TAB1——基于蛋白质组学的卵巢癌紫杉醇耐药的潜在生物标志物探讨  被引量：1

作　　者：丁亚伟 陈君君 张湘奇[3] 张葳 周丽 孔欠文 石美智 姜波 周阳云 汪晓河 许剑锋[1,2] 韩永龙 杨姣[3] DING Ya-wei;CHEN Jun-jun;ZHANG Xiang-qi;ZHANG Wei;ZHOU Li;KONG Qian-wen;SHI Mei-zhi;JIANG Bo;ZHOU Yang-yun;WANG Xiao-he;XU Jian-feng;HAN Yong-long;YANG Jiao(College of Food Science and Technology,Shanghai Ocean University,Shanghai 201306,China;Laboratory of Quality and Safety Risk Assessment for Aquatic Product on Storage and Preservation(Shanghai),Ministry of Agriculture,Shanghai 201306,China;Shanghai Jiao Tong University Affiliated Sixth People's Hospital,Shanghai 200233,China)

机构地区：[1]上海海洋大学食品学院,上海201306 [2]农业部水产品贮藏保鲜质量安全风险评估实验室,上海201306 [3]上海交通大学附属第六人民医院,上海200233

出　　处：《中国实验方剂学杂志》2021年第8期168-178,共11页Chinese Journal of Experimental Traditional Medical Formulae

基　　金：国家自然科学基金项目(81773949,82003987);上海市自然科学基金项目(20ZR1442400);上海市卫生和计划生育委员会中医药科研课题(2018YP003);上海市浦东新区科技发展基金民生科研专项资金项目(PKJ2020-Y08);上海市第六人民医院医疗集团课题;中国药学会全国医药经济信息网科技传播创新工程(CME12019KPYJ00421)。

摘　　要：目的:探究卵巢癌对紫杉醇(PTX)耐药的潜在靶点及其相关机制。方法:体外培养卵巢癌A2780细胞和A2780PTX耐药细胞(A2780/T),采用不同浓度(2,4,8,16,32,64,128,256μmol·L^(-1))PTX分别干预24 h或48 h,噻唑蓝(MTT)比色法检测PTX对A2780细胞和A2780/T细胞存活率的影响,利用液相色谱质谱/质谱(LC-MS/MS)非标记(Label-Free)定量蛋白质组学方法鉴定和筛选两组细胞中表达差异的蛋白,通过基因本体(GO)注释和京都基因与基因组百科全书(KEGG)通路分析,筛选卵巢癌细胞对PTX耐药的潜在生物标志物。以正常培养的A2780细胞作为空白组,采用0,1,4μmol·L^(-1)的PTX处理A2780/T细胞,采用实时荧光定量聚合酶链式反应(Real-time PCR)和蛋白免疫印迹法(Western blot)检测验证潜在靶点转化生长因子-β活化激酶1结合蛋白1(TAB1)及其下游相关分子转化生长因子-β活化激酶1(TAK1),p38有丝分裂活化蛋白酶(MAPK)mRNA和蛋白的表达水平。结果:与空白组比较,PTX干预组的A2780和A2780/T细胞的活力均降低。PTX对A2780细胞的抑制率明显高于A2780/T细胞。A2780细胞中,PTX处理48 h的半抑制浓度(IC50)为0.002μmol·L^(-1),A2780/T细胞中,PTX的IC50>设置的最高浓度128μmol·L^(-1),与A2780细胞相比,A2780/T细胞对PTX具有耐药性。通过非标记定量蛋白质组学分析筛选出A2780/T和A2780细胞之间有441种差异表达蛋白和421种特殊差异表达蛋白。GO功能富集分析显示,在差异表达的蛋白质中,结合蛋白占大多数(80%)。根据KEGG通路分析结果和表达位点分析,TAB1被认为可能是卵巢癌对PTX耐药的潜在生物标志物。与A2780细胞比较,A2780/T细胞的TAB1 mRNA和蛋白表达显著降低(P<0.01),与TAB1相互作用的TAK1 mRNA和p38 MAPK mRNA亦明显降低(P<0.05,P<0.01),但蛋白表达无显著变化。结论:TAB1可能是卵巢癌对PTX耐药的潜在生物标志物,其机制可能与TAB1/TAK1/p38 MAPK通路有关。Objective: To explore the potential targets and related mechanism involved in the paclitaxel resistance to ovarian cancer. Method: Ovarian cancer A2780 cells and A2780 paclitaxel-resistant cells(A2780/T)were treated by 2,4,8,16,32,64,128,256 μmol·L^(-1) paclitaxel(PTX)for 24 h or 48 h respectively in vitro. The proliferation rate of A2780 cells and A2780/T cells treated with paclitaxel was determined by methyl thiazolyl tetrazolium(MTT)colorimetric method assay. A2780 and A2780/T cells were analyzed by LC-MS/MS Label-Free quantitative proteomics to identify and screen differentially expressed proteins in the two groups of cells. Gene ontology(GO)annotation and Kyoto encyclopedia of genes and genomes(KEGG)pathway analysis were used to determine the potential biomarkers of paclitaxel resistance in ovarian cancer. Conventionally cultured A2780 cells were used as a control group,and A2780/T cells were treated with 0,1,4 μmol·L^(-1) PTX. Real-time fluorescence quantitative polymerase chain reaction(Real-time PCR)and Western blot methods were used to detect and verify the m RNA and protein expression levels of potential target transforming growth factor-β-activated kinase 1 binding protein 1(TAB1)and its downstream related molecules transforming growth factor-β-activated kinase(TAK1)and p38. Result:After PTX treatment for 24 h and 48 h,the cell viability of A2780 and A2780/T cells decreased. The inhibitory rate of PTX on A2780 cells was significantly higher than that of A2780/T cells. In A2780 cells,the IC50 of PTX treatment for 48 h was0.002 μmol·L^(-1),while in A2780/T cells,the IC50 of PTX was greater than the maximum concentration of 128μmol·L^(-1),indicating that A2780/T cells were resistant to PTX compared with A2780 cells. 441 differentially expressed proteins and 421 special differentially expressed proteins between A2780/T and A2780 cells were screened by label-free quantitative proteomic analysis. GO function enrichment analysis showed that the binding proteins accounted for the majority(80%)among t

关 键 词：转化生长因子-β活化激酶1结合蛋白1(TAB1) 卵巢癌 紫杉醇耐药 非标记定量蛋白组学 生物信息学 

分 类 号：R2-0[医药卫生—中医学] R22