Figure 3.
Initiation of MHC II expression shapes B-cell development. (A) Flow cytometric identification of bone marrow Fr A-F B cells. (B-C) MHC II expression (B) and mean frequency (plus or minus SEM) of MHC II+ cells (C) in Fr A-F bone marrow B cells from mice of the indicated genotype (WT, n = 3; ItgaxcreH2-Ab1c, n = 5; Fcer2acreH2-Ab1c, n = 6). (D) MHC II expression (green), detected by immunofluorescence staining in WT Fr A-C bone marrow B cells (MHC II antibody clone M5/114.15.2 stain; scale bar, 5 μM). ItgaxcreH2-Ab1c Fr A bone marrow B cells are included as staining control. (E) Mean change (plus or minus SEM) from input frequency of CD45.2+ cells in Fr A-F bone marrow B cells from chimeras between CD45.1+ WT control and CD45.2+ test genotype donors (WT: WT, n = 9; WT: ItgaxcreH2-Ab1c, n = 6; WT: Fcer2acreH2-Ab1c, n = 5). *P < .001 between WT and other genotypes by Student t tests. (F-G) In vitro development of purified Fr A ItgaxcreH2-Ab1c B-cell precursors into pre-B (pre; B220+CD2+IgD−IgM−) and immature B cells (imm; B220+CD2+IgD−IgM+) (F), and mean change (plus or minus SEM) from input frequency of CD45.2+ cells in Fr A, pre-B cells, and immature B cells following in vitro development of purified Fr A cells in competitive cultures between CD45.1+ WT control and CD45.2+ test genotype input Fr A cells (G) (WT: WT, n = 6; WT: ItgaxcreH2-Ab1c, n = 2; WT: Fcer2acreH2-Ab1c, n = 8). *P < .02 between WT and other genotypes by Student t tests. FSC, forward scatter.

Initiation of MHC II expression shapes B-cell development. (A) Flow cytometric identification of bone marrow Fr A-F B cells. (B-C) MHC II expression (B) and mean frequency (plus or minus SEM) of MHC II+ cells (C) in Fr A-F bone marrow B cells from mice of the indicated genotype (WT, n = 3; ItgaxcreH2-Ab1c, n = 5; Fcer2acreH2-Ab1c, n = 6). (D) MHC II expression (green), detected by immunofluorescence staining in WT Fr A-C bone marrow B cells (MHC II antibody clone M5/114.15.2 stain; scale bar, 5 μM). ItgaxcreH2-Ab1c Fr A bone marrow B cells are included as staining control. (E) Mean change (plus or minus SEM) from input frequency of CD45.2+ cells in Fr A-F bone marrow B cells from chimeras between CD45.1+ WT control and CD45.2+ test genotype donors (WT: WT, n = 9; WT: ItgaxcreH2-Ab1c, n = 6; WT: Fcer2acreH2-Ab1c, n = 5). *P < .001 between WT and other genotypes by Student t tests. (F-G) In vitro development of purified Fr A ItgaxcreH2-Ab1c B-cell precursors into pre-B (pre; B220+CD2+IgDIgM) and immature B cells (imm; B220+CD2+IgDIgM+) (F), and mean change (plus or minus SEM) from input frequency of CD45.2+ cells in Fr A, pre-B cells, and immature B cells following in vitro development of purified Fr A cells in competitive cultures between CD45.1+ WT control and CD45.2+ test genotype input Fr A cells (G) (WT: WT, n = 6; WT: ItgaxcreH2-Ab1c, n = 2; WT: Fcer2acreH2-Ab1c, n = 8). *P < .02 between WT and other genotypes by Student t tests. FSC, forward scatter.

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