Fig. 3. Rapid inhibition of VP-16–induced apoptosis by H2O2. / JLP 119 cells were treated for 4 hours with 8.5 μmol/L VP-16 in the presence or absence of 75 μmol/L H2O2, added 30 minutes after the VP-16. Cell death was assayed by fluorescence microscopy, as described in “Materials and methods.”
Fig. 3.

Rapid inhibition of VP-16–induced apoptosis by H2O2.

JLP 119 cells were treated for 4 hours with 8.5 μmol/L VP-16 in the presence or absence of 75 μmol/L H2O2, added 30 minutes after the VP-16. Cell death was assayed by fluorescence microscopy, as described in “Materials and methods.”

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