Figure 6
Figure 6. Akt/mTORC1 hyperactivity in Itpkb−/− HSC. (A-B) WT (solid) or Itpkb−/− (hatched) LSK cells were treated in vitro with medium or SCF ± cell-permeable IP4/PM or Akt-inhibitor VIII (Akt-I) and analyzed by FACS for T308-phosphorylated Akt (pAktT308) content. (A) Representative FACS data from 4 independent experiments. (B) pAktT308 median fluorescence intensity (MFI) in WT (black squares) or Itpkb−/− (gray circles) LSK cells, normalized to the MFI of unstimulated WT cells (n = 4). Statistical significance of genotype differences was determined by unpaired Student t test. (C) Total Akt protein content in WT or Itpkb−/− LSK cells. Shaded histogram, isotype control. (D) WT (solid) or Itpkb−/− (hatched) LSK cells treated as in (A) were analyzed for pAktT308 and phospho-ribosomal protein S6 (pS6S235/S236) content in LSK CD34−CD48−CD150+ LT-HSC, and MPP1-3 subpopulations. (E) Itpkb−/− or WT LT-HSC enriched GSEA gene sets associated with Akt/mTOR signaling and metabolic activation were identified as in Figure 3C. Gene set descriptions are shown in supplemental Table 5.

Akt/mTORC1 hyperactivity in Itpkb−/− HSC. (A-B) WT (solid) or Itpkb−/− (hatched) LSK cells were treated in vitro with medium or SCF ± cell-permeable IP4/PM or Akt-inhibitor VIII (Akt-I) and analyzed by FACS for T308-phosphorylated Akt (pAktT308) content. (A) Representative FACS data from 4 independent experiments. (B) pAktT308 median fluorescence intensity (MFI) in WT (black squares) or Itpkb−/− (gray circles) LSK cells, normalized to the MFI of unstimulated WT cells (n = 4). Statistical significance of genotype differences was determined by unpaired Student t test. (C) Total Akt protein content in WT or Itpkb−/− LSK cells. Shaded histogram, isotype control. (D) WT (solid) or Itpkb−/− (hatched) LSK cells treated as in (A) were analyzed for pAktT308 and phospho-ribosomal protein S6 (pS6S235/S236) content in LSK CD34CD48CD150+ LT-HSC, and MPP1-3 subpopulations. (E) Itpkb−/− or WT LT-HSC enriched GSEA gene sets associated with Akt/mTOR signaling and metabolic activation were identified as in Figure 3C. Gene set descriptions are shown in supplemental Table 5.

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