Figure 6
Figure 6. Pharmacologic inhibition of ROS formation inhibits FLT3 ITD–mediated cell transformation in a DEP-1–dependent manner. (A) 32D cells, stably transduced with FLT3 ITD, and additionally nontargeting shRNA (control), or DEP-1 targeting shRNA (as indicated), were subjected to colony formation assays in methylcellulose in absence or presence of 1μM DPI (as indicated) for 6 days. Left panel: example images. Pictures were taken with a 4× magnification objective lens using an Olympus CKX41 microscope equipped with a CAMEDIA C-7070 camera (Olympus). Right panel: quantification of colony formation. Only colonies > 0.4 mm were counted. Knockdown efficiencies were assessed by qRT-PCR and by immunoblotting after the treatment period, and are depicted under the graph. Note also equal DEP-1 expression levels in the cells harboring control shRNA. (B) The cells were treated with DPI or were mock-treated in suspension culture for 6 hours, and subsequently lysed and subjected to immunoblotting for assessing STAT5 (left panel) and FLT3 ITD (right panel) activation (representative experiment of 3 with consistent results). (C) Same experiment as in panel A, except that treatment was performed in absence or presence of 5mM TROLOX (TX).

Pharmacologic inhibition of ROS formation inhibits FLT3 ITD–mediated cell transformation in a DEP-1–dependent manner. (A) 32D cells, stably transduced with FLT3 ITD, and additionally nontargeting shRNA (control), or DEP-1 targeting shRNA (as indicated), were subjected to colony formation assays in methylcellulose in absence or presence of 1μM DPI (as indicated) for 6 days. Left panel: example images. Pictures were taken with a 4× magnification objective lens using an Olympus CKX41 microscope equipped with a CAMEDIA C-7070 camera (Olympus). Right panel: quantification of colony formation. Only colonies > 0.4 mm were counted. Knockdown efficiencies were assessed by qRT-PCR and by immunoblotting after the treatment period, and are depicted under the graph. Note also equal DEP-1 expression levels in the cells harboring control shRNA. (B) The cells were treated with DPI or were mock-treated in suspension culture for 6 hours, and subsequently lysed and subjected to immunoblotting for assessing STAT5 (left panel) and FLT3 ITD (right panel) activation (representative experiment of 3 with consistent results). (C) Same experiment as in panel A, except that treatment was performed in absence or presence of 5mM TROLOX (TX).

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