实用医学杂志 ›› 2023, Vol. 39 ›› Issue (9): 1086-1091.doi: 10.3969/j.issn.1006⁃5725.2023.09.004

• 基础研究 • 上一篇    下一篇

低温缺氧/复氧后大鼠心肌成纤维细胞对心肌 H9c2细胞间通讯的影响 

佟睿1,2 高鸿3 安丽3 易菁3 曹莹4 蒙富雪5 吴学艳1 马艳燕1    

  1. 1 贵州医科大学麻醉学院(贵阳 550000);2 哈尔滨医科大学附属第六医院麻醉科(哈尔滨 150000);3 贵州 医科大学附属医院麻醉科(贵阳 550000);4 贵州医科大学附属金阳医院麻醉科(贵阳 550000);5 贵州医科 大学第三附属医院医学实验中心(贵州都匀 558000)

  • 出版日期:2023-05-10 发布日期:2023-05-10
  • 通讯作者: 高鸿 E⁃mail:anesth@qq.com
  • 基金资助:
    贵州省卫生健康委科学技术基金项目(编号:gzwkj2021⁃270,gzwkj2022⁃131) 

Effect of rat cardiac fibroblasts on H9c2 cardiomyocytes intercellular communication after hypothermia hypoxia/reoxygenation

TONG Rui* ,GAO Hong,AN Li,YI Jing,CAO Ying,MENG Fuxue,WU Xueyan,MA Yanyan.   

  1. School of Anesthesiology,Guizhou Medical University,Guiyang 550004,China;*Department of Anesthesi⁃ ology,the Sixth Affiliated Hospital of Harbin Medical University,Haerbin 150000,China

  • Online:2023-05-10 Published:2023-05-10
  • Contact: GAO Hong E⁃mail:anesth@qq.com

摘要:

目的 观察低温缺氧/复氧(hypothermia hypoxia/reoxygen,H/R)后大鼠心肌成纤维细胞(rat cardiac fibroblasts,RCFs)对心肌 H9c2 细胞间通讯的影响并探讨其可能机制。方法 将 RCFs 细胞与 H9c2 细胞以 2:1 数量比 Transwell 共培养后随机分为 6 组。其中 T+AngⅡ组及 H/R⁃T+AngⅡ组加入 1.5 nmol/L Ang Ⅱ,T+ARB 组及 H/R⁃T+ARB 组加入 1 nmol/L 缬沙坦。T 组、T+AngⅡ组及 T+ARB 组进行正常培养,H/R⁃T 组、H/R⁃T+AngⅡ及 H/R⁃T+ARB 组进行 H/R 处理。检测各组培养液中 AngⅡ含量;H9c2 细胞 Cx43、ERK1/2 表达量及磷酸化及细胞间通讯情况。结果 与 T 组相比,H/R⁃T 组及 T+AngⅡ组 H9c2 细胞 ERK1/2、Cx43 表达及磷酸化水平降低(P < 0.05),细胞间通讯减弱(P < 0.05);T+ARB 组 H9c2 细胞 ERK1/2、Cx43 表达及 磷酸化水平增高(P < 0.05),细胞间通讯增强(P < 0.05)。与 H/R⁃T 组相比,H/R⁃T+AngⅡ组 H9c2 细胞 ERK1/2、Cx43 表达及磷酸化水平降低(P < 0.05),细胞间通讯减弱(P < 0.05);H/R⁃T+ARB 组 H9c2 细胞 ERK1/2、Cx43 表达及磷酸化水平增加(P < 0.05),细胞间通讯增强(P < 0.05)。结论 H/R 处理后,RCFs 细胞分泌增多的AngⅡ可能通过抑制H9c2细胞MAPK/ERK 通路下调Cx43表达,导致H9c2细胞间通讯减弱。

关键词:

低温缺氧/复氧, 心肌成纤维细胞, H9c2细胞, 缝隙连接蛋白43, 细胞间通讯

Abstract:

Objective To observe the effect on myocardial H9c2 cells gap junction intercellular communi⁃ cation(GJIC)by rat cardiac fibroblasts(RCFs)after hypothermia hypoxia/reoxygen(H/R)and to explore the pos⁃ sible mechanisms. Methods After co⁃cultured of RCFs cells with H9c2 cells in a 2:1 number ratio by Transwell, cells was randomly divided into 6 groups. The T+AngⅡ group and H/R⁃T+AngⅡ group were added 1.5nM AngⅡ, and the T+ARB group and H/R⁃T+ARB group were added 1nM valsartan. The T group,T+AngⅡ group and T+ ARB group were cultured normally,and the H/R⁃T group,H/R⁃T+AngⅡ and H/R⁃T+ARB group were treated with H/R. The AngⅡ concentration in the culture medium;the expression and phosphorylation of Cx43 and ERK1/2; and GJIC of H9c2 cells were detected. Results Compared with the T group,the expression and phosphorylation of ERK1/2 and Cx43 were decreased(P < 0.05)and GJIC was diminished(P < 0.05)in H9c2 cells in the H/R⁃T and T+Ang II group; he expression and phosphorylation of ERK1/2 and Cx43 were increased(P < 0.05)and GJIC was enhanced(P < 0.05)in H9c2 cells in the T+ARB group. Compared with H/R ⁃T group,he expression and phosphorylation of ERK1/2 and Cx43 were decreased(P < 0.05)and GJIC was diminished(P < 0.05)in H9c2 cells in H/R ⁃T+Ang II group; and the expression and phosphorylation of ERK1/2 and Cx43 were increased(P < 0.05)and GJIC was diminished(P < 0.05)in H9c2 cells in H/R ⁃T+ARB group. Conclusion After H/R,in⁃ creased AngⅡ secretion by RCFs may downregulate Cx43 expression by inhibiting the MAPK/ERK pathway in H9c2 cells,resulting in diminished GJIC between H9c2 cells.

Key words:

hypothermia hypoxia/reoxygenation, cardiac fibroblasts, H9c2 cells, connexin 43, gap junction intercellular communication

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