Next, we evaluated the potential interactions
www.selleckchem.com/products/psi-7977-gs-7977.html between opioid and somatostatin receptors. U266 cells were exposed or not (control) either to Sst alone, to a combination of Sst plus 10 μM morphine (Morph) or Css, but still no modification of U266 cell viability was noted after 24, 48 or 72 h (Figure 2C). Effects of Sst and Oct on cell cycle distribution in U266 cells We confirmed by using an alternative method, that SSTR agonists were ineffective to regulate U266 cell proliferation. Distribution in the cell cycle of control or agonist-pretreated U266 cells was determined after PI staining by flow cytometry. A low (10 nM) or a high concentration (10 μM) of Sst or Oct alone, or in combination with Css were selected and cells were exposed Fosbretabulin during 24, 48 or 72 h. A representative experiment is depicted in the Figure 3 showing that neither Sst (10 μM) nor Oct (10 μM) were able to promote changes in cell cycle distribution compared to control cells after 72 h. Similar data were obtained for 24 and
48 h pretreatment (data not shown). The check details percentage of each phase was determined for control or agonist-pretreated cells and these data are summarised in the Table 3. Table 3 Cell cycle distribution of U266 MM cell line treated with SSTR ligands and 7C11 Treatment G0-G1 (%) S (%) G2-M (%) Sub-G1 (%) Control 56,6 ± 3,0 25,1 ± 2,3 12,4 ± 1,1 2,5 ± 0,3 Sst 10 μM 57,4 ± 2,0 26,3 ± 0,8 9,6 ± 1,8 3,3 ± 0,2 Css 10 μM 60,8 ± 2,4 20,7 ± 2,4 11,2 ± 0,1 3,7 ± 0,8 Sst 10 μM/Css 10 μM 57,3 ± 2,2 26,2 ± 0,9 10,0 ± 2,5 2,9 ± 0,4 7C11 39,9 ± 1,5* 26,8 ± 1,1 9,9 ± 1,0 16,0 ± 0,9* 7C11/Sst 10 μM 40,3 ± 1,8* 27,2 ± 0,4 8,6 ± 1,1 14,0 ± 0,7* 7C11/Sst 10 μM/Css 10 μM 38,3 ± 3,3* 27,3 ± 1,0 8,9 ± 0,8 12,0
± 1,1* Oct 10 μM 55,2 ± 4,6 25,1 ± 3,5 13,6 ± 1,5 3,0 ± 0,5 Oct 10 μM/Css 10 μM 55,6 ± 4,7 24,9 ± 3,6 12,6 ± 1,6 4,0 ± 0,8 7C11/Oct 10 μM 43,1 ± Bumetanide 0,5* 27,2 ± 1,7 12,2 ± 1,5 13,6 ± 1,9* 7C11/Oct 10 μM/Css 10 μM 41,9 ± 0,8* 26,4 ± 2,6 8,1 ± 0,4 18,2 ± 4,6* U266 cells were pretreated or not (control) with Sst, Oct, Css or the agonistic Fas antibody 7C11 (7C11) for 72 h. Cells were stained with PI, analyzed by flow cytometry and each fraction of the cell cycle was determined using Wincycle®. Data are mean ± S.E.M. of 3 independent experiments. *, ANOVA followed by Bonferroni-Dunn (p < 0.05), statistically significant differences compared to control cells. Figure 3 Cell cycle distribution of U266 cells after SSTR stimulation. Exponentially growing cells were incubated with 10 μM Sst or Oct, or with 0.1 mg/mL 7C11 (agonistic Fas antibody) for 72 h. DNA content analysis was done after PI staining of ethanol-permeabilized cells.