Anti igg1 pe

Mononuclear BM cells, B cells after culture or splenocytes were treated 10 minutes with FC block solution (BD Bioscience) then labelled 20 minutes on ice with combination of different anti-mouse antibodies (Abs) as indicated in legends of figures. Abs included anti-B220-eFluor660 (Ebioscience, Clone RA3-6B2), anti-IgM-Fitc (Ebioscience, Clone eB121-15F9), anti-IgG1-PE (Ebioscience, Clone m1-14D12), biotin anti-IgG2a^b (BD Bioscience, Clone 5.7), biotin anti-mouse IgG3 (BD Bioscience, Clone R40-82), anti-CD138-BrillantViolet421 (BD Bioscience, Clone 281-2), anti-CD43-PE (BD biosciences, Clone S7), anti-CD45.1-PeCy7 (BD biosciences, Clone A20) and anti-CD45.2-APC-Cy7 (BD biosciences, Clone 104). Biotinylated primary antibodies were detected by incubation of labeled cells with streptavidin-PE (BD Bioscience). For apoptosis analysis, B cells were first surface labeled for ASC detection, then washed and re-suspended in 1x Binding buffer (Ebioscience) and labeled with anti-AnnexinV-Fitc (Ebioscience). Ten minutes before flow cytometry acquisition, propidium iodide (Ebioscience) was added to all samples for detection and/or exclusion of dead cells. Cells were analyzed with a FACSFortessa or a FACSCanto (BD Bioscience) and Diva (BD Bioscience) or FLowJo (TreeStar) softwares.