Figure 1.
Acute codepletion of NR4A1/3 leads to loss of quiescence and increased proliferation of HCSs. (A) Experimental design for tamoxifen-dependent depletion of Nr4a1 in CDKO mice, using 4 daily treatments with tamoxifen (Nr4a1fl/fl; Nr4a3−/−; Rosa26-ERT2). (B) NR4A1 depletion efficiency measured by quantitative reverse transcription polymerase chain reaction (RT-qPCR) in HSCs after 4 daily tamoxifen injections (n = 3). (C) Representative flow cytometry plots illustrating subfractionation strategy of the HSPC (LSK) compartment to identify HSCs and early progenitors (MPP, HPC1, HPC2), based on surface expression of CD150 and CD48.65 (D) Quantitation of HSPC (left and center, n = 5 CDKO and 3 control) and lineage-restricted progenitor cell frequencies (right, n = 3) at 4 days after acute NR4A1/3 codepletion. (E) Bone marrow cellularity after acute NR4A1/3 codepletion (n = 3). (F) Frequency of HSPCs using CD34, Flt3, CD48, and CD150 markers (n = 4). For F, statistical significance was calculated between wild-type and CDKO samples. Results expressed as mean ± SD. *P ≤ .05; **P ≤ .01; ***P ≤ .001. CLP, common lymphoid progenitors (Lin−CD11c−CD27+IL7r+Flt3+Ly6d−); CMP, common myeloid progenitors (Lin−Sca1−Kit+CD16/32−CD34+); GMP, granulocyte-macrophage progenitors (Lin−Sca1−Kit+CD16/32+CD34+); MEP, megakaryocyte-erythrocyte progenitors (Lin−Sca1−Kit+CD16/32−CD34−).