Figure 1
Figure 1. Efficient immortalization of myeloid progenitors by Setbp1 expression. (A) Schematic diagram of the immortalization procedure. (B) Representative cytospin preparation and Wright-Giemsa staining of cells infected with Setbp1 (top panel) or empty retrovirus (bottom panel) at 1 month after infection. Original magnification ×400. Images were obtained using a Nikon Eclipse E800 microscope and a Qimaging Micropublisher 5.0 digital camera. (C) Cytospin preparation of Setbp1-immortalized cells (BM70 and P3 population) before and after treatment with G-CSF for 2 days. BM70 cells are immortalized by insertional activation of endogenous Setbp1.12,13 Original magnification ×400. (D) Southern blotting analysis of viral integrations present in 6 Setbp1-immortalized myeloid progenitor populations (P1-P6) using a GFP-specific probe. Seven ug of genomic DNA from each population was digested with EcoRI, resulting the generation of a single GFP-containing DNA fragment from each provirus. Each band represents an independent integration. (E) Real-time RT-PCR analysis of total RNA isolated from purified LSK, CMP, and GMP populations of C57BL/6 mice using Setbp1-specific primers. Relative expression levels were calculated by normalizing to β-actin mRNA levels in the same sample and also in LSK cells. The mean and SD of each relative expression level is shown.

Efficient immortalization of myeloid progenitors by Setbp1 expression. (A) Schematic diagram of the immortalization procedure. (B) Representative cytospin preparation and Wright-Giemsa staining of cells infected with Setbp1 (top panel) or empty retrovirus (bottom panel) at 1 month after infection. Original magnification ×400. Images were obtained using a Nikon Eclipse E800 microscope and a Qimaging Micropublisher 5.0 digital camera. (C) Cytospin preparation of Setbp1-immortalized cells (BM70 and P3 population) before and after treatment with G-CSF for 2 days. BM70 cells are immortalized by insertional activation of endogenous Setbp1.12,13  Original magnification ×400. (D) Southern blotting analysis of viral integrations present in 6 Setbp1-immortalized myeloid progenitor populations (P1-P6) using a GFP-specific probe. Seven ug of genomic DNA from each population was digested with EcoRI, resulting the generation of a single GFP-containing DNA fragment from each provirus. Each band represents an independent integration. (E) Real-time RT-PCR analysis of total RNA isolated from purified LSK, CMP, and GMP populations of C57BL/6 mice using Setbp1-specific primers. Relative expression levels were calculated by normalizing to β-actin mRNA levels in the same sample and also in LSK cells. The mean and SD of each relative expression level is shown.

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