Runx1−/− status leads to stem cell exhaustion. (A) Absolute number of KSL CD34−Flt3− cells, Lin− SP cells, KSL CD34+Flt3+ cells and KSL CD34+Flt3− cells per 0.5 million BM cells from Runx1+/+ and Runx1−/− mice of 2 distinct ages (10 and 40 weeks old). Each group comprises 3 to 4 mice. (B) Limiting dilution analysis using varying numbers of BM cells from 40-week-old CD45.2+Runx1+/+ (▲), or Runx1−/− (■) mice. Mice were considered negative when the percent chimerism was less than 1%. Left panel: estimated frequencies of the repopulating cells are indicated as vertical dashed lines (1 repopulating cell per indicated numbers of BM cells) for each genotype. Right panel: for each indicated number of transplanted cells from CD45.2+Runx1+/+ or Runx1−/− mice, the proportion of mice that are positive for test CD45.2+ cells is given as (number of positive mice)/(number of analyzed mice). Frequencies of HSCs were calculated using Poisson statistics. (C) GFP chimerism in PB of recipients of Runx1+/+ (n = 6) and Runx1−/− (n = 6) cells at 6 and 40 weeks after transplantation. Each open circle represents data from an individual mouse and each closed circle is the average of a cohort. Statistical difference using unpaired Student t test is given at the bottom. NS indicates not significant. (D) Kaplan-Meier survival curves of secondary recipients of mock MIG vector–transfected Runx1+/+ (dashed line; n = 10) and Runx1−/− (solid line; n = 10) BM cells. Circles represent end point of analysis.