Figure 5. Gadd45β has no effect on the early events in Fas apoptotic signaling. (A) Gadd45β does not affect DISC formation. DISC analysis with lysates from Neo, HA-Gadd45β (Gadd45β), Bcl-xL, and DN-FADD BJAB clones treated with anti–APO-1 for the times indicated. Western blots were performed using anti–APO-1 immunoprecipitates (left panels) or total cell lysates (right panels) and antibodies against caspase-8, FADD, or Fas, as indicated. Fas served as loading control. Note that in the particular BJAB clone shown, DN-FADD inhibited Fas-induced recruitment of endogenous FADD. Specific and nonspecific (n.s.) bands are labeled. Shown is one representative of 3 independent experiments. (B) DISC-associated caspase-8 activity in untreated (–) and anti–APO-1–treated (30 minutes; +) BJAB clones. Clones, Fas stimulation, and DISC immunoprecipitations were as in panel A. Caspase-8–specific activity was measured by fluorimetric assays using zIETD-AFC as in Figure 4B. Values show absolute fluorescence units and represent the mean ± standard deviation of 3 independent experiments. (C) Gadd45β has no effect on the direct Fas-induced processing of Bid. Western blots (50 μg) showing Bid cleavage in Neo and HA-Gadd45β BJAB clones transduced with pBabe-Bid and treated with anti–APO-1 for the times indicated. pBabe-transduced cells were left untreated. Antibodies and Bid-specific bands are labeled.
Figure 5.

Gadd45β has no effect on the early events in Fas apoptotic signaling. (A) Gadd45β does not affect DISC formation. DISC analysis with lysates from Neo, HA-Gadd45β (Gadd45β), Bcl-xL, and DN-FADD BJAB clones treated with anti–APO-1 for the times indicated. Western blots were performed using anti–APO-1 immunoprecipitates (left panels) or total cell lysates (right panels) and antibodies against caspase-8, FADD, or Fas, as indicated. Fas served as loading control. Note that in the particular BJAB clone shown, DN-FADD inhibited Fas-induced recruitment of endogenous FADD. Specific and nonspecific (n.s.) bands are labeled. Shown is one representative of 3 independent experiments. (B) DISC-associated caspase-8 activity in untreated (–) and anti–APO-1–treated (30 minutes; +) BJAB clones. Clones, Fas stimulation, and DISC immunoprecipitations were as in panel A. Caspase-8–specific activity was measured by fluorimetric assays using zIETD-AFC as in Figure 4B. Values show absolute fluorescence units and represent the mean ± standard deviation of 3 independent experiments. (C) Gadd45β has no effect on the direct Fas-induced processing of Bid. Western blots (50 μg) showing Bid cleavage in Neo and HA-Gadd45β BJAB clones transduced with pBabe-Bid and treated with anti–APO-1 for the times indicated. pBabe-transduced cells were left untreated. Antibodies and Bid-specific bands are labeled.

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