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吉马酮抑制JAK2/STAT3信号通路对食管癌细胞增殖、凋亡和侵袭的影响OACSTPCD

Influences of germacrone on proliferation,apoptosis and invasion of esophageal cancer cells by inhibiting JAK2/STAT3 signaling pathway

中文摘要英文摘要

目的 探讨吉马酮抑制蛋白酪氨酸激酶2(Janus kinase 2,JAK2)/信号转导子与激活子3(signal transducer and activator of transcription 3,STAT3)信号通路对食管癌细胞增殖、凋亡和侵袭的影响.方法 甲基噻唑蓝(methyl thiazolyl tetrazolium,MTT)法检测不同浓度(0、10、20、40、80、160和320 μmol/L)的吉马酮分别处理人食管癌细胞Eca109和KYSE450以及人食管上皮细胞Het-1A后的细胞存活率.将Eca109细胞分为对照组(常规培养)、吉马酮低剂量组(40μmol/L吉马酮干预24 h)、吉马酮中剂量组(80 μmol/L吉马酮干预24 h)、吉马酮高剂量组(160 μmol/L吉马酮干预24 h)、Coumermycin A1 组(10 μmol/L JAK2 激活剂 coumermycin A1+160 μmol/L 吉马酮干预 24 h)和 AG490 组(50 μmol/L JAK2 抑制剂AG490+160 μmol/L吉马酮干预24 h).Transwell检测细胞迁移和侵袭能力.平板克隆实验检测细胞克隆能力.流式细胞术检测细胞凋亡和周期.Western blot 检测 JAK2、磷酸化 JAK2(phos-JAK2,p-JAK2)、STAT3、p-STAT3、Ki-67、Bax、Bcl-2和p53表达情况.结果 与0μmol/L比较,10、20、40、80、160和320μmol/L的吉马酮处理下,Eca109和KYSE450细胞存活率均呈浓度依赖性降低(均P<0.05),半抑制浓度(half-inhibitory concentration,IC50)分别为(98.18±2.12)μmol/L和(154.77±2.32)μmol/L,而Het-1A细胞存活率差异无统计学意义(均P>0.05).由于吉马酮对Eea109细胞效果更明显,后续选择Eea109细胞并采用40、80和160 μmol/L吉马酮浓度进行作用机制研究.与对照组比较,吉马酮低、中和高剂量组Eca109细胞迁移、侵袭、克隆个数以及p-JAK2、p-STAT3、Ki-67和Bcl-2蛋白表达均降低(均P<0.05),Eca109细胞G0/G1期比例、早期凋亡率和总凋亡率以及Bax和p53表达均升高(均P<0.05).与吉马酮高剂量组比较,Coumermycin A1组Eca109细胞迁移、侵袭、克隆个数以及p-JAK2、p-STAT3、Ki-67和Bcl-2蛋白表达均增加,Eca109细胞G0/G1期比例、早期凋亡率和总凋亡率以及Bax和p53表达均降低(均P<0.05);AG490组Eca109细胞迁移、侵袭、克隆个数以及p-JAK2、p-STAT3、Ki-67和Bcl-2表达均降低,Eca109细胞G0/G1期比例、早期凋亡率和总凋亡率以及Bax和p53表达均升高(均P<0.05).结论 吉马酮可通过抑制JAK2/STAT3通路抑制食管癌细胞的增殖和侵袭能力,并促进细胞凋亡.

Objective To investigate the influences of germacrone on the proliferation,apoptosis and invasion of esophageal cancer cells by inhibiting Janus kinase 2(JAK2)/signal transducer and activator of transcription 3(STAT3)signaling pathway.Methods Meth-yl thiazolyl tetrazolium(MTT)assay was used to detect the survival rates of esophageal cancer cells Eca109 and KYSE450 and human esophageal epithelial cells Het-1A treated with germacrone at different concentrations including 0,10,20,40,80,160,and 320 μmol/L,respectively.Eca109 cells were divided into control group(conventional culture),low-dose germacrone group(40 μmol/L germacrone inter-vention for 24 h),medium-dose germacrone group(80 μmol/L germacrone intervention for 24 h),high-dose germacrone group(160 μmol/L germacrone intervention for 24 h),Coumermycin A1 group(10 μmol/L JAK2 activator coumermycin A1+160 μmol/L germacrone intervention for 24 h),and AG490 group(50 μmol/L JAK2 inhibitor AG490+160 μmol/L germacrone intervention for 24 h).Transwell assay was used to detect the migration and invasion of cells.Plate cloning assay was used to test cell cloning ability.Flow cytometry was applied to detect apop-tosis and cell cycle.Western blot was applied to detect the expression of JAK2,phos-JAK2(p-JAK2),STAT3,p-STAT3,Ki-67,Bax,Bcl-2,and p53 proteins.Results Compared with 0 μmol/L,the survival rates of Eca109 and KYSE450 cells decreased in a concentration-de-pendent manner under treatment with 10,20,40,80,160,and 320 μmol/L germacrone(all P<0.05),and the half-inhibitory concentrations(IC50)were(98.18±2.12)μmol/L and(154.77±2.32)μmol/L,respectively,while there was no difference in the survival rate of Het-1 A cells treated with different concentrations of germacrone(all P>0.05).Due to the more significant effect of germacrone on Eca1 09 cells,sub-sequent studies on the mechanism were conducted on Eca109 cells with germacrone treatment at concentrations of 40,80,and 160 μmol/L.For Eca109 cells,compared with the control group,the migration and invasion of cells,number of clones,and the protein expressions of p-JAK2,p-STAT3,Ki-67 and Bel-2 in the low-,medium-and high-dose germacrone groups all decreased(all P<0.05),while the pro-portion of cells in the G0/G1 phase,early apoptosis rate,total apoptosis rate,and the protein expression of Bax and p53 all increased(all P<0.05).Compared with the high-dose germacrone group,the migration and invasion of cells,number of clones,and the protein expression of p-JAK2,p-STAT3,Ki-67 and Bcl-2 all increased in the Coumermycin A1 group,while the proportion of cells in the G0/G1 phase,early apoptosis rate,total apoptosis rate,and the protein expression of Bax and p53 all decreased(all P<0.05).Compared with the high-dose germacrone group,the migration and invasion of Eca109 cells,number of clones,and the protein expression of p-JAK2,p-STAT3,Ki-67 and Bcl-2 in the AG490 group reduced,while the proportion of cells in the G0/G1 phase,early apoptosis rate,total apoptosis rate,the pro-tein expression of Bax and p53 all increased(all P<0.05).Conclusions Germacrone can inhibit the proliferation and invasion of esopha-geal cancer cells and promote cell apoptosis by inhibiting the JAK2/STAT3 pathway.

马骏;刘倩;王孝彬

空军军医大学第二附属医院/唐都医院胸腔外科,陕西西安 710038

食管癌吉马酮JAK2/STAT3通路细胞增殖细胞凋亡细胞侵袭

esophageal cancergermacroneJAK2/STAT3 pathwaycell proliferationcell apoptosiscell invasion

《实用肿瘤杂志》 2024 (003)

228-235 / 8

陕西省重点研发计划项目(2022SF-230)

10.13267/j.cnki.syzlzz.2024.035

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