Figure 4
Figure 4. Increasing proteasome workload through ER stress sensitizes MMCs to PIs. Pharmacologic ER stressors increase proteasome workload and PI-induced cytotoxicity in MMCs. (A) FACS analysis of apoptosis upon treatment with tunicamycin (Tm; 2.5 μg/mL) or bortezomib (Btz; 10 nM for U266 and 1 nM for MM.1S), alone or together for 48 hours. Top panels show the level of XBP-1 splicing after 24 hours (u and s for unspliced and spliced, respectively). (B) Twenty-four–hour treatment with Tm (2.5 μg/mL) and Btz (5 nM) synergistically causes ER stress (XBP-1 splicing; top panel) and accumulation of UbG76V-GFP (bottom overlay FACS histogram) in engineered U266 cells. (C) Forty-eight–hour treatment with Tm and Btz triggers synergistic death of engineered U266 cells. Cell death was assessed by modifications of physical parameters by FACS. One representative experiment is shown.

Increasing proteasome workload through ER stress sensitizes MMCs to PIs. Pharmacologic ER stressors increase proteasome workload and PI-induced cytotoxicity in MMCs. (A) FACS analysis of apoptosis upon treatment with tunicamycin (Tm; 2.5 μg/mL) or bortezomib (Btz; 10 nM for U266 and 1 nM for MM.1S), alone or together for 48 hours. Top panels show the level of XBP-1 splicing after 24 hours (u and s for unspliced and spliced, respectively). (B) Twenty-four–hour treatment with Tm (2.5 μg/mL) and Btz (5 nM) synergistically causes ER stress (XBP-1 splicing; top panel) and accumulation of UbG76V-GFP (bottom overlay FACS histogram) in engineered U266 cells. (C) Forty-eight–hour treatment with Tm and Btz triggers synergistic death of engineered U266 cells. Cell death was assessed by modifications of physical parameters by FACS. One representative experiment is shown.

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