Figure 3.
Figure 3. In vivo homing analysis of CXCR4+/+ and CXCR4–/– FL cells. Freshly isolated FL cells were stained with the CFSE dye as described in “In vivo homing assay.” A range of 20 × 106 to 30 × 106 CFSE+ cells for each genotype were injected in lethally syngenic irradiated and nonirradiated mice. Recipients were killed 3 and 24 hours after transplantation and BM, spleen, and blood were harvested and analyzed for the percentage of homed CFSE+ cells by flow cytometry. (A) Representative flow cytometry analysis of BM, spleen, and blood from control uninjected mice, CXCR4+/+ CFSE+–injected mice, and CXCR4–/– CFSE+–injected mice after 3 hours' homing in either irradiated or nonirradiated recipients. CFSE+ cell populations are shown in a gate and their relative numbers are indicated. (B) Histograms showing the percentage of recovered CFSE+ cells per organ (% Homing) in the BM, spleen, and blood 3 and 24 hours after transplantation. The results are calculated based on the formula described in “In vivo homing assay.” The formula is based on the percentage of homed CFSE+ donor cells multiplied by the cellularities of each organ recovered from mice after being lethally irradiated 24 hours before injected by CFSE+ donor cells and divided by the number of CFSE+ donor cells injected per mouse. Data representing mean ± SD of BM, spleen, and blood (n = 24 for each) cellularities (B as mentioned in the formula) were as follows: at 3 hours after injections Bmarrow = 171.8 × 106 ± 20.8 × 106 cells, Bspleen = 4.12 × 106 ± 1.4 × 106 cells, and Bblood = 15.86 × 106 ± 2.15 × 106 cells; and at 24 hours after injections Bmarrow = 30 × 106 ± 10.7 × 106 cells, Bspleen = 1.86 × 106 ± 0.5 × 106 cells, and Bblood = 1.2 × 106 ± 0.3 × 106 cells. Each histogram bar represents the mean ± SD of the percentage of homing obtained in 4 independent experiments (3 mice/genotype/time). *P < .01.

In vivo homing analysis of CXCR4+/+ and CXCR4–/– FL cells. Freshly isolated FL cells were stained with the CFSE dye as described in “In vivo homing assay.” A range of 20 × 106 to 30 × 106 CFSE+ cells for each genotype were injected in lethally syngenic irradiated and nonirradiated mice. Recipients were killed 3 and 24 hours after transplantation and BM, spleen, and blood were harvested and analyzed for the percentage of homed CFSE+ cells by flow cytometry. (A) Representative flow cytometry analysis of BM, spleen, and blood from control uninjected mice, CXCR4+/+ CFSE+–injected mice, and CXCR4–/– CFSE+–injected mice after 3 hours' homing in either irradiated or nonirradiated recipients. CFSE+ cell populations are shown in a gate and their relative numbers are indicated. (B) Histograms showing the percentage of recovered CFSE+ cells per organ (% Homing) in the BM, spleen, and blood 3 and 24 hours after transplantation. The results are calculated based on the formula described in “In vivo homing assay.” The formula is based on the percentage of homed CFSE+ donor cells multiplied by the cellularities of each organ recovered from mice after being lethally irradiated 24 hours before injected by CFSE+ donor cells and divided by the number of CFSE+ donor cells injected per mouse. Data representing mean ± SD of BM, spleen, and blood (n = 24 for each) cellularities (B as mentioned in the formula) were as follows: at 3 hours after injections Bmarrow = 171.8 × 106 ± 20.8 × 106 cells, Bspleen = 4.12 × 106 ± 1.4 × 106 cells, and Bblood = 15.86 × 106 ± 2.15 × 106 cells; and at 24 hours after injections Bmarrow = 30 × 106 ± 10.7 × 106 cells, Bspleen = 1.86 × 106 ± 0.5 × 106 cells, and Bblood = 1.2 × 106 ± 0.3 × 106 cells. Each histogram bar represents the mean ± SD of the percentage of homing obtained in 4 independent experiments (3 mice/genotype/time). *P < .01.

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