Figure 2.
Figure 2. c-FL/P overexpression in ALCL. (A-C) Immunohistochemical detection of extrinsic apoptotic pathway proteins in reactive lymph node and ALK+ anaplastic large-cell lymphoma (ALCL) tumors. (A) CD95/FAS was weakly expressed in a subset of centroblasts within the germinal centers (GCs) of reactive lymph nodes (left). Strong cytoplasmic and membranous CD95/FAS expression was observed in most ALK+ ALCL tumors (right). (B) CD95L/FASL was strongly positive in the mantle and marginal zones of reactive lymph nodes (left). CD95L/FASL was not expressed in most ALK+ ALCL tumors (right). Infiltrating small reactive lymphocytes strongly expressed CD95L/FASL and served as internal positive controls in all tumor specimens. (C) c-FLIP expression was restricted to a subset of GC cells (left). Strong cytoplasmic expression for c-FLIP was observed in most ALK+ ALCL tumors (right). (D-E) c-FLIP up-regulation may result from activation of PI3K/Akt and JAK3/ALK oncogenic pathways. Immunohistochemistry: × 200 original magnification (20 ×/0.75 NA objective; left panels) or × 400 (40 ×/0.75 NA objective; right panels). Images were obtained with a BX51 Olympus microscope, a DP12 Olympus camera, and a universal semi-apochromat UPlan FI lens. (D, left panel) Karpas 299 and SU-DHL1 cells were treated with a PI3K inhibitor, LY294002, at concentrations of 0, 5, or 20 μg/μL. Whole-cell lysates were then prepared at 48 hours. Immunoblots showed that serine 473 phosphorylation of Akt is almost completely inhibited at a concentration of 20 μg/μL that is associated with a substantial decrease of c-FLIP levels. (D, right panel) Karpas 299 and SU-DHL1 cells were infected with the constitutively active, myrAkt adenovirus21 at an MOI of 20, which significantly increases Ser473pAKT levels in these cells. Expression of myrAkt was confirmed by Western blot analysis using a monoclonal antibody specific for the hemagglutinin (HA) tag. An adeno-β-Gal adenovirus construct expressing β-Gal served as a control in this experiment. Whole-cell lysates were prepared from control and infected cells 48 hours after infection. Immunoblots showed a dramatic increase of Akt phosphorylation, which was associated with an increase of c-FLIPS splice variant. (E) ALK+ ALCL cells were treated with 2 known JAK3 inhibitors, WHI-P131 and WHI-P154, at concentrations previously shown to inhibit JAK3 and ALK enzymatic activity. 25Whole-cell lysates were prepared 24 hours following treatment. Immunoblots demonstrate that c-FLIP levels are decreased after treatment with WHI-P131 or WHI-P154 in a dose-dependent manner.

c-FL/P overexpression in ALCL. (A-C) Immunohistochemical detection of extrinsic apoptotic pathway proteins in reactive lymph node and ALK+ anaplastic large-cell lymphoma (ALCL) tumors. (A) CD95/FAS was weakly expressed in a subset of centroblasts within the germinal centers (GCs) of reactive lymph nodes (left). Strong cytoplasmic and membranous CD95/FAS expression was observed in most ALK+ ALCL tumors (right). (B) CD95L/FASL was strongly positive in the mantle and marginal zones of reactive lymph nodes (left). CD95L/FASL was not expressed in most ALK+ ALCL tumors (right). Infiltrating small reactive lymphocytes strongly expressed CD95L/FASL and served as internal positive controls in all tumor specimens. (C) c-FLIP expression was restricted to a subset of GC cells (left). Strong cytoplasmic expression for c-FLIP was observed in most ALK+ ALCL tumors (right). (D-E) c-FLIP up-regulation may result from activation of PI3K/Akt and JAK3/ALK oncogenic pathways. Immunohistochemistry: × 200 original magnification (20 ×/0.75 NA objective; left panels) or × 400 (40 ×/0.75 NA objective; right panels). Images were obtained with a BX51 Olympus microscope, a DP12 Olympus camera, and a universal semi-apochromat UPlan FI lens. (D, left panel) Karpas 299 and SU-DHL1 cells were treated with a PI3K inhibitor, LY294002, at concentrations of 0, 5, or 20 μg/μL. Whole-cell lysates were then prepared at 48 hours. Immunoblots showed that serine 473 phosphorylation of Akt is almost completely inhibited at a concentration of 20 μg/μL that is associated with a substantial decrease of c-FLIP levels. (D, right panel) Karpas 299 and SU-DHL1 cells were infected with the constitutively active, myrAkt adenovirus21  at an MOI of 20, which significantly increases Ser473pAKT levels in these cells. Expression of myrAkt was confirmed by Western blot analysis using a monoclonal antibody specific for the hemagglutinin (HA) tag. An adeno-β-Gal adenovirus construct expressing β-Gal served as a control in this experiment. Whole-cell lysates were prepared from control and infected cells 48 hours after infection. Immunoblots showed a dramatic increase of Akt phosphorylation, which was associated with an increase of c-FLIPS splice variant. (E) ALK+ ALCL cells were treated with 2 known JAK3 inhibitors, WHI-P131 and WHI-P154, at concentrations previously shown to inhibit JAK3 and ALK enzymatic activity. 25 Whole-cell lysates were prepared 24 hours following treatment. Immunoblots demonstrate that c-FLIP levels are decreased after treatment with WHI-P131 or WHI-P154 in a dose-dependent manner.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal