Figure 3
Figure 3. IVIg binds to CD22 on the surface of B cells. (A) Tonsillar B cells were incubated with IVIg (left panel), or with aggregate IgG (middle panel). The binding of IgG was revealed using FITC-conjugated goat Fab′2 anti–human IgG. The right panel shows binding of the secondary Ab alone with the TRITC-conjugated donkey anti–rabbit IgAb, used as negative control. (B) Tonsillar B cells were stained with rabbit anti-CD22 followed by TRITC conjugated anti–rabbit Ab. After several washes, the cells were incubated with IVIg and and followed by FITC-conjugated anti–human IgG F(ab′)2. (C) Sialylated IVIg (IVIg SA+) and asialylated (IVIg SA−) fractions were used to stain B cells followed by FITC-conjugated F(ab′)2 anti–human IgG antibody. B cells were also stained with anti-CD22. (D) IVIg was separated according to their SA content using SNA affinity chromatography. Purity of the fractions was assessed by lectin blotting. Staining for CD22 was followed by secondary HRP-conjugated Ab, and the blots developed using the ECL system. (E) Tonsillar B cells were incubated with IVIg before warming the cells up at 37°C (middle lane) or examined without warming (left lane). Control for warming up at 37°C without IVIg is also shown (right lane) is shown. After the incubation, cell lysates were prepared and immunoprecipates with protein G Sepharose beads and analyzed by WB using anti–human CD22 Ab followed by secondary HRP conjugated Ab. The blots were developed using the ECL system.

IVIg binds to CD22 on the surface of B cells. (A) Tonsillar B cells were incubated with IVIg (left panel), or with aggregate IgG (middle panel). The binding of IgG was revealed using FITC-conjugated goat Fab′2 anti–human IgG. The right panel shows binding of the secondary Ab alone with the TRITC-conjugated donkey anti–rabbit IgAb, used as negative control. (B) Tonsillar B cells were stained with rabbit anti-CD22 followed by TRITC conjugated anti–rabbit Ab. After several washes, the cells were incubated with IVIg and and followed by FITC-conjugated anti–human IgG F(ab′)2. (C) Sialylated IVIg (IVIg SA+) and asialylated (IVIg SA−) fractions were used to stain B cells followed by FITC-conjugated F(ab′)2 anti–human IgG antibody. B cells were also stained with anti-CD22. (D) IVIg was separated according to their SA content using SNA affinity chromatography. Purity of the fractions was assessed by lectin blotting. Staining for CD22 was followed by secondary HRP-conjugated Ab, and the blots developed using the ECL system. (E) Tonsillar B cells were incubated with IVIg before warming the cells up at 37°C (middle lane) or examined without warming (left lane). Control for warming up at 37°C without IVIg is also shown (right lane) is shown. After the incubation, cell lysates were prepared and immunoprecipates with protein G Sepharose beads and analyzed by WB using anti–human CD22 Ab followed by secondary HRP conjugated Ab. The blots were developed using the ECL system.

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