Figure 3
Figure 3. Examination of oncogenic effect of Bcl11a overexpression using the BMTT assay in mice. (A) The BMTT scheme used in this study. (B) Survival analysis on the BMTT-recipient mice, which received Bcl11a- or empty vector (used as a negative control)–transduced Nf1-intact (“Nf1(+/+).EV” and “Nf1(+/+). Bcl11a”) or Nf1-deficient bone marrow cells (“Nf1(Flox/Fcr).EV” and “Nf1(Flox/Fcr).Bcl11a”). (C) Histopathologic examination of the Bcl11a-induced leukemia in the recipient mice. Hematoxylin and eosin staining. Representative images with magnification of 60-fold are shown here. Bars represent 25 μm. Slides were viewed with a Nikon Eclipse E600 bright light microscope (Nikon, Tokyo, Japan) using a Nikon Plan Fluor 40×/0.75 objective lens. Images were acquired using a Spot Insight digital camera (model 14.2, Color Mosaic; Diagnostic Instruments, Sterling Heights, MI), and were processed with Spotsoftware Advanced (version 4.6 for Windows; Diagnostic Instruments) and Adobe Photoshop version 7.0 software (Adobe Systems, San Jose, CA). (D) Determination of donor origin of the Bcl11a-induced leukemia developing in the BMTT-recipient mice. Antibodies staining for CD45.1 or CD45.2 cell-surface molecules were used. (E,F) Determination of cell-lineage origin of the Bcl11a leukemia developed in the BMTT-recipient mice. Antibodies against Mac-1, Gr-1, B220, or TCR-β were used to stain lymph nodes and bone marrows harvested from either healthy C57BL/6J mice or mice transplanted with Bcl11a-transduced Nf1-deficient bone marrow cells to collect evidence for acute myeloid leukemia (E) or T-cell acute lymphoid leukemia (F).

Examination of oncogenic effect of Bcl11a overexpression using the BMTT assay in mice. (A) The BMTT scheme used in this study. (B) Survival analysis on the BMTT-recipient mice, which received Bcl11a- or empty vector (used as a negative control)–transduced Nf1-intact (“Nf1(+/+).EV” and “Nf1(+/+). Bcl11a”) or Nf1-deficient bone marrow cells (“Nf1(Flox/Fcr).EV” and “Nf1(Flox/Fcr).Bcl11a”). (C) Histopathologic examination of the Bcl11a-induced leukemia in the recipient mice. Hematoxylin and eosin staining. Representative images with magnification of 60-fold are shown here. Bars represent 25 μm. Slides were viewed with a Nikon Eclipse E600 bright light microscope (Nikon, Tokyo, Japan) using a Nikon Plan Fluor 40×/0.75 objective lens. Images were acquired using a Spot Insight digital camera (model 14.2, Color Mosaic; Diagnostic Instruments, Sterling Heights, MI), and were processed with Spotsoftware Advanced (version 4.6 for Windows; Diagnostic Instruments) and Adobe Photoshop version 7.0 software (Adobe Systems, San Jose, CA). (D) Determination of donor origin of the Bcl11a-induced leukemia developing in the BMTT-recipient mice. Antibodies staining for CD45.1 or CD45.2 cell-surface molecules were used. (E,F) Determination of cell-lineage origin of the Bcl11a leukemia developed in the BMTT-recipient mice. Antibodies against Mac-1, Gr-1, B220, or TCR-β were used to stain lymph nodes and bone marrows harvested from either healthy C57BL/6J mice or mice transplanted with Bcl11a-transduced Nf1-deficient bone marrow cells to collect evidence for acute myeloid leukemia (E) or T-cell acute lymphoid leukemia (F).

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