Proliferation Inhibition, DNA Damage, and Cell-Cycle Arrest of Human Astrocytoma Cells after Acrylamide Exposure

被引:33
作者
Chen, Jong-Hang [1 ]
Tsou, Tsui-Chun [2 ]
Chiu, Ing-Ming [3 ,4 ]
Chou, Chin-Cheng [1 ,5 ]
机构
[1] Natl Taiwan Univ, Dept Vet Med, Taipei 106, Taiwan
[2] Natl Hlth Res Inst, Div Environm Hlth & Occupat Med, Zhunan 350, Miaoli County, Taiwan
[3] Natl Hlth Res Inst, Inst Cellular & Syst Med, Zhunan 350, Miaoli County, Taiwan
[4] Ohio State Univ, Dept Internal Med, Columbus, OH 43210 USA
[5] Natl Taiwan Univ, Coll Bioresources & Agr, Ctr Zoonoses Res, Taipei 106, Taiwan
关键词
FIBRILLARY ACIDIC PROTEIN; HUMAN NEUROBLASTOMA-CELLS; CENTRAL-NERVOUS-SYSTEM; GROWTH; ACTIVATION; PROMOTER; AGENT; KI-67; PHOSPHORYLATION; ONCOGENICITY;
D O I
10.1021/tx1000893
中图分类号
R914 [药物化学];
学科分类号
100701 ;
摘要
Acrylamide (ACR) has been recognized as a neurological and reproductive toxin in humans and laboratory animals. This study aimed to determine the effects of ACR-induced DNA damage on cell cycle regulation in human astrocytoma cell lines. Treatment of U-I 240 MG cells with 2 mM ACR for h resulted hi a significant inhibition of cell proliferation as evaluated by Ki-67 protein expression and MTT assay. The analysis of DNA damage with the comet assay showed that treatment of the cells with 0.5, 1, and 2 mM ACR for 48 h caused significant increases in DNA damage by 3.5-, 4-, and 14-fold, respectively. Meanwhile, analysis of cell-cycle arrest with flow cytometry revealed that the ACR treatments resulted in significant increases in the G(0)/G(1)-arrested cells in a time- and dose-dependent manner. Expression of DNA damage-associated/checkpoint-related signaling molecules, including phosphorylated-p53 (pp53), p53, p21, p27, Cdk2, and cyclin D-1, in three human astrocytoma cell lines (U-1240 MG, U-251 MG, and U-87 MG) was also analyzed by immunoblotting. Treatment of the three cell lines with 2 mM ACR for 48 h caused marked increases in pp53 and Cdk2, as well as decreases in cyclin D-1 and p27. Moreover, increases in p53 and p21 were detected in both U-I240 and U-87 MG cells, whereas no marked change in p53 and a decrease in p21 were observed in U-251 MG cells. To address the involvement of ataxia telangiectasia mutated/ATM-Rad3-related (ATM/ATR) kinase in the signaling of ACR-induced G(0)/G(1) arrest, caffeine was used to block the ATM/ATR pathway in U-1240 MG cells. Caffeine significantly attenuated the ACR-induced G(0)/G(1) arrest as well as the expression of DNA damage-associated/checkpointrelated signaling molecules in a dose-dependent manner. This in vitro study clearly demonstrates the critical role of ATM/ATR in the signaling of ACR-induced cell-cycle arrest in astrocytoma cells.
引用
收藏
页码:1449 / 1458
页数:10
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