Fig. 4.
Fig. 4. Nfv inhibits apoptosis induced by PTPC opening. / (A) Jurkat T cells were pretreated with MeOH (♦) or 7 μM Nfv (■) for 1 hour before overnight stimulation with the indicated doses of Vpr. Apoptosis was assessed by annexin-V and propidium iodide. Data are representative of 3 independent experiments. (B) Mitochondrial Δψm was assessed using DiOC6. Data are representative of 3 independent experiments. ♦, Vpr; ■, Vpr + Nfv. (C) Jurkat cells were treated with MeOH or 7 μM Nfv for 1 hour before overnight stimulation with 2.5 μM bovine serum albumin (BSA) or 2.5 μM Vpr and immunoblotted for cytochrome-c release (upper) and pro–caspase-8 cleavage (lower) in the cytosolic fraction. (D) Immunoblot of Hsp 70 in pellet and cytosolic fractions. (E) Isolated mitochondria were treated overnight with methanol (▪), 7 μM Nfv (░), or 50 μM BA (▤) before being stimulated with 2.5 μM Vpr or 5 mM ATR. Loss of Δψm was assessed using DiOC6.

Nfv inhibits apoptosis induced by PTPC opening.

(A) Jurkat T cells were pretreated with MeOH (♦) or 7 μM Nfv (■) for 1 hour before overnight stimulation with the indicated doses of Vpr. Apoptosis was assessed by annexin-V and propidium iodide. Data are representative of 3 independent experiments. (B) Mitochondrial Δψm was assessed using DiOC6. Data are representative of 3 independent experiments. ♦, Vpr; ■, Vpr + Nfv. (C) Jurkat cells were treated with MeOH or 7 μM Nfv for 1 hour before overnight stimulation with 2.5 μM bovine serum albumin (BSA) or 2.5 μM Vpr and immunoblotted for cytochrome-c release (upper) and pro–caspase-8 cleavage (lower) in the cytosolic fraction. (D) Immunoblot of Hsp 70 in pellet and cytosolic fractions. (E) Isolated mitochondria were treated overnight with methanol (▪), 7 μM Nfv (░), or 50 μM BA (▤) before being stimulated with 2.5 μM Vpr or 5 mM ATR. Loss of Δψm was assessed using DiOC6.

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