Figure 4
Figure 4. Wnt3a induces expression of matrix molecules, and one of them mediates most Wnt3a-regulated changes in murine hematopoiesis. (A) RT-PCR was performed using Wnt3a-transduced OP9 stromal cells. The results are expressed as the fold changes relative to the vector control OP9 cells and are representative of those obtained in 3 independent experiments. (B) Murine Lin−Sca-1+c-KithiFlk-2− HSCs were then cocultured with decorin plus OP9 or on OP9-Wnt3a in the presence of IL-7, SCF, and FL for 3 days. Levels of c-Kit are shown as typical histograms or mean fluorescence intensities (MFI). (C) Lin−Sca-1+c-KithiRag1-GFP+ ELPs were held for 3 days in primary cultures before subculture in stromal cell–free, erythropoiesis-supporting conditions. After an additional 2 weeks of culture, the generation of Ter119+ erythroid cells was analyzed using flow cytometry. (D) Numbers of Ter119+ erythroid cells were determined by flow cytometry after Lin−Sca-1+c-Kithi cells were held for 2 weeks of culture under stromal cell–free, erythroid-supporting conditions. (E) Proliferation of Lin−Sca-1+c-KithiFlk-2− HSCs was unaffected by decorin, as reflected in Ki-67 staining. (F-G) The influence of recombinant decorin on B lymphopoiesis was tested with 1-week stromal cell cocultures (F) or stromal cell–free cultures (G) initiated with ELPs. Generation of B220+ lymphocytes in triplicate wells ± SD is shown. (H) The same transmembrane culture system shown in Figure 2D was used to analyze gene-expression patterns in OP9 cells exposed to diffusible Wnt3a produced by transduced cells in the lower wells. Similar results were obtained in 3 independent experiments. Statistical significance was determined by unpaired 2-tailed t test analysis: *P < .05; **P < .01.

Wnt3a induces expression of matrix molecules, and one of them mediates most Wnt3a-regulated changes in murine hematopoiesis. (A) RT-PCR was performed using Wnt3a-transduced OP9 stromal cells. The results are expressed as the fold changes relative to the vector control OP9 cells and are representative of those obtained in 3 independent experiments. (B) Murine LinSca-1+c-KithiFlk-2 HSCs were then cocultured with decorin plus OP9 or on OP9-Wnt3a in the presence of IL-7, SCF, and FL for 3 days. Levels of c-Kit are shown as typical histograms or mean fluorescence intensities (MFI). (C) LinSca-1+c-KithiRag1-GFP+ ELPs were held for 3 days in primary cultures before subculture in stromal cell–free, erythropoiesis-supporting conditions. After an additional 2 weeks of culture, the generation of Ter119+ erythroid cells was analyzed using flow cytometry. (D) Numbers of Ter119+ erythroid cells were determined by flow cytometry after LinSca-1+c-Kithi cells were held for 2 weeks of culture under stromal cell–free, erythroid-supporting conditions. (E) Proliferation of LinSca-1+c-KithiFlk-2 HSCs was unaffected by decorin, as reflected in Ki-67 staining. (F-G) The influence of recombinant decorin on B lymphopoiesis was tested with 1-week stromal cell cocultures (F) or stromal cell–free cultures (G) initiated with ELPs. Generation of B220+ lymphocytes in triplicate wells ± SD is shown. (H) The same transmembrane culture system shown in Figure 2D was used to analyze gene-expression patterns in OP9 cells exposed to diffusible Wnt3a produced by transduced cells in the lower wells. Similar results were obtained in 3 independent experiments. Statistical significance was determined by unpaired 2-tailed t test analysis: *P < .05; **P < .01.

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