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新藤黄酸对S180细胞株的体内外抗肿瘤作用
引用本文:肖国丽,赵学军,刘卫海,赵爱国.新藤黄酸对S180细胞株的体内外抗肿瘤作用[J].中国实验方剂学杂志,2012,18(13):193-197.
作者姓名:肖国丽  赵学军  刘卫海  赵爱国
作者单位:1. 广州中医药大学新药开发研究中心,广州,510006
2. 东莞广州中医药大学中医药数理工程研究院,广东东莞523808;广州中医药大学新药开发研究中心,广州 510006
3. 清远医药集团,广东清远511518;东莞广州中医药大学中医药数理工程研究院,广东东莞523808
基金项目:广东省高等学校科技创新团队项目(06CXTD004);广东省科技计划重点项目(2008A030101002);东莞市科技计划高等院校和科研机构项目(2007108101080)
摘    要:目的:评价新藤黄酸对S180肿瘤细胞株的体内外抗肿瘤作用.方法:将不同浓度的新藤黄酸分别作用于体外培养的S180细胞48 h,用CCK-8法检测药物对S180细胞的增殖抑制作用;以8.0,4.0,2.0 mg·kg-1剂量ip给予S180腹水瘤小鼠,每天1次,连续7d,观察45 d对存活时间的影响;以16.0,8.0,4.0 mg·kg-1剂量ig给予荷S180实体瘤小鼠,每天1次,连续12d,评价新藤黄酸的体内抗肿瘤作用;测单次ip给药对小鼠的LD50.结果:新藤黄酸对体外培养S180细胞的增殖有明显的抑制作用,药物作用48 h其IC50为(1.54±0.12) mg·L-1;4.0 mg· kg-1新藤黄酸ip给药可使S180腹水瘤小鼠存活时间较荷瘤对照组延长141.6%,新藤黄酸对S180实体瘤的抑制作用随着剂量的增大而升高,并呈一定剂量依赖性,体内抗肿瘤显著(P<0.05);单次ip给药对小鼠的LD50为36.66 mg·kg-1.结论:新藤黄酸对S180细胞株具有明显的体内外抗肿瘤作用.

关 键 词:新藤黄酸  S180细胞株  抗肿瘤
收稿时间:2011/12/25 0:00:00

Anti-tumor Effects of Neogambogic Acid on S180 Cell Line Both in vivo and in vitro
XIAO Guo-li,ZHAO Xue-jun,LIU Wei-hai and ZHAO Ai-guo.Anti-tumor Effects of Neogambogic Acid on S180 Cell Line Both in vivo and in vitro[J].China Journal of Experimental Traditional Medical Formulae,2012,18(13):193-197.
Authors:XIAO Guo-li  ZHAO Xue-jun  LIU Wei-hai and ZHAO Ai-guo
Institution:New Drug R & D Center, Guangzhou University of Chinese Medicine, Guangzhou 510006, China;New Drug R & D Center, Guangzhou University of Chinese Medicine, Guangzhou 510006, China;New Drug R & D Center, Guangzhou University of Chinese Medicine, Guangzhou 510006, China;Dongguan Institution for Mathematics and Theoretics Engineering Research, Guangzhou University of Chinese Medicine, Dongguan 523808, China;Dongguan Institution for Mathematics and Theoretics Engineering Research, Guangzhou University of Chinese Medicine, Dongguan 523808, China;Qingyuan Medicine Group, Qingyuan 511518, China
Abstract:Objective: To evaluate the anti-tumor effects of neogambogic acid on S180 cell line both in vivo and in vitro. Method: CCK-8 method was used to assay the anti-proliferative effect of neogambogic acid with different concentrations for 48 h on S180 cell line in vitro. The anti-tumor effect in vivo was evaluated by the survival time of the mice bearing S180 ascitic tumor, which was ip treated with 8.0, 4.0, 2.0 mg·kg-1 neogambogic acid respectively, once per day for continuous 7 days, and observation period lasted for 45 days, and the mice bearing S180 xenograft was ig treated with 16.0, 8.0, 4.0 mg·kg-1 neogambogic acid respectively, once per day for continuous 12 days. The LD50 of mice was determined based on single administration (ip)of different doses of neogambogic acid. Result: Neogambogic acid showed obvious anti-proliferative effect on S180 cell culture, the IC50 of 48 h was (1.54±0.12) mg·L-1. And the in vivo test showed that the survival time of the mice administrated with 4.0 mg·kg-1 neogambogic acid was prolonged 141.6%. The inhibitory effects of the mice bearing tumor increased with the increasing of the concentration of neogambogic acid in a dose-dependent manner (P<0.05). The LD50 of neogambogic acid (ip) was 36.66 mg·kg-1. Conclusion: The results suggest that the anti-tumor effect of neogambogic acid on S180 cell line is significant both in vivo and in vitro.
Keywords:neogambogic acid  S180 cell line  anti-tumor
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