Figure 3.
Figure 3. Analysis of primitive progenitors in Hmgb3–/Y mice. (A) Representative isolation of wild-type common lymphoid and myeloid progenitors by flow cytometry. (Ai) Lin– bone marrow isolated from wild-type mice. (Aii) CLP and HSC populations were isolated from c-kit and Sca-1 double-positive lin– bone marrow cells. Double-positive cells were further segregated into c-kitLO, Sca-1LO (solid box) and c-kitHI, Sca-1HI (dotted box) populations. Regions were drawn based on isotype staining of littermate control cells. (Aiii) The CMP population was isolated from c-kit+, Sca-1–, and IL-7Rα– lin– bone marrow cells. (Aiv) Further isolation of the HSC population based on IL-7Rα expression in c-kitHI, Sca-1HI cells. Approximately 90% of c-kitLO, Sca-1LO cells were IL-7Rα– (HSC phenotype). (Av) Isolation of the CLP population based on IL-7Rα expression in c-kitLO, Sca-1LO cells. Approximately 89% of c-kitLO, Sca-1LO cells were IL-7Rα+ (CLP phenotype). (Avi) Isolation of the CMP population based on FcγRII/III and CD34 expression in c-kit+, Sca-1–, and IL-7Rα– cells. Cells that are FcγRII/IIILO and CD34+ represent the CMP phenotype. (B) Average number of HSCs (lin–, c-kitHI, Sca-1HI, IL-7Rα–; n = 3), CLPs (lin–, c-kitLO, Sca-1LO, IL-7Rα+; n = 3), and CMPs (lin–, c-kit+, Sca-1–, IL-7Rα–, FcγRII/IIILO, CD34+; n = 4) as determined by the percentage of lineage-negative (lin–) bone marrow cells that stained positive for the HSC, CLP, or CMP phenotype. Staining was performed on lineage-depleted cells isolated from groups of 3 Hmgb3–/Y or wild-type mice prior to analysis by flow cytometry. The data represent the pooled results of 3 (HSCs and CLPs) or 4 (CMPs) independent experiments. (C) Mean CFU–Pre-B frequency generated from wild-type and Hmgb3–/Y CLP populations. CFU–Pre-B frequency within the CLP population was determined by scoring pre–B-cell colonies per 1000 cells cultured: wild-type (n = 8; 355 CFU–Pre-Bs counted); Hmgb3–/Y (n = 8; 890 CFU–Pre-Bs counted). The data represent the pooled results of 2 independent experiments. (D) Mean myeloid colony (CFU-C) frequency generated from wild-type and Hmgb3–/Y CMP populations. Myeloid CFU-C frequency within the CMP population was determined by scoring CFU-GM, BFU-E, and CFU-GEMM colonies per 500 cells cultured: wild-type (n = 10; 813 CFU-GMs, 177 BFU-Es, and 91 CFU-GEMMs counted); Hmgb3–/Y (n = 10; 239 CFU-GMs, 47 BFU-Es, and 17 CFU-GEMMs counted). The data represent the pooled results of 2 independent experiments. P values in panels B-D were determined by Student t test. In panels B-D, error bars represent standard deviation.

Analysis of primitive progenitors in Hmgb3/Y mice. (A) Representative isolation of wild-type common lymphoid and myeloid progenitors by flow cytometry. (Ai) Lin bone marrow isolated from wild-type mice. (Aii) CLP and HSC populations were isolated from c-kit and Sca-1 double-positive lin bone marrow cells. Double-positive cells were further segregated into c-kitLO, Sca-1LO (solid box) and c-kitHI, Sca-1HI (dotted box) populations. Regions were drawn based on isotype staining of littermate control cells. (Aiii) The CMP population was isolated from c-kit+, Sca-1, and IL-7Rα lin bone marrow cells. (Aiv) Further isolation of the HSC population based on IL-7Rα expression in c-kitHI, Sca-1HI cells. Approximately 90% of c-kitLO, Sca-1LO cells were IL-7Rα (HSC phenotype). (Av) Isolation of the CLP population based on IL-7Rα expression in c-kitLO, Sca-1LO cells. Approximately 89% of c-kitLO, Sca-1LO cells were IL-7Rα+ (CLP phenotype). (Avi) Isolation of the CMP population based on FcγRII/III and CD34 expression in c-kit+, Sca-1, and IL-7Rα cells. Cells that are FcγRII/IIILO and CD34+ represent the CMP phenotype. (B) Average number of HSCs (lin, c-kitHI, Sca-1HI, IL-7Rα; n = 3), CLPs (lin, c-kitLO, Sca-1LO, IL-7Rα+; n = 3), and CMPs (lin, c-kit+, Sca-1, IL-7Rα, FcγRII/IIILO, CD34+; n = 4) as determined by the percentage of lineage-negative (lin) bone marrow cells that stained positive for the HSC, CLP, or CMP phenotype. Staining was performed on lineage-depleted cells isolated from groups of 3 Hmgb3/Y or wild-type mice prior to analysis by flow cytometry. The data represent the pooled results of 3 (HSCs and CLPs) or 4 (CMPs) independent experiments. (C) Mean CFU–Pre-B frequency generated from wild-type and Hmgb3/Y CLP populations. CFU–Pre-B frequency within the CLP population was determined by scoring pre–B-cell colonies per 1000 cells cultured: wild-type (n = 8; 355 CFU–Pre-Bs counted); Hmgb3/Y (n = 8; 890 CFU–Pre-Bs counted). The data represent the pooled results of 2 independent experiments. (D) Mean myeloid colony (CFU-C) frequency generated from wild-type and Hmgb3/Y CMP populations. Myeloid CFU-C frequency within the CMP population was determined by scoring CFU-GM, BFU-E, and CFU-GEMM colonies per 500 cells cultured: wild-type (n = 10; 813 CFU-GMs, 177 BFU-Es, and 91 CFU-GEMMs counted); Hmgb3/Y (n = 10; 239 CFU-GMs, 47 BFU-Es, and 17 CFU-GEMMs counted). The data represent the pooled results of 2 independent experiments. P values in panels B-D were determined by Student t test. In panels B-D, error bars represent standard deviation.

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