Figure 2
Figure 2. Analysis of the HOXA transforming potential in primary hematopoietic cells. (A) Schematic map of the retroviral constructs used in this study. The expression of the HA-tagged HOXA cDNAs is driven by the long terminal repeat (LTR) promoter of pMSCVhygro (Ψ-packaging signal), whereas the hygromycin resistance gene is under control of a phosphoglycerate kinase (pgk) promoter. (B) HA-specific immunoblot of cellular proteins extracted from retroviral packaging cell lines transfected as indicated. To exclude a potential spill-over of HA-HOXA11 into the HA-HOXA13 lane, expression of HA-HOXA13 is shown again next to a vector control in a separate blot. Please note that because of the highly acidic carboxy-terminus, HA-HOXA7 migrates aberrantly slow in sodium dodecyl sulfate–polyacrylamide gel electrophoresis. (C) Serial replating assays of HOXA-transduced cells. The figure shows colonies arising after 3 replating rounds. Cells were transduced with HOXA genes either individually or in combination with Meis1 as indicated. Two typical examples for each construct are shown of up to 4 experiments performed in total. (D) Replating assays with Meis1. Transduction of Meis1 alone did not have any effect on hematopoietic differentiation, as evidenced by a lack of colony-forming capacity in replating assays like those described previously. (E) Generation of HOXA-transformed cell lines. HOXA or HOXA/Meis1-transduced cells that were able to generate permanently growing cell lines (> 2 months continuously in culture) at least twice in 3 attempts are marked by filled squares. HOXA7 yielded lines only in the presence of Meis1.

Analysis of the HOXA transforming potential in primary hematopoietic cells. (A) Schematic map of the retroviral constructs used in this study. The expression of the HA-tagged HOXA cDNAs is driven by the long terminal repeat (LTR) promoter of pMSCVhygro (Ψ-packaging signal), whereas the hygromycin resistance gene is under control of a phosphoglycerate kinase (pgk) promoter. (B) HA-specific immunoblot of cellular proteins extracted from retroviral packaging cell lines transfected as indicated. To exclude a potential spill-over of HA-HOXA11 into the HA-HOXA13 lane, expression of HA-HOXA13 is shown again next to a vector control in a separate blot. Please note that because of the highly acidic carboxy-terminus, HA-HOXA7 migrates aberrantly slow in sodium dodecyl sulfate–polyacrylamide gel electrophoresis. (C) Serial replating assays of HOXA-transduced cells. The figure shows colonies arising after 3 replating rounds. Cells were transduced with HOXA genes either individually or in combination with Meis1 as indicated. Two typical examples for each construct are shown of up to 4 experiments performed in total. (D) Replating assays with Meis1. Transduction of Meis1 alone did not have any effect on hematopoietic differentiation, as evidenced by a lack of colony-forming capacity in replating assays like those described previously. (E) Generation of HOXA-transformed cell lines. HOXA or HOXA/Meis1-transduced cells that were able to generate permanently growing cell lines (> 2 months continuously in culture) at least twice in 3 attempts are marked by filled squares. HOXA7 yielded lines only in the presence of Meis1.

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