Fig. 4.
Fig. 4. Activated Notch1 expands primitive RAG-1−/−hematopoietic cells in vivo and enhances the self-renewal of RAG-1−/− hematopoietic stem cells in serial bone marrow transplantation. / Competitive repopulation of C57BL/6 Ly5.1 mice (n = 5 for each group), lethally irradiated and transplanted with 2000 RAG-1−/−Sca1+lin−Ly5.2+bone marrow cells expressing control vector (MSCV-GFP) or activated Notch1 (MSCV-ICN/GFP) along with 1.5 × 105Ly5.1+ competing bone marrow cells. Bone marrow cells were stained 5 months after transplantation. (A) Bone marrow cells were stained for Sca1 and lineage markers (CD3, CD4, CD8, B220, Mac1, Gr-1, and Ter119) or Sca1 and c-kit or c-kit and Thy1. Plots represent fluorescence intensity for the indicated markers on the x-axis and Sca1 or c-kit on the y-axis in the GFP+Ly5.2+ cell population of the bone marrow of 3 representative animals. Numbers in corners represent percent of events within that quadrant or gate. (B) Charts show the average percentage ± SEM of Sca1+lin−, Sca1+c-kit+, or c-kit+Thy1low cells in the GFP+Ly5.2+ bone marrow population. The Student t test was used to analyze the data (Sca1+lin−, P = .002; Sca1+c-kit+, P = .01; c-kit+Thy1low, P = .03). (C) Charts show the average of total Sca1+lin− or Sca1+c-kit+ or c-kit+Thy1low cells ± SEM in the GFP+Ly5.2+ bone marrow of animals receiving transplants. The Student t test was used to analyze the data. (Sca1+lin−, P = .03; Sca1+c-kit+, P = .06; c-kit+Thy1low, P = .05). (D) After 1.5, 5, and 8 months the bone marrow of competitive repopulated animals was analyzed by flow cytometry for Sca1+lin−cells in GFP+Ly5.2+ bone marrow. Chart represents total number of Sca1+lin− cells at different time points. (E) Bone marrow cells of competitive repopulated animals were pooled for each group 6 weeks after transplantation (first transplant; n = 5) containing equal numbers of Sca1+lin−GFP+Ly5.2+cells and again transplanted into lethally irradiated C57BL/6 Ly5.1 mice. The bone marrow was analyzed after a further 5 months by flow cytometry (second transplant; n = 4). Bone marrow cells were stained for Ly5.2, Sca1, and lineage markers (CD3, CD4, CD8, B220, Mac1, Gr-1, and Ter119). Total Sca1+lin− cells, which were also GFP+Ly5.2+, were measured by flow cytometric analysis and total cell count of the bone marrow of competitive repopulated animals of the first and second transplant. Chart shows the average ± SEM of total Sca1+lin−GFP+Ly5.2+cells in the bone marrow.

Activated Notch1 expands primitive RAG-1−/−hematopoietic cells in vivo and enhances the self-renewal of RAG-1−/− hematopoietic stem cells in serial bone marrow transplantation.

Competitive repopulation of C57BL/6 Ly5.1 mice (n = 5 for each group), lethally irradiated and transplanted with 2000 RAG-1−/−Sca1+linLy5.2+bone marrow cells expressing control vector (MSCV-GFP) or activated Notch1 (MSCV-ICN/GFP) along with 1.5 × 105Ly5.1+ competing bone marrow cells. Bone marrow cells were stained 5 months after transplantation. (A) Bone marrow cells were stained for Sca1 and lineage markers (CD3, CD4, CD8, B220, Mac1, Gr-1, and Ter119) or Sca1 and c-kit or c-kit and Thy1. Plots represent fluorescence intensity for the indicated markers on the x-axis and Sca1 or c-kit on the y-axis in the GFP+Ly5.2+ cell population of the bone marrow of 3 representative animals. Numbers in corners represent percent of events within that quadrant or gate. (B) Charts show the average percentage ± SEM of Sca1+lin, Sca1+c-kit+, or c-kit+Thy1low cells in the GFP+Ly5.2+ bone marrow population. The Student t test was used to analyze the data (Sca1+lin, P = .002; Sca1+c-kit+, P = .01; c-kit+Thy1low, P = .03). (C) Charts show the average of total Sca1+lin or Sca1+c-kit+ or c-kit+Thy1low cells ± SEM in the GFP+Ly5.2+ bone marrow of animals receiving transplants. The Student t test was used to analyze the data. (Sca1+lin, P = .03; Sca1+c-kit+, P = .06; c-kit+Thy1low, P = .05). (D) After 1.5, 5, and 8 months the bone marrow of competitive repopulated animals was analyzed by flow cytometry for Sca1+lincells in GFP+Ly5.2+ bone marrow. Chart represents total number of Sca1+lin cells at different time points. (E) Bone marrow cells of competitive repopulated animals were pooled for each group 6 weeks after transplantation (first transplant; n = 5) containing equal numbers of Sca1+linGFP+Ly5.2+cells and again transplanted into lethally irradiated C57BL/6 Ly5.1 mice. The bone marrow was analyzed after a further 5 months by flow cytometry (second transplant; n = 4). Bone marrow cells were stained for Ly5.2, Sca1, and lineage markers (CD3, CD4, CD8, B220, Mac1, Gr-1, and Ter119). Total Sca1+lin cells, which were also GFP+Ly5.2+, were measured by flow cytometric analysis and total cell count of the bone marrow of competitive repopulated animals of the first and second transplant. Chart shows the average ± SEM of total Sca1+linGFP+Ly5.2+cells in the bone marrow.

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