Figure 3
Figure 3. Osteoblasts support the differentiation of RAG2− LSK cells to RAG2+ cells, and to B-lymphoid precursors. (A) BM LSK cells from RAG2 GFP NG BAC mice were analyzed for GFP expression by FACS, and sorted into GFP− and GFP+ populations. GFP− LSKs were cultured for 14 days on either primary osteoblasts, MS-1 endothelial cells, or S17 stromal cells, after which the hematopoietic cells were recovered, stained with nonfluorescein dyes for B220 and CD19, and analyzed for Rag2−GFP, CD19, and B220 expression by flow cytometry. (A) Rag-2−GFP− BM cells generate EGFP-bright cells after 14-day coculture with osteoblasts, and S-17 cells, but not MS-1 endothelial cells. Each coculture was initiated with 3000 LSK Rag2− cells. After 14 days, 1.09 × 105 total hematopoietic cells were recovered from the OB coculture, of which 1.64 × 104 were EGFP bright, whereas none of the 1.2 × 105 cells recovered from the MS-1 coculture was EGFP bright. S17 cocultures generated 7.6 × 104 total cells, of which 1.67 × 104 were EGFP bright. Percent of output cells with green fluorescence higher than control (nontransgenic and transgenic, sorted, Rag-2 GFP−) cells is shown in the figure. (B) GFP+B220+CD19+ B lymphocytes are generated from both GFP− LSK cells and GFP+ LSK cells isolated from RAG2 GFP NG BAC mice, following 14-day cultures on osteoblast monolayers. (C) Absolute numbers of B-lymphocyte precursors produced from cocultures initiated with 105 LSK cells.

Osteoblasts support the differentiation of RAG2 LSK cells to RAG2+ cells, and to B-lymphoid precursors. (A) BM LSK cells from RAG2 GFP NG BAC mice were analyzed for GFP expression by FACS, and sorted into GFP and GFP+ populations. GFP LSKs were cultured for 14 days on either primary osteoblasts, MS-1 endothelial cells, or S17 stromal cells, after which the hematopoietic cells were recovered, stained with nonfluorescein dyes for B220 and CD19, and analyzed for Rag2GFP, CD19, and B220 expression by flow cytometry. (A) Rag-2GFP BM cells generate EGFP-bright cells after 14-day coculture with osteoblasts, and S-17 cells, but not MS-1 endothelial cells. Each coculture was initiated with 3000 LSK Rag2 cells. After 14 days, 1.09 × 105 total hematopoietic cells were recovered from the OB coculture, of which 1.64 × 104 were EGFP bright, whereas none of the 1.2 × 105 cells recovered from the MS-1 coculture was EGFP bright. S17 cocultures generated 7.6 × 104 total cells, of which 1.67 × 104 were EGFP bright. Percent of output cells with green fluorescence higher than control (nontransgenic and transgenic, sorted, Rag-2 GFP) cells is shown in the figure. (B) GFP+B220+CD19+ B lymphocytes are generated from both GFP LSK cells and GFP+ LSK cells isolated from RAG2 GFP NG BAC mice, following 14-day cultures on osteoblast monolayers. (C) Absolute numbers of B-lymphocyte precursors produced from cocultures initiated with 105 LSK cells.

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