Figure 7.
Upregulation of Cebpα and Cebpδ in MycV394DAML cells contributes to the partial differentiation phenotype. (A) Representative upregulated genes in MycV394-AML cells as identified from RNA sequencing are presented in a heatmap. (B) MycV394D-AML cells were collected at the indicated times after 4-OHT treatment as described in Figure 6G-H. The expression of Cebpα and Cebpδ was examined by qRT-PCR. (C) The expression of Cebpα and Cebpδ was examined by qRT-PCR in MSCV-, Myc- and MycV394D-transduced HSPCs on day 4 after transduction. (D-E) The binding of Myc, MycV394D, and Miz1 to the promoters of the Cebpα or Cebpδ genes was examined in AML cells by ChIP/quantitative PCR (qPCR) assay. (F-G) H3K9Me3 and H3K9Ac status of the promoters of Cebpα or Cebpδ genes were examined by ChIP/qPCR assay. (H-J) Cebpα or Cebpδ or both were knocked down in MycV394D AML cells by short hairpin RNA (shRNA) specific for Cebpα (shCα) or Cebpδ (shCδ) (H). The third replating CFC (I) and response to DNR or Ara-C treatment (J) of the gene knockdown cells were compared with scrambled shRNA (scr)-transduced MycV394D AML cells. Myc AML cells were used as controls. (K-M) Cebpα or Cebpδ or both were overexpressed in Myc AML cells by viral transduction (K). The third replating CFC (L) and response to DNR or Ara-C treatment (M) of the gene overexpressed cells were compared with empty vector (EV)-transduced Myc-AML cells. **P < .01, ##P < .01, and #P < .05, compared with corresponding Myc groups in panel J and corresponding EV groups in panel M. $$P < .01 and $P < .05, compared with corresponding scr groups. D, distal promoto; P, proximal promoter.

Upregulation of Cebpα and Cebpδ in MycV394DAML cells contributes to the partial differentiation phenotype. (A) Representative upregulated genes in MycV394-AML cells as identified from RNA sequencing are presented in a heatmap. (B) MycV394D-AML cells were collected at the indicated times after 4-OHT treatment as described in Figure 6G-H. The expression of Cebpα and Cebpδ was examined by qRT-PCR. (C) The expression of Cebpα and Cebpδ was examined by qRT-PCR in MSCV-, Myc- and MycV394D-transduced HSPCs on day 4 after transduction. (D-E) The binding of Myc, MycV394D, and Miz1 to the promoters of the Cebpα or Cebpδ genes was examined in AML cells by ChIP/quantitative PCR (qPCR) assay. (F-G) H3K9Me3 and H3K9Ac status of the promoters of Cebpα or Cebpδ genes were examined by ChIP/qPCR assay. (H-J) Cebpα or Cebpδ or both were knocked down in MycV394D AML cells by short hairpin RNA (shRNA) specific for Cebpα (shCα) or Cebpδ (shCδ) (H). The third replating CFC (I) and response to DNR or Ara-C treatment (J) of the gene knockdown cells were compared with scrambled shRNA (scr)-transduced MycV394D AML cells. Myc AML cells were used as controls. (K-M) Cebpα or Cebpδ or both were overexpressed in Myc AML cells by viral transduction (K). The third replating CFC (L) and response to DNR or Ara-C treatment (M) of the gene overexpressed cells were compared with empty vector (EV)-transduced Myc-AML cells. **P < .01, ##P < .01, and #P < .05, compared with corresponding Myc groups in panel J and corresponding EV groups in panel M. $$P < .01 and $P < .05, compared with corresponding scr groups. D, distal promoto; P, proximal promoter.

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