![Deletion of Hoxa cluster genes in adult mice and transcriptome analysis of Hoxa−/− HSCs. (A) Bar graphs depicting absolute numbers of CD150+/CD48−/CD244−/LKS HSCs and CD150+/CD48−/CD244+/LKS MPPs in BM of Hoxa−/− and control mice (n = 4). BM cells isolated from femur and tibia 4 weeks after pIpC injection. (B) Polymerase chain reaction analysis showing the deletion of the Hoxa cluster in purified LKS cells at 4 weeks following the last pIpC injection (n = 5). (C) Engraftment of Hoxa−/− (n = 14) and control (n = 15) cells in the PB, BM, spleen, and thymus of recipient mice at ∼24 weeks after transplantation. Each dot represents a CD45.1 recipient mouse transplanted with 106 congenic CD45.2 BM cells. (D) Proportions of B (B220+), myeloid (Mac1+), T (CD3+), and erythroid (Ter119+) cells in PB of reconstituted mice shown in (C). (E) Scatterplot showing transcriptome analysis of genes that were up- (above axis) or downregulated (below axis) in Hoxa−/− vs WT control CD150+/CD48−/LKS cells sorted 1 month after the last pIpC injection. Values are expressed as average (log10 [(average RPKM)*1000 + 1]). Cut-off limit for showing gene identify was set at 3, representing a RPKM value of ∼0.1. Highlighted genes show 10-fold differences between the 2 groups. (F-G) Comparative expression of Hoxa (F) and Hoxb (G) genes in pairs of Hoxa−/− and control HSC samples (n = 3). *P < .05; **P < .01; ***P < .001. Cre, causes recombination; CT, cycle time; HPRT, hypoxanthine-guanine phosphoribosyltransferase; MPP, multipotent progenitors; RQ, relative quantification; Spl, spleen; Thy, thymus.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/127/1/10.1182_blood-2015-02-626390/5/87f1.jpeg?Expires=1722256364&Signature=qMUehRg5b9dTR48PJgICxL~Y3PBsaRFqLPMMBG~z~t2EQK2lHQQ8Qp1INrVz1u6aftlmBz2A~q30togWbNcSEOV-U9-BSRz3wOx27e1uQ~mAsQNGUmrWRc300EQ0qfeJNWmFzQn~hefq3WlK~-OD0HzwXp9eLVldQEok1AFuBkW6609AZZbkeb0mxvhWYDnkHCzlOKm9e07SPGNvS2DBpBUIqtLbU8ia2~vCpdS9y-y~1Kd6qi~Bcl29OemcGQil22vvP4toUCTtGWy5brkAeOMG9l3T2Po2Mnv~mVWDR6duenzs2y4WqR7mEmniLstdRgyGEiTGLFLriJYl~TUCqw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Deletion of Hoxa cluster genes in adult mice and transcriptome analysis of Hoxa−/− HSCs. (A) Bar graphs depicting absolute numbers of CD150+/CD48−/CD244−/LKS HSCs and CD150+/CD48−/CD244+/LKS MPPs in BM of Hoxa−/− and control mice (n = 4). BM cells isolated from femur and tibia 4 weeks after pIpC injection. (B) Polymerase chain reaction analysis showing the deletion of the Hoxa cluster in purified LKS cells at 4 weeks following the last pIpC injection (n = 5). (C) Engraftment of Hoxa−/− (n = 14) and control (n = 15) cells in the PB, BM, spleen, and thymus of recipient mice at ∼24 weeks after transplantation. Each dot represents a CD45.1 recipient mouse transplanted with 106 congenic CD45.2 BM cells. (D) Proportions of B (B220+), myeloid (Mac1+), T (CD3+), and erythroid (Ter119+) cells in PB of reconstituted mice shown in (C). (E) Scatterplot showing transcriptome analysis of genes that were up- (above axis) or downregulated (below axis) in Hoxa−/− vs WT control CD150+/CD48−/LKS cells sorted 1 month after the last pIpC injection. Values are expressed as average (log10 [(average RPKM)*1000 + 1]). Cut-off limit for showing gene identify was set at 3, representing a RPKM value of ∼0.1. Highlighted genes show 10-fold differences between the 2 groups. (F-G) Comparative expression of Hoxa (F) and Hoxb (G) genes in pairs of Hoxa−/− and control HSC samples (n = 3). *P < .05; **P < .01; ***P < .001. Cre, causes recombination; CT, cycle time; HPRT, hypoxanthine-guanine phosphoribosyltransferase; MPP, multipotent progenitors; RQ, relative quantification; Spl, spleen; Thy, thymus.
