Effect of P15INK4b expression on the cell cycle and G1 phase related regulatory genes in human melanoma cells

被引:0
|
作者
Liu, J [1 ]
Tong, YK [1 ]
Liu, HT [1 ]
Zhang, W [1 ]
Gao, P [1 ]
机构
[1] Beijing Normal Univ, Coll Life Sci, State Key Lab Cell Proliferat & Regulat Biol Educ, Beijing 100875, Peoples R China
关键词
P15(INK4b); CKI; cell cycle; G(1) phase-related gene; cell synchronization;
D O I
暂无
中图分类号
T [工业技术];
学科分类号
08 ;
摘要
Using the transfection technique, P15(INK4b) was introduced into P15(INK4b) gene deleted human melanoma A375 tells, and a cell model MLIK6 overexpressing P15(INK4b) was constructed. Comparing with the control cells MLC2, MLIK6 cells in G(t) phase increased by 11%, but those in S phase decreased by 15% by FCM. By the method of thymidine (TdR) and N2O arresting, the proportions of synchronized M phase cells of MLIK6 and MLC2 were measured and found to be 89.1% and 76.8%, respectively, and the tells in G(1) phase were 74.3% for MLIK6 and 76. 4% for MLC2. The result of H-3-TdR incorporation indicated that the transition of G(1)/S of MLIK6 cell was delayed 2 h as compared with that of MLC2 cells, and incorporation rate also decreased. The observation on expressions of some G(1)/S-related relatory regulating genes showed that in MLIK6 cells the protein level of P27(KIP1) increased with the decreasing expressions of cycllinD1, cyclinE and c-myc, especially cyclinD1 in late G(1) phase. The expression of cyclinE obviously decreased at G(1)/S transition, and c-myc was inhibited throughout all the process of G(1)-->S phase. All the results suggest that P15(INK4b) call delay G(1)/S transition of MLIK6 cells by inhibiting the cell cycle engine molecule, and by increasing the expression of Cdk inhibitor P27(KIP1) in different stages of G(1) phase.
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页码:40 / 45
页数:6
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