神经药理学报

神经药理学报 ›› 2023, Vol. 13 ›› Issue (3): 1-.DOI: 10.3969/j.issn.2095-1396.2023.03.001

• 研究论文 •    下一篇

BI-D1870对N2a细胞毒作用

易妍,商亚珍   

  1. 承德医学院中药研究所,河北省中医药抗痴呆重点研究室,河北省中药研究与开发重点实验室,河北省神经损伤与修复重点实验室,承德,067000,中国
  • 出版日期:2023-06-26 发布日期:2024-05-09
  • 通讯作者: 商亚珍,医学博士,博士生导师,二级教授;研究方向:从事中药复方或提取成分抗阿尔茨海默病药理作用及机制研究;E-mail: 973358769@qq.com
  • 作者简介:易妍,女,硕士研究生;研究方向:中药药理;E-mail: 1350407346@qq.com
  • 基金资助:
    河北省自然基金资助项目(No. H2019406063);河北省中医药管理局资助项目 (No. 05027, No.2014062);河北省教育厅重点项目(No.ZD20131022, No.ZD2019057);河北省中药学重点学科建设项目;河北省中医药中药药理重点学科建设项目(冀中医药函[2021]12号);承德医学院科技创新团队项目(No. [2020]50)

Cytotoxic Effect of BI-D1870 in N2a Cells

YI Yan, SHANG Ya-zhen   

  1. Institute of Traditional Chinese Medicine, Chengde Medical College, Hebei Province Key Research Office of Traditional Chinese Medicine Against Dementia, Hebei Province Key Laboratory of Traditional Chinese Medicine Research and Development, Hebei Key Laboratory of Nerve Injury and Repair, Chengde, 067000, China
  • Online:2023-06-26 Published:2024-05-09
  • Contact: 商亚珍,医学博士,博士生导师,二级教授;研究方向:从事中药复方或提取成分抗阿尔茨海默病药理作用及机制研究;E-mail: 973358769@qq.com
  • About author:易妍,女,硕士研究生;研究方向:中药药理;E-mail: 1350407346@qq.com

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摘要:

目的:探讨RSK抑制剂BI-D1870对N2a细胞毒作用,确定产生细胞毒作用的浓度和时间。方法:N2a细胞体外培养,免疫荧光法鉴定神经细胞特异性蛋白NeuroD1、NeuN和DCX。N2a细胞用10~80 μmol·L-1 BI-D1870,分别作用4~24 h。倒置显微镜观察N2a细胞形态,CCK-8法检测细胞存活率,丙酮酸还原法检测细胞培养液中乳酸脱氢酶(lactate dehydrogenase, LDH)释放量。结果:免疫荧光可检测到N2a细胞有NeuroD1、NeuN和DCX 阳性表达。与对照组比较,随着BI-D1870作用浓度增加和作用时间延长,N2a细胞受损程度逐渐增加,细胞形态发生异常改变,细胞存活率逐渐降低(P<0.05),培养液中LDH先升高后降低(P<0.05)。40 μmol·L-1作用12 h条件下N2a细胞肿胀明显,折光率降低,细胞存活率在60%左右,LDH释放量增长率最高。结论:N2a细胞具有神经细胞特性,BI-D1870 对N2a细胞有细胞毒作用,产生细胞毒作用的最适条件为40 μmol·L-1作用12 h。

关键词: BI-D1870, N2a细胞, 乳酸脱氢酶, 细胞毒作用

Abstract:

Objective: To investigate the cytotoxic effect of RSK inhibitor BI-D1870 in N2a and determine the concentration and time of cytotoxic effect. Methods: N2a cells were cultured in vitro, and the specific proteins NeuroD1, NeuN and DCX were identified by immunofluorescence. N2a cells were exposed to a series concentration of 10 μmol•L-1 to 80 μmol•L-1 BI-D1870 and a series duration of 4 h to 24 h. The morphology of N2a cell was observed with the inverted microscope, and the cell viability was measured with CCK-8 method, and lactate dehydrogenase (LDH) release of cell culture medium was assayed by pyruvate reduction method. Results: NeuroD1, NeuN and DCX were detected in N2a cells by immunofluorescence. Compared with the DMSO solvent control group, with the increase of BI-D1870 concentration and the exposure prolongation of BI-D1870, the damage degree of N2a cells gradually increased. The cell morphology changed abnormally, the cell viability decreased gradually (P<0.05) and LDH level in culture medium went up and then went down (P<0.05). Under the treatment of 40 μmol•L-1 for 12 h, the swelling of N2a cells was obvious, the refraction was reduced, the cell viability was about 60%, and the LDH release in culture medium was the highest. Conclusion: N2a cells have the characteristics of neuron. BI-D1870 has cytotoxic effect for N2a cells and the optimal cytotoxic condition is 40 μmol•L-1 for 12 h.

Key words: BI-D1870, N2a Cells, LDH, cytotoxic effect