![Fig. 3. Fluoxetine actions on and Bcl-2 levels in normal B cells and non-BL cell lines. / (A) Resting tonsilar B cells were cultured at 105 cells per 200 μL culture medium for 48 hours in flat-bottom microtiter wells with either no addition (CM), Staphylococcus aureus Cowan 1 (SAC, 1:10 000), phorbol 12-myristate 13-acetate (PMA, 5 ng/mL), SAC+sCD40L (1μg/mL), or PMA + ionomycin (PMA/I, 1 μg/mL), before addition of fluoxetine at 0 to 20 μM as indicated. Cells were then cultured for a further 24 hours, pulsed with 3[H]-thymidine for the last 7 hours for the analysis of DNA synthesis. (B) Cells from lines indicated were cultured for 24 hours with fluoxetine as in panel A before assessment of DNA synthesis as described in Figure 1A-D. Data are means ± SEMs from 3 separate experiments. (C-D) Cell lysates were prepared from pelleted cells and equal amounts of protein (25 μg) resolved on 12.5% SDS-PAGE before blotting for Bcl-2, the protein migrating with an apparent molecular weight of 26 kDa as indicated. Panel C is a representative blot of protein from L3055 (wild type), L3055 vector controls, L3055/Bcl-2 transfectants, Namalwa, Elijah, Mutu I, and resting tonsilar B cells; panel D, from Nalm 6, CEM, Jurkat, J10, RPMI8226, resting tonsilar B cells, and B cells activated for 48 hours with PMA+ionomycin.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/101/8/10.1182_blood-2002-07-2044/4/h80834123003.jpeg?Expires=1725020819&Signature=NTBKaul0XrXcbBkqi1qHUXTu3B3hrJnlIKdev5GZg1dNyLxblfxClUROdMFz-Vj0MhhsX346LE3VPYIJ2cjbLs770ilKy81MFCMmt74B8wzk2aqah6MUReIiQBoGNl1WcKUYgk~I~KCHXCs8SLF55veLG~RRw1ZVXXPlE1hwQR4q6CwZ6SOJaNjITT0CirfDGQ5eT-mcwfeEj5RJA~ihSxEy9-2d8Pu~E-YzvilqhHIhxyHwHa73YU7h~u2p1ZzQQf5ikEJ~hJH~oN1wVwSXg4LuiMMbEoRyGmRKkdp2bbS4lc3MEO~OXJfx0EFNFSNKOKj8U5hp1bNBL~JhcVbT7A__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Fluoxetine actions on and Bcl-2 levels in normal B cells and non-BL cell lines.
(A) Resting tonsilar B cells were cultured at 105 cells per 200 μL culture medium for 48 hours in flat-bottom microtiter wells with either no addition (CM), Staphylococcus aureus Cowan 1 (SAC, 1:10 000), phorbol 12-myristate 13-acetate (PMA, 5 ng/mL), SAC+sCD40L (1μg/mL), or PMA + ionomycin (PMA/I, 1 μg/mL), before addition of fluoxetine at 0 to 20 μM as indicated. Cells were then cultured for a further 24 hours, pulsed with 3[H]-thymidine for the last 7 hours for the analysis of DNA synthesis. (B) Cells from lines indicated were cultured for 24 hours with fluoxetine as in panel A before assessment of DNA synthesis as described in Figure 1A-D. Data are means ± SEMs from 3 separate experiments. (C-D) Cell lysates were prepared from pelleted cells and equal amounts of protein (25 μg) resolved on 12.5% SDS-PAGE before blotting for Bcl-2, the protein migrating with an apparent molecular weight of 26 kDa as indicated. Panel C is a representative blot of protein from L3055 (wild type), L3055 vector controls, L3055/Bcl-2 transfectants, Namalwa, Elijah, Mutu I, and resting tonsilar B cells; panel D, from Nalm 6, CEM, Jurkat, J10, RPMI8226, resting tonsilar B cells, and B cells activated for 48 hours with PMA+ionomycin.
