Figure 1
Figure 1. BM content of HSPCs is reduced in number in MllPTD/WTmice. (A) BM of age- and sex-matched littermate WT controls and MllPTD/WT mice were analyzed at 2, 4, and 12 months of age, based on the immunophenotype analysis. Representative flow cytometry (FACS) contour diagram shows the frequency of LSK and LSK/SLAM+ BM cells of WT and MllPTD/WT mice. Shown is a representative of 8 experiments with similar results. (B) Absolute number of LSK cells of WT and MllPTD/WT mice. MllPTD/WT LSK population is reduced in absolute number during aging (n = 8). The difference between control and MllPTD/WT was significant at 8 and 12 months. *P < .05. (C) Absolute number of LSK/SLAM+ cells of WT and MllPTD/WT mice. MllPTD/WT LSK/SLAM+ populations are reduced in absolute number during aging (n = 8). The difference between control and MllPTD/WT was significant at 4, 8, and 12 months. *P < .05. **P < .01. (D) Absolute number of progenitors HPC, GMP, common myeloid progenitor cells (Lin−c-Kit+Sca1−CD34+CD16/32mid; CMPs), and MEP of WT and MllPTD/WT mice. MllPTD/WT mice GMP population is increased at the expense of the MEP population (2 experiments, n = 8; 4-month-old mice were used). The differences of GMP and MEP between control and MllPTD/WT were significant (P < .05). (E) Apoptosis was checked by annexin V staining. Data are the mean percentage ± SD of annexin V+/7 AAD− and annexin V+/7 AAD+. *P < .05. **P < .01. Experiments were performed in duplicate groups for 4 mice at 4-month-old per genotype repeated in 3 separate experiments. (F) Cell-cycle analysis was performed with a BrdU flow kit. Percentage of cycling cells: G0/G1 and S/G2/M are shown for LK (Lin−Kit+) and LSK fractions (2 experiments, n = 4; 4-month-old mice were used). *P < .05. (G) H3K4 methylation in LSK fractions. BM cells were harvested and LSK cells were selected using autoMACS. Western blots were done using indicated antibodies (anti-H3K4me3, anti-H3K4me2, and anti-H3). Representative data were from 3 independent experiments.

BM content of HSPCs is reduced in number in MllPTD/WTmice. (A) BM of age- and sex-matched littermate WT controls and MllPTD/WT mice were analyzed at 2, 4, and 12 months of age, based on the immunophenotype analysis. Representative flow cytometry (FACS) contour diagram shows the frequency of LSK and LSK/SLAM+ BM cells of WT and MllPTD/WT mice. Shown is a representative of 8 experiments with similar results. (B) Absolute number of LSK cells of WT and MllPTD/WT mice. MllPTD/WT LSK population is reduced in absolute number during aging (n = 8). The difference between control and MllPTD/WT was significant at 8 and 12 months. *P < .05. (C) Absolute number of LSK/SLAM+ cells of WT and MllPTD/WT mice. MllPTD/WT LSK/SLAM+ populations are reduced in absolute number during aging (n = 8). The difference between control and MllPTD/WT was significant at 4, 8, and 12 months. *P < .05. **P < .01. (D) Absolute number of progenitors HPC, GMP, common myeloid progenitor cells (Linc-Kit+Sca1CD34+CD16/32mid; CMPs), and MEP of WT and MllPTD/WT mice. MllPTD/WT mice GMP population is increased at the expense of the MEP population (2 experiments, n = 8; 4-month-old mice were used). The differences of GMP and MEP between control and MllPTD/WT were significant (P < .05). (E) Apoptosis was checked by annexin V staining. Data are the mean percentage ± SD of annexin V+/7 AAD and annexin V+/7 AAD+. *P < .05. **P < .01. Experiments were performed in duplicate groups for 4 mice at 4-month-old per genotype repeated in 3 separate experiments. (F) Cell-cycle analysis was performed with a BrdU flow kit. Percentage of cycling cells: G0/G1 and S/G2/M are shown for LK (LinKit+) and LSK fractions (2 experiments, n = 4; 4-month-old mice were used). *P < .05. (G) H3K4 methylation in LSK fractions. BM cells were harvested and LSK cells were selected using autoMACS. Western blots were done using indicated antibodies (anti-H3K4me3, anti-H3K4me2, and anti-H3). Representative data were from 3 independent experiments.

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