![Figure 2. Normal binding and endocytosis of IgG-immune complexes (IgG-ICs) by GPI-anchor-deficient DCs. (A) Staining of AMs (left panels) or DCs (right panels) with anti-FcγRII/III mAb 2.4G2 (top panels) or monomeric mouse IgG2a as a marker for FcγRI (bottom panels). (B) Staining of DCs with IgG-ICs; mean fluorescence intensity for WT cells was 111 and for KO cells was 165. (A-B) Shown are fluorescence intensity plots of cells from littermate control (thin lines) or LysMCre/Pig-aflox mice (bold lines), and antibody controls (dotted lines). (C) Blocking of IgG-IC binding by 2.4G2. Control DCs were preincubated with medium (left), 2.4G2 (25 μg/mL; middle), or isotype-matched control mAb anti-CD11b (M1/70; 25 μg/mL; right) for 30 minutes on ice, and next stained with IgG-ICs (solid line) or medium (dotted line). (D) Endocytosis of IgG-ICs. Control (WT, top panels) or GPI-anchor-deficient (KO, bottom panels) DCs were incubated on ice with FITC-containing IgGICs, washed, and kept on ice (4°C; left panels) or incubated at 37°C for 20 minutes (middle panels) or 30 minutes (right panels). Percentages of cells having endocytosed IgG-ICs (ie, gated cells exhibiting decreased extracellular IgG-IC staining [FL2] and unchanged FL1 signal) are shown in the upper right quadrants.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/104/9/10.1182_blood-2004-02-0671/6/zh80210468490002.jpeg?Expires=1724126076&Signature=oTgXYyRGCeSG9YHlkFM8aM3ajjmt0Ms5mItbteLLGVNYtKgP6xHGUCTp4inmoJ-hqQRY2IuGDQazINl5e70~D54WQoRRtpDiBMMFTR51FP2ysz8F9RIwQLa01vQmJLUWC8JAiMFTpR8chLts1iZz6mqs6QoW4coLLZjZHPpVt0m-Op4gicZJVs-0GPTIzFvpP9pj~u~jXjTFBjCFqrBL4zwd6xMdYXnr0Tp7mfFSl~HoU00xeH~WnhkkDBXD0Nu9CSwAXhRB96tefAPV7~fymy344wi5Tirylpz6TS7gpaDMkQE4iq6c93TRs2MDzBOW6~xxfL5eqFDOqfZe~S71cQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Normal binding and endocytosis of IgG-immune complexes (IgG-ICs) by GPI-anchor-deficient DCs. (A) Staining of AMs (left panels) or DCs (right panels) with anti-FcγRII/III mAb 2.4G2 (top panels) or monomeric mouse IgG2a as a marker for FcγRI (bottom panels). (B) Staining of DCs with IgG-ICs; mean fluorescence intensity for WT cells was 111 and for KO cells was 165. (A-B) Shown are fluorescence intensity plots of cells from littermate control (thin lines) or LysMCre/Pig-aflox mice (bold lines), and antibody controls (dotted lines). (C) Blocking of IgG-IC binding by 2.4G2. Control DCs were preincubated with medium (left), 2.4G2 (25 μg/mL; middle), or isotype-matched control mAb anti-CD11b (M1/70; 25 μg/mL; right) for 30 minutes on ice, and next stained with IgG-ICs (solid line) or medium (dotted line). (D) Endocytosis of IgG-ICs. Control (WT, top panels) or GPI-anchor-deficient (KO, bottom panels) DCs were incubated on ice with FITC-containing IgGICs, washed, and kept on ice (4°C; left panels) or incubated at 37°C for 20 minutes (middle panels) or 30 minutes (right panels). Percentages of cells having endocytosed IgG-ICs (ie, gated cells exhibiting decreased extracellular IgG-IC staining [FL2] and unchanged FL1 signal) are shown in the upper right quadrants.
