Figure 5.
Figure 5. Transgenic expression of ASXL1aa1-587 affects HSC pool in vivo. (A) Flow cytometric analysis of Gr-1+/Mac1+ cell population in PB of representative WT (left) and Asxl1Y588XTg mice (right, 8 months old). (B) Quantitation of the percent of Gr-1+/Mac1+ cell populations in PB (*P = .024), BM (P = .074), and spleen (P = .080) of WT and Asxl1Y588XTg mice. Data are presented as mean ± SEM from 8 to 11 WT and Asxl1Y588XTg mice (8-19 months old). Unpaired Student t test was used to assess statistical significance. (C) Flow cytometric analysis of LSK compartments in BM of representative WT and Asxl1Y588XTg mice (8-19 months old) (left). Cells are gated on Lin− cells. Quantitation of the percentage of LSK compartments in BM Lin− of WT and Asxl1Y588XTg mice (right), n = 8 per group; **P = .002. (D) Flow cytometric analysis of the percent LT-HSC, ST-HSC, and multipotent progenitor cell populations (LSK/CD34+/FLK2+) in the BM LSK cells of representative WT and Asxl1Y588XTg mice (8-19 months old) (left). Cells are gated on LSK cells. Quantitation of the percent LT-HSC (P = .089) and ST-HSC (***P = .0006) populations in the BM Lin− cells of each genotype of mice (right). Unpaired Student t test was used to assess statistical significance. (E) Flow cytometric analysis of the GMP, common myeloid progenitor, and MEP populations in the BM LKS− cells of representative WT and Asxl1Y588XTg mice (8-19 months old) (left). Cells are gated on LKS− cells. Quantitation of the percent GMP (**P = .002) and MEP (**P = .0098) populations in the BM Lin− cells of each genotype of mice (right). Blue square, MPN; red square, leukemia; blue triangle, MDS/MPN; red triangle, MDS. (F) Colonies from 15 000 bone marrow mononuclear cells of WT and Asxl1Y588XTg mice. Blue bars, CFU-granulocytes/macrophages (GM); green bars, burst forming unit-erythrocyte (BFU-E); red bars, granulocyte, erythroid, macrophage, megakaryocyte (GEMM). Three mice per genotype were analyzed. ***P = .000424. (G) Serial cell replating assays using whole BM cells (3 mice per genotype) were performed to determine HSC self-renewal capability. A total of 15 000 bone marrow mononuclear cells were used for each methylcellulose cultures. The cells were replated weekly for 4 weeks. *P < .05. (H) Monthly assessment of donor chimerism (line II) in the peripheral blood of recipient animals is shown up to 16 weeks after transplant (n = 5 recipient mice were used for each genotype).

Transgenic expression of ASXL1aa1-587affects HSC pool in vivo. (A) Flow cytometric analysis of Gr-1+/Mac1+ cell population in PB of representative WT (left) and Asxl1Y588XTg mice (right, 8 months old). (B) Quantitation of the percent of Gr-1+/Mac1+ cell populations in PB (*P = .024), BM (P = .074), and spleen (P = .080) of WT and Asxl1Y588XTg mice. Data are presented as mean ± SEM from 8 to 11 WT and Asxl1Y588XTg mice (8-19 months old). Unpaired Student t test was used to assess statistical significance. (C) Flow cytometric analysis of LSK compartments in BM of representative WT and Asxl1Y588XTg mice (8-19 months old) (left). Cells are gated on Lin cells. Quantitation of the percentage of LSK compartments in BM Lin of WT and Asxl1Y588XTg mice (right), n = 8 per group; **P = .002. (D) Flow cytometric analysis of the percent LT-HSC, ST-HSC, and multipotent progenitor cell populations (LSK/CD34+/FLK2+) in the BM LSK cells of representative WT and Asxl1Y588XTg mice (8-19 months old) (left). Cells are gated on LSK cells. Quantitation of the percent LT-HSC (P = .089) and ST-HSC (***P = .0006) populations in the BM Lin cells of each genotype of mice (right). Unpaired Student t test was used to assess statistical significance. (E) Flow cytometric analysis of the GMP, common myeloid progenitor, and MEP populations in the BM LKS cells of representative WT and Asxl1Y588XTg mice (8-19 months old) (left). Cells are gated on LKS cells. Quantitation of the percent GMP (**P = .002) and MEP (**P = .0098) populations in the BM Lin cells of each genotype of mice (right). Blue square, MPN; red square, leukemia; blue triangle, MDS/MPN; red triangle, MDS. (F) Colonies from 15 000 bone marrow mononuclear cells of WT and Asxl1Y588XTg mice. Blue bars, CFU-granulocytes/macrophages (GM); green bars, burst forming unit-erythrocyte (BFU-E); red bars, granulocyte, erythroid, macrophage, megakaryocyte (GEMM). Three mice per genotype were analyzed. ***P = .000424. (G) Serial cell replating assays using whole BM cells (3 mice per genotype) were performed to determine HSC self-renewal capability. A total of 15 000 bone marrow mononuclear cells were used for each methylcellulose cultures. The cells were replated weekly for 4 weeks. *P < .05. (H) Monthly assessment of donor chimerism (line II) in the peripheral blood of recipient animals is shown up to 16 weeks after transplant (n = 5 recipient mice were used for each genotype).

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