![Anti-BR3 mAb reduces mouse B-cell subsets more efficiently than BR3-Fc. BALB/c mice were treated with anti-BR3 (500 μg), BR3-Fc (150 μg × 3/week) or isotype control (500 μg); 15 days later, tissues were analyzed by flow cytometry (A,C) and immunofluorescence (B). Percentages of cells in B-cell subsets are displayed near each gate as follows: Spleen: follicular (FO) B cells (CD23+CD21+), marginal zone (MZ) B cells (CD23−CD21hi), and plasma cells (PC, CD138+B220lo); Lymph nodes: B cells (CD23+CD21+), blood (BL) B cells (CD23+CD21+), Peyer patches (PP), follicular B cells (B220+CD38+), and germinal center (GC) B cells (B220+CD38lo); peritoneal cavity (PEC): B2 cells (B220+CD23+) and B1 cells (B220+CD23−) (A,C). B cells (blue) and T cells (green) are stained in spleen sections after treatment with control, BR3-Fc or anti-BR3 mAb. Marginal zone and follicular B-cell areas are separated by the layer of metallophilic macrophages (MM [red]) (B). See “Immunofluorescence and immunohistochemistry staining” for image acquisition details. Absolute B-cell numbers or percentage of lymphocyte gate belonging to a defined subset are shown as mean plus or minus standard error. Statistical significance compared with the control treated group is indicated with asterisk (C). When 2 treatment groups are significantly different from each other, the P value is displayed. These data are representative of more than 10 independent experiments done with several maximally depleting doses of anti-BR3, using at least 5 mice/group.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/110/12/10.1182_blood-2007-04-088088/4/zh80230709560001.jpeg?Expires=1722193149&Signature=4In6TRFG3Znc82jTPDKc77YnqvMaMLXa4u1hE53ZfSWJgLcExQsxriLVkyEX2Q5ULhfXx9c3WAS56HwMwb4DC8gCavU~jWL3SNp89yR3F1GDon~I0g39vQ65yhQ4qlcWF2LCENmqhM7MBi6WFmTm8g11i8nckbtFRvV~yf8TCJ7SCRxBuHddsSaX92k3gFvf~7fD8y2X-o3-azqJUfmfGEdW6G-43rt-PsxnU4fwagCf7ItNEgLNkWL3aUHDz89ApA9xjtPayBbUbi9d-aVJ4Yd16clhL8OpVhmfmaJQ0O-aXeflefOQUUcVqfTUsZQC0geLu5yBS9v2YBJd2US5lQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Anti-BR3 mAb reduces mouse B-cell subsets more efficiently than BR3-Fc. BALB/c mice were treated with anti-BR3 (500 μg), BR3-Fc (150 μg × 3/week) or isotype control (500 μg); 15 days later, tissues were analyzed by flow cytometry (A,C) and immunofluorescence (B). Percentages of cells in B-cell subsets are displayed near each gate as follows: Spleen: follicular (FO) B cells (CD23+CD21+), marginal zone (MZ) B cells (CD23−CD21hi), and plasma cells (PC, CD138+B220lo); Lymph nodes: B cells (CD23+CD21+), blood (BL) B cells (CD23+CD21+), Peyer patches (PP), follicular B cells (B220+CD38+), and germinal center (GC) B cells (B220+CD38lo); peritoneal cavity (PEC): B2 cells (B220+CD23+) and B1 cells (B220+CD23−) (A,C). B cells (blue) and T cells (green) are stained in spleen sections after treatment with control, BR3-Fc or anti-BR3 mAb. Marginal zone and follicular B-cell areas are separated by the layer of metallophilic macrophages (MM [red]) (B). See “Immunofluorescence and immunohistochemistry staining” for image acquisition details. Absolute B-cell numbers or percentage of lymphocyte gate belonging to a defined subset are shown as mean plus or minus standard error. Statistical significance compared with the control treated group is indicated with asterisk (C). When 2 treatment groups are significantly different from each other, the P value is displayed. These data are representative of more than 10 independent experiments done with several maximally depleting doses of anti-BR3, using at least 5 mice/group.
