Figure 5
Figure 5. DEK is necessary for normal granulocytic differentiation of CD34+ cells. BM-derived CD34+ cells were transduced with lentiviral particles carrying shRNA sequences that targeted either DEK (shDEK1 or shDEK2) or an insertless construct as a negative control (KH1), or shRNA sequences targeting DEK #13104 and 04 or a nontargeting sequence (NT) as a negative control (Mission pLKO.1-puro UbC-TurboGFP vector, SHC014; Sigma-Aldrich; supplemental Table 3). After 3 days, separate aliquots of transduced cell cultures were assayed for either DEK protein expression or differentiation capacity. Cells were enriched for a GFPhigh population and then probed by Western blot using 2 different anti-DEK Abs to determine the efficiency of DEK depletion through use of KH1 (A) or Mission (B) constructs. TATA-binding protein was used as a loading control. GFPhigh enriched populations (1000 cells) from KH1 (C) and Mission (D) transduction constructs were plated in triplicate in MethoCult SF complete methylcellulose medium supplemented with cytokines the rhSCF, rhGM-CSF, rhG-CSF, rhIL-3, and rhIL-6. Colonies were scored after 14 days of incubation according to morphologic criteria: CFU-GM, CFU-GMM, CFU-G, or CFU-M. Each bar represents the mean of triplicate measurements ± SEM. (E-H) Transduced cells were incubated in the presence of rhG-CSF (20 ng/mL) for up to 10 days to induce granulocytic differentiation. Expression of the myeloid surface markers CD11b (E-F) and CD15 (G-H) were assessed after 7 or 10 days as indicated. Each bar represents the mean of 2 independent experiments ± SEM. Expression of CEBPE (I) and GCSFR3 (J) mRNA in GFPhigh populations carrying KH1 transduction constructs after G-CSF treatment for 0 and 4 days. Expression levels are normalized against mRNA expression of 36B4. Error bars indicate the SD resulting from 2 independent experiments performed in triplicate. ***P < .001; **P < .01; *P < .05.

DEK is necessary for normal granulocytic differentiation of CD34+ cells. BM-derived CD34+ cells were transduced with lentiviral particles carrying shRNA sequences that targeted either DEK (shDEK1 or shDEK2) or an insertless construct as a negative control (KH1), or shRNA sequences targeting DEK #13104 and 04 or a nontargeting sequence (NT) as a negative control (Mission pLKO.1-puro UbC-TurboGFP vector, SHC014; Sigma-Aldrich; supplemental Table 3). After 3 days, separate aliquots of transduced cell cultures were assayed for either DEK protein expression or differentiation capacity. Cells were enriched for a GFPhigh population and then probed by Western blot using 2 different anti-DEK Abs to determine the efficiency of DEK depletion through use of KH1 (A) or Mission (B) constructs. TATA-binding protein was used as a loading control. GFPhigh enriched populations (1000 cells) from KH1 (C) and Mission (D) transduction constructs were plated in triplicate in MethoCult SF complete methylcellulose medium supplemented with cytokines the rhSCF, rhGM-CSF, rhG-CSF, rhIL-3, and rhIL-6. Colonies were scored after 14 days of incubation according to morphologic criteria: CFU-GM, CFU-GMM, CFU-G, or CFU-M. Each bar represents the mean of triplicate measurements ± SEM. (E-H) Transduced cells were incubated in the presence of rhG-CSF (20 ng/mL) for up to 10 days to induce granulocytic differentiation. Expression of the myeloid surface markers CD11b (E-F) and CD15 (G-H) were assessed after 7 or 10 days as indicated. Each bar represents the mean of 2 independent experiments ± SEM. Expression of CEBPE (I) and GCSFR3 (J) mRNA in GFPhigh populations carrying KH1 transduction constructs after G-CSF treatment for 0 and 4 days. Expression levels are normalized against mRNA expression of 36B4. Error bars indicate the SD resulting from 2 independent experiments performed in triplicate. ***P < .001; **P < .01; *P < .05.

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