医学分子生物学杂志 ›› 2024, Vol. 21 ›› Issue (3): 231-238.doi: 10.3870/j.issn.1672-8009.2024.03.007

• 论著 • 上一篇    下一篇

芒柄花黄素通过 HNF4A 抑制食管癌细胞增殖迁移和侵袭 #br#

  

  1. 西安国际医学中心医院1胸外科,3呼吸科 西安市, 710075 2广州中医药大学中医科 广州市, 510006
  • 出版日期:2024-05-31 发布日期:2024-06-14
  • 基金资助:
    陕西省重点研发计划项目 (No. 2022SF-325)

Formononetin Inhibits Proliferation, Migration and Invasion of Esophageal Carcinoma Cells by HNF4A #br#

  1. 1Department of Thoracic Surgery,3Department of Respiratory, Xian International Medical Center Hospital, Xian, 710075, China 2Department of Traditional Chinese Medicine, Guangzhou University of Traditional Chinese Medicine, Guangzhou, 510006, China
  • Online:2024-05-31 Published:2024-06-14

摘要: 目的 分析芒柄花黄素 ( formononetin, FORM) 通过肝细胞核因子 4α ( hepatocyte nuclear factor4α, HNF4A) 抑制食管癌细胞增殖迁移和侵袭的机制方法 使用不同浓度的芒柄花黄素处理 EC109 KYSE510, 利用 CCK8 检测细胞相对存活率和细胞的增殖, 利用细胞克隆实验培养癌细胞, 并检测加入芒柄花黄素前后细胞克隆数量, 利用 Transwell 检测加入芒柄花黄素前后 EC109 KYSE510 细胞的迁移和侵袭裸鼠皮下注射肿瘤细胞, 加入芒柄花黄素, 观察移植瘤体积和重量变化, 并利用免疫组化检测移植瘤组织中 Ki67 蛋白表达采用蛋白质印迹法检测芒柄花黄素对 HNF4A 基因表达的影响构建稳定过表达HNF4A EC109 KYSE510 细胞系, 加入芒柄花黄素, 观察 HNF4A 的表达情况结果 加入芒柄花黄素后, EC109 KYSE510 的细胞相对存活率明显降低 (P< 0. 05), 0 μmol / L 芒柄花黄素作用比较, EC109细胞系在芒柄花黄素浓度≥ 150 μmol / L , 细胞相对存活率降低显著 (P< 0. 05), KYSE510 细胞系在芒柄花黄素浓度≥ 120 μmol / L , 细胞相对存活率降低显著 ( P< 0. 05); 芒柄花黄素组 EC109 KYSE510 增殖侵袭迁移的细胞数量均明显低于对照组 (P< 0. 05)。 移植瘤体积和重量明显低于对照组 (P< 0. 05), Ki67 蛋白表达明显低于对照组 (P< 0. 05)。 随着芒柄花黄素浓度越高作用时间越久, HNF4A 蛋白表达下调更为明显。 HNF4A 过表达可以恢复芒柄花黄素抑制的细胞增殖侵袭和迁移 (P< 0. 05)。 结论 芒柄花黄素通过 HNF4A 抑制食管癌细胞增殖迁移和侵袭

关键词: 芒柄花黄素, 食管癌细胞, 增殖, 侵袭, 迁移

Abstract: Objective To analyze the mechanism of formononetin on inhibiting the proliferation, migration and invasion of esophageal carcinoma (EC) cells by hepatocyte nuclear factor 4α(HNF4A). Methods It was concluded by network pharmacology analysis that HNF4A might beone of the targets of formononetin. The expression level of HNF4A was closely related to clinical phenotypes of EC. EC109 and KYSE510 were treated with different concentrations of formononetin. The relative survival rate of cells was detected by CCK8. The cells proliferation was detected by CCK-8. The cancer cells were cultured by cells cloning assay. The number of colony cells before and afterformononetin treatment was detected. The migration and invasion of EC109 and KYSE510 cells before and after formononetin treatment were detected by transwell assay. Nude mice were subcutaneously injected with tumor cells and treated with formononetin to observe the changes in volume andweight of xenograft tumors. The expression level of Ki67 protein in xenograft tissues was detected byimmunohistochemistry. The effect of formononetin on the expression of HNF4A gene were detected byWestern blotting. EC109 and KYSE510 cell lines with stable overexpression of HNF4A were constructed and treated with formononetin to observe the effect on the expression of HNF4A. Results After formononetin treatment, the relative survival rates of EC109 and KYSE510 cells were significantly decreased (P< 0. 05). Compared with that of cells without formononetin treatment, the relative survival rate of cells was significantly decreased after treated with formononetin (≥150 μmol / Lfor EC109 cell line, and ≥ 120 μmol / L for KYSE510 cell line) ( P < 0. 05). The proliferation,migration and invasion of EC109 and KYSE510 cells in the formononetin group was significantly decreased when compared with those in the control group (P< 0. 05). The volume and weight of xenograft tumors were significantly decreased in the formononetin group (P< 0. 05), and the expression level of Ki67 protein was significantly lower than that in the control group (P< 0. 05). The effect offormononetin on the down-regulation of HNF4A protein was dependent on the concentration and time of the treatment. HNF4A overexpression could promote cells proliferation, invasion and migrationwhich were inhibited by formononetin (P< 0. 05). Conclusion formononetin can inhibit the proliferation, migration and invasion of EC cells by regulation of HNF4A.

Key words: formononetin, esophageal carcinoma cell, proliferation, invasion, migration

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