Figure 3
Figure 3. Defective development of iNKT cells in Elf-1−/− mice is cell intrinsic. (A-B) BM cells from WT and Elf-1−/− mice were transferred into irradiated WT or Elf-1−/− recipients. After 6 weeks, cells were harvested from recipient mice, stained with CD1d/αGalCer tetramer and anti–TCRβ, and analyzed by flow cytometry. (A) Numbers indicate the percentage of tetramer+TCRβ+ in the spleen of indicated recipients. Data shown are representative of 3 independent experiments using a minimum of 2 recipients per donor genotype. (B) Bar graphs depict the means ± SD for the proportion of iNKT cells in the spleen of indicated recipients (n = 9 for each group; *P < .05; **P < .01). (C) BM cells from Elf-1−/− or CD45.1+ WT congenic mice or mixed BM (1:1) from Elf-1−/− and WT congenic mice were transferred into irradiated Jα18−/− recipients. After 6 weeks, cells were harvested from recipient mice, stained with CD1d/αGalCer tetramer and anti–CD45.1, and analyzed by flow cytometry. Numbers in each quadrant indicate the percentage of tetramer+CD45.1+ cells in the spleen of indicated recipients. Data are representative of 3 independent experiments using a minimum of 2 recipients per donor genotype.

Defective development of iNKT cells in Elf-1−/−mice is cell intrinsic. (A-B) BM cells from WT and Elf-1−/− mice were transferred into irradiated WT or Elf-1−/− recipients. After 6 weeks, cells were harvested from recipient mice, stained with CD1d/αGalCer tetramer and anti–TCRβ, and analyzed by flow cytometry. (A) Numbers indicate the percentage of tetramer+TCRβ+ in the spleen of indicated recipients. Data shown are representative of 3 independent experiments using a minimum of 2 recipients per donor genotype. (B) Bar graphs depict the means ± SD for the proportion of iNKT cells in the spleen of indicated recipients (n = 9 for each group; *P < .05; **P < .01). (C) BM cells from Elf-1−/− or CD45.1+ WT congenic mice or mixed BM (1:1) from Elf-1−/− and WT congenic mice were transferred into irradiated Jα18−/− recipients. After 6 weeks, cells were harvested from recipient mice, stained with CD1d/αGalCer tetramer and anti–CD45.1, and analyzed by flow cytometry. Numbers in each quadrant indicate the percentage of tetramer+CD45.1+ cells in the spleen of indicated recipients. Data are representative of 3 independent experiments using a minimum of 2 recipients per donor genotype.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal