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Fig. 2. CD95 capping does not correlate with induction of apoptosis. (A) Jurkat and (B) H9 cells were pre-treated for 1 hour with cytD or zIETD and were then incubated with 200 ng/ml {alpha}CD95 for 2 hours (Jurkat) or 6 hours (H9) to induce apoptosis. Cells were then labeled and analyzed for the presence of activated caspase-3, by flow cytometry. The data are mean values (±s.e.m.) from a minimum of three separate experiments. (C) Nuclear morphology of CytD- and {alpha}CD95-treated cells was further analyzed by DAPI labeling. Typical apoptotic cells with condensed chromatin can be seen in the {alpha}CD95 treated samples. CytD treatment did not inhibit the nuclear alterations associated with apoptosis. (D) Cells were treated as in A. and were then assessed for overall cleavage of caspase-8 by immunoblotting. Overall caspase-8 cleavage does not correlate with the capping of CD95 (Fig. 1C,D). Representative immunoblots from two separate experiments are shown.





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