Figure 1.
JMJD6 is required for steady-state multilineage hematopoiesis, whereas Jmjd6-deficient HSCs have a normal apoptotic and cell cycle status. (A) Relative levels of Jmjd6 messenger RNA (normalized to Hprt) in cells isolated from BM of 8- to 12-week-old adult C57BL/6 mice: LSKCD48−CD150+ HSCs, LSKCD48−CD150− MPPs, primitive HPCs (ie, LSKCD48+CD150− HPC-1 and LSKCD48+CD150+ HPC-2 populations), LSKs, and LK MPPs (n = 3). Data are mean ± SEM. (B) The expression of Jmjd6 in HSCs (LSKCD34−CD135−), MPP1 (LSKCD34+CD135−CD150+CD48−), MPP2 (LSKCD34+CD135−CD150+CD48+), MPP3 (LSKCD34+CD135−CD150−CD48+), and lymphoid-primed multipotent progenitor (LMPP)/MPP4 (LSKCD34+CD135+) populations, as well as in CMP (LKCD34+FcγRII/IIIlow), GMP (LKCD34+FcγRII/IIIhigh), and MEP (LKCD34−FcγRII/IIIlow) compartments, determined using single-cell SMART-seq2.29 Data are mean ± SEM. (C) Jmjd6 expression in HSCs and indicated committed progenitor cell compartments determined by 10× genomics single-cell RNA-seq.30 Bins represent clusters annotated via marker genes. Data are mean ± SEM. Ery, erythrocytes. (D) Genomic structure of the conditional Jmjd6 allele. Exon 3 is flanked by LoxP sites (red triangles). Following Cre-mediated recombination, exon 3 is excised, resulting in a frameshift mutation and a non-sense–mediated decay. (E) Levels of Jmjd6 messenger RNA in Jmjd6fl/fl;Vav-iCre (Jmjd6cKO) and control Jmjd6fl/fl (Jmjd6CTL) BM c-Kit+ cells (n = 4). Data are mean ± SEM. (F) Western blots for JMJD6 and β-actin from BM c-Kit+ cells from Jmjd6cKO and Jmjd6CTL mice (n = 3). (G) PB counts of white blood cells (WBCs), CD19+B220+ B cells, CD4+ and CD8+ T cells, and CD11b+Gr-1+ myeloid cells in 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 9-10). Data are mean ± SEM. (H) Total BM cellularity of Jmjd6cKO and Jmjd6CTL 8- to 10-week-old mice (2 femurs and 2 tibias) (n = 13-16). Data are mean ± SEM. (I) Total numbers of CMPs (LKCD34+FcγRII/IIIlow), GMPs (LKCD34+FcγRII/IIIhigh), MEPs (LKCD34−FcγRII/IIIlow), and CLPs (Lin−Sca-1lowc-KitlowCD127+CD135+) in BM from 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 13-16). Data are mean ± SEM. (J-K) Total numbers of HSCs, MPPs, HPC-1, and HPC-2 populations in BM of Jmjd6cKO and Jmjd6CTL mice. (J) Eight- to 10-week-old mice (n = 13-16). (K) Fifty-two–week-old mice (n = 6-9). Data are mean ± SEM. (L) Fold change in HSC, MPP, HPC-1, and HPC-2 populations in 52-week-old vs 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 6-13). (M) Percentage of DAPI−Annexin V+ and DAPI+Annexin V+ cells in HSCs, MPPs, HPC-1, and HPC-2 populations in BM from 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 6). Data are mean ± SEM. (N) Percentage of HSCs from 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice in the G0 (DAPI−Ki67−), G1 (DAPI−Ki67+), and G2/S/M (DAPI+Ki67+) phases of the cell cycle (n = 6-7). Data are mean ± SEM. *P < .05, **P < .01, ***P < .001, ****P < .0001, Mann-Whitney U test.

JMJD6 is required for steady-state multilineage hematopoiesis, whereas Jmjd6-deficient HSCs have a normal apoptotic and cell cycle status. (A) Relative levels of Jmjd6 messenger RNA (normalized to Hprt) in cells isolated from BM of 8- to 12-week-old adult C57BL/6 mice: LSKCD48CD150+ HSCs, LSKCD48CD150 MPPs, primitive HPCs (ie, LSKCD48+CD150 HPC-1 and LSKCD48+CD150+ HPC-2 populations), LSKs, and LK MPPs (n = 3). Data are mean ± SEM. (B) The expression of Jmjd6 in HSCs (LSKCD34CD135), MPP1 (LSKCD34+CD135CD150+CD48), MPP2 (LSKCD34+CD135CD150+CD48+), MPP3 (LSKCD34+CD135CD150CD48+), and lymphoid-primed multipotent progenitor (LMPP)/MPP4 (LSKCD34+CD135+) populations, as well as in CMP (LKCD34+FcγRII/IIIlow), GMP (LKCD34+FcγRII/IIIhigh), and MEP (LKCD34FcγRII/IIIlow) compartments, determined using single-cell SMART-seq2.29  Data are mean ± SEM. (C) Jmjd6 expression in HSCs and indicated committed progenitor cell compartments determined by 10× genomics single-cell RNA-seq.30  Bins represent clusters annotated via marker genes. Data are mean ± SEM. Ery, erythrocytes. (D) Genomic structure of the conditional Jmjd6 allele. Exon 3 is flanked by LoxP sites (red triangles). Following Cre-mediated recombination, exon 3 is excised, resulting in a frameshift mutation and a non-sense–mediated decay. (E) Levels of Jmjd6 messenger RNA in Jmjd6fl/fl;Vav-iCre (Jmjd6cKO) and control Jmjd6fl/fl (Jmjd6CTL) BM c-Kit+ cells (n = 4). Data are mean ± SEM. (F) Western blots for JMJD6 and β-actin from BM c-Kit+ cells from Jmjd6cKO and Jmjd6CTL mice (n = 3). (G) PB counts of white blood cells (WBCs), CD19+B220+ B cells, CD4+ and CD8+ T cells, and CD11b+Gr-1+ myeloid cells in 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 9-10). Data are mean ± SEM. (H) Total BM cellularity of Jmjd6cKO and Jmjd6CTL 8- to 10-week-old mice (2 femurs and 2 tibias) (n = 13-16). Data are mean ± SEM. (I) Total numbers of CMPs (LKCD34+FcγRII/IIIlow), GMPs (LKCD34+FcγRII/IIIhigh), MEPs (LKCD34FcγRII/IIIlow), and CLPs (LinSca-1lowc-KitlowCD127+CD135+) in BM from 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 13-16). Data are mean ± SEM. (J-K) Total numbers of HSCs, MPPs, HPC-1, and HPC-2 populations in BM of Jmjd6cKO and Jmjd6CTL mice. (J) Eight- to 10-week-old mice (n = 13-16). (K) Fifty-two–week-old mice (n = 6-9). Data are mean ± SEM. (L) Fold change in HSC, MPP, HPC-1, and HPC-2 populations in 52-week-old vs 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 6-13). (M) Percentage of DAPIAnnexin V+ and DAPI+Annexin V+ cells in HSCs, MPPs, HPC-1, and HPC-2 populations in BM from 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice (n = 6). Data are mean ± SEM. (N) Percentage of HSCs from 8- to 10-week-old Jmjd6cKO and Jmjd6CTL mice in the G0 (DAPIKi67), G1 (DAPIKi67+), and G2/S/M (DAPI+Ki67+) phases of the cell cycle (n = 6-7). Data are mean ± SEM. *P < .05, **P < .01, ***P < .001, ****P < .0001, Mann-Whitney U test.

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