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©2005 Baishideng Publishing Group Inc.
World J Gastroenterol. Oct 28, 2005; 11(40): 6373-6380
Published online Oct 28, 2005. doi: 10.3748/wjg.v11.i40.6373
Published online Oct 28, 2005. doi: 10.3748/wjg.v11.i40.6373
Figure 1 Effect of DEX on the growth and chemosensitivity in carcinoma cell lines.
Cell numbers were measured by MTT assay and were plotted as a percentage of the control (cells not exposed to drugs); A: Growth of MCF-7, MCF-7/MXR1, MCF-7/TPT300, and HeLa cells were suppressed by DEX. Data of AGS represent the other 10 cell lines, growth of which was not affected by DEX; B: SiHa cells pretreated with DEX for 3 h were more sensitive to cisplatin; C and D: Pretreatment with DEX 1 mmol/L for 24 h diminished cisplatin cytotoxicity in H460 cells and Hep3B cells; E: Data of AGS represent the seven cell lines (AGS, N87, Caski, Hut 7, SNU1, NPC-TW01, and NPC-TW04), of which cytotoxicity of cisplatin was not affected by DEX. All values represent mean±SD of six separate wells.
Figure 2 Functional assay of the GR in NPC-TW01 and NPC-TW04 cells.
NPC-TW01, NPC-TW04, and MCF-7 cells were transiently transfected with MMTV reporter plasmid (lanes M and M+DEX) or co-transfected with MMTV reporter plasmid and pS-hGR (lane M/G+DEX). The cells were then treated with 1 μmol/L DEX for 6 h (lanes M+DEX and M/G+DEX). Then the luciferase activity was assayed and represented in terms of folds of the induction activity of the control (lane M). All values represent mean±SD of three experiments(A,B).
Figure 3 Increased drug resistance to cisplatin in pS-hGR-transfected AGS.
AGS cells were transfected with pS-hGR and MTT assay were performed. A: GR number measured by [3H]-labeled ligand binding assay. Pool: AGS/GR-pool; AGS cells transfected with pS-hGR, pooled cells. c1: AGS/GR-c1; AGS cells transfected with pS-hGR, single cell cloned, clone 1. c2: AGS/GR-c2; AGS cells transfected with pS-hGR, single cell cloned, clone 2. Mock: AGS/empty vector; AGS cells transfected with empty vector. c3: AGS/GR-c3; AGS cells transfected with pS-hGR, single cell cloned, clone 3; B-D: Pretreatment with DEX 1 μmol/L for 3 h diminished cisplatin cytotoxicity in AGS/GR-pool, AGS/GR-c1, and AGS/GR-c2 cells; E and F: Pretreatment with DEX 1 μmol/L for 3 h had no effect on the cisplatin cytotoxicity in AGS/empty vector cells and AGS/GR-c3. All values represent mean±SD of six separate wells.
Figure 4 A: Immunocytochemical stain for GR expression in representing carcinoma cell lines.
(A1) and A2): SiHa cells, which had GR content about 8.1×104/cell according to ligand binding assay; (A3) and (A4): HeLa cells, with GR content about 1.97×104/cell; (A5) and (A6): N87 cells, with GR content about 5.0×103/cell. (A2), (A4), and (A5): cells treated with DEX for 3 h before harvest. In (A1) and (A3), the GR immunoreactivity localized in cytoplasm. After DEX treatment, the immunoreactive GR translocalized to nuclei (A2) and (A4). The low GR content cancer cells N87 showed negligible immunoreactivity. B: Immunohistochemical stain for GR expression in human carcinoma tumor tissue samples. Non-small cell lung cancer tumor samples, with high GR expression (Ba), and low GR expression (B2). Breast cancer tumor samples, with high GR expression (B3), and low GR expression (B4).
- Citation: Lu YS, Lien HC, Yeh PY, Yeh KH, Kuo ML, Kuo SH, Cheng AL. Effects of glucocorticoids on the growth and chemosensitivity of carcinoma cells are heterogeneous and require high concentration of functional glucocorticoid receptors. World J Gastroenterol 2005; 11(40): 6373-6380
- URL: https://www.wjgnet.com/1007-9327/full/v11/i40/6373.htm
- DOI: https://dx.doi.org/10.3748/wjg.v11.i40.6373