Figure 3.
Figure 3. Reconstitution of B-lineage development in MBS-treated BtkTec–/– mice. BM, splenocytes, peripheral blood, and peritoneal cells were harvested from BtkTec–/– recipient mice 3 to 5 months after transplantation, evaluated by flow cytometry, and characterized based on “Hardy Fraction” stages of B-cell development. (A) BM (harvested 21 weeks after transplantation) was stained for B220, CD43, and IgM. Levels of Fractions A to C (pro-B) and Fraction D (pre-B), presented as percentages of the B220+ B-cell compartment, are shown in the upper panel (CD43/B220, gated on IgM– cells). Fractions E to F (immature B, mature B) are shown in the lower panel (IgM+/B220, gated on live cells as determined by forward and side scatter profiles), and also as percentages of B220+ cells. (B) Splenocytes (harvested 15 weeks after transplantation) were stained for B220, IgM, and IgD. B220+ cells, shown as percentages of total splenocytes, are shown in the upper panel (IgM/B220, gated on live cells). Late-stage splenic B-cell profiles are shown in the lower panel (IgM/IgD, gated on B220+ cells); the sequence of maturation is from Fraction FIII (IgMhi/IgDlo) to FII (IgMhi/IgDhi) to FI (IgMlo/IgDhi) as percentages of B220+ B cells. (C) Peripheral blood (collected 21 weeks after transplantation) was analyzed by the same parameters as for splenocytes. (D) Representative plots of peritoneal cells collected from BtkTec–/– transplant recipients 21 weeks after transplantation and stained for IgM, Mac1, and CD5 are shown. Total B1 cells are shown in the upper panel (IgM/Mac1, gated on live cells); percentages are relative to total peritoneal cells. Further resolution into CD5+ B1a and CD5– B1b, also presented as a percentage of the total peritoneal population, is shown in the lower panel (CD5/Mac1, gated on IgM– cells). Representative data from 2 of 3 independent experiments are shown.

Reconstitution of B-lineage development in MBS-treated BtkTec–/– mice. BM, splenocytes, peripheral blood, and peritoneal cells were harvested from BtkTec–/– recipient mice 3 to 5 months after transplantation, evaluated by flow cytometry, and characterized based on “Hardy Fraction” stages of B-cell development. (A) BM (harvested 21 weeks after transplantation) was stained for B220, CD43, and IgM. Levels of Fractions A to C (pro-B) and Fraction D (pre-B), presented as percentages of the B220+ B-cell compartment, are shown in the upper panel (CD43/B220, gated on IgM cells). Fractions E to F (immature B, mature B) are shown in the lower panel (IgM+/B220, gated on live cells as determined by forward and side scatter profiles), and also as percentages of B220+ cells. (B) Splenocytes (harvested 15 weeks after transplantation) were stained for B220, IgM, and IgD. B220+ cells, shown as percentages of total splenocytes, are shown in the upper panel (IgM/B220, gated on live cells). Late-stage splenic B-cell profiles are shown in the lower panel (IgM/IgD, gated on B220+ cells); the sequence of maturation is from Fraction FIII (IgMhi/IgDlo) to FII (IgMhi/IgDhi) to FI (IgMlo/IgDhi) as percentages of B220+ B cells. (C) Peripheral blood (collected 21 weeks after transplantation) was analyzed by the same parameters as for splenocytes. (D) Representative plots of peritoneal cells collected from BtkTec–/– transplant recipients 21 weeks after transplantation and stained for IgM, Mac1, and CD5 are shown. Total B1 cells are shown in the upper panel (IgM/Mac1, gated on live cells); percentages are relative to total peritoneal cells. Further resolution into CD5+ B1a and CD5 B1b, also presented as a percentage of the total peritoneal population, is shown in the lower panel (CD5/Mac1, gated on IgM cells). Representative data from 2 of 3 independent experiments are shown.

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