P<0.001).The number of migrated RBE cells was also remarkably reduced,decreasing from 899.67±85.13 in the control group to 344.00±67.02 in the siFbxl8#1 group(q=7.46,P<0.05)and 355.00±51.00 in the siFbxl8#2 group(q=27.49,P<0.01).Consistent results were observed after FBXL8 silencing in SNU-1079 cells.Mechanistically,p53 was identified as the top-ranked potential substrate of FBXL8.Co-IP assay confirmed the endogenous interaction between FBXL8 and p53.FBXL8 overexpression reduced p53 protein level,while such degradation was blocked after the addition of MG132,with p53 protein levels recovering.In vivo ubiquitination assay further verified that FBXL8 overexpression enhanced the ubiquitination level of p53.Conclusion FBXL8 is highly expressed in ICC tissues,and its high expression is closely associated with adverse clinicopathological characteristics of ICC patients,including increased tumor volume,lymph node metastasis,advanced TNM stage and poor differentiation,serving as a potential biomarker for poor prognosis in the patients.FBXL8 promotes the proliferation and migration of ICC cells and drives the malignant progression by ubiquitinating and degrading p53 protein through the ubiquitin-proteasome pathway.Therefore,FBXL8 may be regarded as a potential target for molecular targeted therapy of ICC,providing a new direction for precision treatment of the disease.

罗清;李春明;钟国超;龚建平

重庆医科大学附属第二医院肝胆外科,重庆重庆医科大学附属第二医院肝胆外科,重庆重庆医科大学附属第二医院肝胆外科,重庆重庆医科大学附属第二医院肝胆外科,重庆

医药卫生

E3泛素连接酶FBXL8肝内胆管细胞癌泛素化

E3 ubiquitin ligaseFBXL8intrahepatic cholangiocarcinomaubiquitination

《陆军军医大学学报》 2026 (11)

1496-1504,9

重庆市自然科学基金面上项目(CSTB2024NSCQ-MSX0285)国家自然科学基金青年项目(82203391) Supported by the General Project of Natural Science Foundation of Chongqing(CSTB2024NSCQ-MSX0285)and the National Natural Science Foundation for Young Scholars of China(82203391).

10.16016/j.2097-0927.202601015

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