Figure 3.
PLAG1-S overexpression promotes self-renewal of long-term human HSCs. (A) Schematic of primary and secondary xenotransplantation in limiting dilution format. (B) Representative flow plots of human CD45+BFP+ multilineage (CD33+, CD19+) engraftment of primary recipient mice in injected femur. Percent human CD45+BFP+ engraftment in injected femur of primary recipient mice across multiple cell input doses. Dashed line indicates cutoff for calling engraftment, which was >0.5% human chimerism including both myeloid (CD45+BFP+CD33+) and lymphoid (CD45+BFP+CD19+) lineages. (C-D) Quantification of HSC frequency by ELDA45 of injected femur of primary recipient mice. Shaded area under the curve represents 95% confidence interval of HSC frequency. (E) Percent human CD45+BFP+ engraftment in injected femur of secondary recipient mice across multiple cell input doses. Dashed line indicates cutoff for calling engraftment, which was the same as for primary mice. (F-G) Quantification of HSC frequency by ELDA of injected femur or uninjected bone marrow of secondary recipient mice and of in vivo expansion. Shaded area under the curve represents 95% confidence interval of HSC frequency. Total BFP+ cells within whole-body BM of primary mice were extrapolated, as previously,47 based on femur and hind limb counts and proportional accounting from Colvin et al,107 and in vivo expansion is measured as the fold difference of total BFP+ HSCs in donor mice relative to total day 0 HSCs initially transplanted into the 6 donor mice. Data are presented as average ± SEM unless otherwise indicated. Each point represents 1 mouse. See also supplemental Figure 3.

PLAG1-S overexpression promotes self-renewal of long-term human HSCs. (A) Schematic of primary and secondary xenotransplantation in limiting dilution format. (B) Representative flow plots of human CD45+BFP+ multilineage (CD33+, CD19+) engraftment of primary recipient mice in injected femur. Percent human CD45+BFP+ engraftment in injected femur of primary recipient mice across multiple cell input doses. Dashed line indicates cutoff for calling engraftment, which was >0.5% human chimerism including both myeloid (CD45+BFP+CD33+) and lymphoid (CD45+BFP+CD19+) lineages. (C-D) Quantification of HSC frequency by ELDA45 of injected femur of primary recipient mice. Shaded area under the curve represents 95% confidence interval of HSC frequency. (E) Percent human CD45+BFP+ engraftment in injected femur of secondary recipient mice across multiple cell input doses. Dashed line indicates cutoff for calling engraftment, which was the same as for primary mice. (F-G) Quantification of HSC frequency by ELDA of injected femur or uninjected bone marrow of secondary recipient mice and of in vivo expansion. Shaded area under the curve represents 95% confidence interval of HSC frequency. Total BFP+ cells within whole-body BM of primary mice were extrapolated, as previously,47 based on femur and hind limb counts and proportional accounting from Colvin et al,107 and in vivo expansion is measured as the fold difference of total BFP+ HSCs in donor mice relative to total day 0 HSCs initially transplanted into the 6 donor mice. Data are presented as average ± SEM unless otherwise indicated. Each point represents 1 mouse. See also supplemental Figure 3.

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