机构地区:[1]Department of Neurosurgery,The First Affiliated Hospital of Nanjing Medical University,Nanjing 210029,China [2]Department of Oncology,Jinling Hospital,Nanjing University,Nanjing 210002,China
出 处:《Acta Pharmacologica Sinica》2012年第7期935-940,共6页中国药理学报(英文版)
基 金:We thank Professor Kun YAO for providing the U251 and U87 human glioblastoma cell line. This work was supported by grants from the Jiangsu Province Natural Science Foundation (No BK2007257).
摘 要:Aim: To examine the effects of anisomycin on glioma cells and the related mechanisms in vitro. Methods: The U251 and U87 human glioblastoma cell lines were tested. The growth of the cells was analyzed using a CCK-8 cell viability assay. Apoptosis was detected using a flow cytometry assay. The expression of proteins and phosphorylated kinases was detected using Western blotting. Results: Treatment of U251 and U87 cells with anisomycin (0.01-8 pmol/L) inhibited the cell growth in time- and concentration- dependent manners (the IC50 values at 48 h were 0.233±0.021 and 0.192±0.018 pmol/L, respectively). Anisomycin (4 pmol/L) caused 21.5%±2.2% and 25.3%±3.1% of apoptosis proportion, respectively, in U251 and U87 cells. In the two cell lines, anisomycin (4 pmol/L) activated p38 MAPK and JNK, and inactivated ERK1/2. However, neither the p38 MAPK inhibitor SB203580 (10 pmol/L) nor the JNK inhibitor SP600125 (10μmol/L) prevented anisomycin-induced cell death. On the other hand, anisomycin (4 μmol/L) reduced the level of PP2A/C subunit (catalytic subunit) in a time-dependent manner in the two cell lines. Treatment of the two cell lines with the PP2A inhibitor okadaic acid (100 nmol/L) caused marked cell death. Conclusion: Anisomycin induces glioma cell death via down-regulation of PP2A catalytic subunit. The regulation of PP2A/C exression by anisomycin provides a clue to further study on its role in glioma therapy.Aim: To examine the effects of anisomycin on glioma cells and the related mechanisms in vitro. Methods: The U251 and U87 human glioblastoma cell lines were tested. The growth of the cells was analyzed using a CCK-8 cell viability assay. Apoptosis was detected using a flow cytometry assay. The expression of proteins and phosphorylated kinases was detected using Western blotting. Results: Treatment of U251 and U87 cells with anisomycin (0.01-8 pmol/L) inhibited the cell growth in time- and concentration- dependent manners (the IC50 values at 48 h were 0.233±0.021 and 0.192±0.018 pmol/L, respectively). Anisomycin (4 pmol/L) caused 21.5%±2.2% and 25.3%±3.1% of apoptosis proportion, respectively, in U251 and U87 cells. In the two cell lines, anisomycin (4 pmol/L) activated p38 MAPK and JNK, and inactivated ERK1/2. However, neither the p38 MAPK inhibitor SB203580 (10 pmol/L) nor the JNK inhibitor SP600125 (10μmol/L) prevented anisomycin-induced cell death. On the other hand, anisomycin (4 μmol/L) reduced the level of PP2A/C subunit (catalytic subunit) in a time-dependent manner in the two cell lines. Treatment of the two cell lines with the PP2A inhibitor okadaic acid (100 nmol/L) caused marked cell death. Conclusion: Anisomycin induces glioma cell death via down-regulation of PP2A catalytic subunit. The regulation of PP2A/C exression by anisomycin provides a clue to further study on its role in glioma therapy.
关 键 词:ANISOMYCIN GLIOMA apoptosis p38 MAPK JNK protein phosphatase 2A
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