Figure 6
Figure 6. CD4highCD25+ alloantigen-specific Treg can be continuously expanded by CD40-activated B cells in large-scale without loss of function, and exogenous IL-2 does not enhance this cell expansion. Freshly purified naive CD4+CD25− T cells were cocultured with CD40-activated allogeneic B cells for the indicated time. (A) The percentages of CD4highCD25+ and CD4mediumCD25− cells in the cultures (n = 10). (B) Expansion of CD4highCD25+ alloantigen-specific Treg from 10 different persons. The expansion was normalized for the CD4highCD25+ cells, and the fold increase of the CD4highCD25+ was shown. (C) Naive CD4+CD25− were cocultured with CD40-activated allogeneic B cells with or without IL-2. The expansion was normalized for the CD4highCD25+ cells, and the fold increase of the CD4highCD25+ is shown (n = 4). (D) Absolute numbers of CD4highCD25+ alloantigen-specific Treg generated from 106 naive CD4+CD25− T cells (n = 10). (E) CD4highCD25+ alloantigen-specific Treg induced and expanded by CD40-activated B cells for 21 days remain functional. Freshly purified naive CD4+CD25− T cells (responder) were cocultured with CD40-activated allogeneic B cells (target antigen) to induce and expand CD4highCD25+ Treg for 21 days with replacement of B cells every 7 days. The sorted CD4highCD25+ and CD4mediumCD25− cells were added into the MLR culture system as described in “Mixed lymphocyte reaction assays.” Data shown here are representative of 3 independent experiments.

CD4highCD25+ alloantigen-specific Treg can be continuously expanded by CD40-activated B cells in large-scale without loss of function, and exogenous IL-2 does not enhance this cell expansion. Freshly purified naive CD4+CD25 T cells were cocultured with CD40-activated allogeneic B cells for the indicated time. (A) The percentages of CD4highCD25+ and CD4mediumCD25 cells in the cultures (n = 10). (B) Expansion of CD4highCD25+ alloantigen-specific Treg from 10 different persons. The expansion was normalized for the CD4highCD25+ cells, and the fold increase of the CD4highCD25+ was shown. (C) Naive CD4+CD25 were cocultured with CD40-activated allogeneic B cells with or without IL-2. The expansion was normalized for the CD4highCD25+ cells, and the fold increase of the CD4highCD25+ is shown (n = 4). (D) Absolute numbers of CD4highCD25+ alloantigen-specific Treg generated from 106 naive CD4+CD25 T cells (n = 10). (E) CD4highCD25+ alloantigen-specific Treg induced and expanded by CD40-activated B cells for 21 days remain functional. Freshly purified naive CD4+CD25 T cells (responder) were cocultured with CD40-activated allogeneic B cells (target antigen) to induce and expand CD4highCD25+ Treg for 21 days with replacement of B cells every 7 days. The sorted CD4highCD25+ and CD4mediumCD25 cells were added into the MLR culture system as described in “Mixed lymphocyte reaction assays.” Data shown here are representative of 3 independent experiments.

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