Cytometric identification of tonsillar GC B cells and quantification of surface CD45RB expression. (A) Human tonsillar B cells were cytometrically identified using procedures previously described.7 Gates Q1 (CD38+IgD−), Q2 (CD38+IgD+), Q3(CD38−IgD+), and Q4(CD38−IgD−) were determined for total tonsillar B cells based on distinct staining patterns using antibodies against CD38 and IgD. (B) GC B cells were identified from Q1 as CD38+IgD− and excluded CD38++ cells. An anti-CD27 antibody was used to further identify the Pblast pool from Q1 as IgD−CD38++CD27+. Antibodies against IgM and/or CD27 were used to identify the pre-GC (from Q2 as IgM+IgD+CD38+CD27−), naive (from Q3 as IgM+IgD+CD38−CD27−), and memory (from Q4 as IgD−CD38−CD27+) B-cell pools. (C) Tonsillar B cells were additionally stained with anti-CD45RB. The percentage of RB+ cells within each B-cell subset is indicated. Values represent the average of 6 tonsils. Standard deviations are included as error bars. Intersubset differences in the percentage of RB+ cells were statistically significant (P ≤ .01, denoted by a double asterisk [**]) between GC and all other subsets.