Figure 3. Cell viability and intracellular distribution of the DUB reporter in intact HeLa cells.

Cells incubated with 30 μM Peptide 4 were washed and counterstained with 4 μM ethidium homodimer (EthD-1) and 8 μM Hoechst. Channels were immediately imaged using Brightfield, FITC (peptide), DAPI (nucleus), and Rhodamine (viability assessed by Ethidium Homodimer) filters. Scale bar is 40 μm.