Figure 5.
Knockdown of Ikaros but not Aiolos resulted in defect of plasma cell differentiation. (A-B) Knockdown of Ikaros or Aiolos in B1-8hi splenic B cells. Cells were transduced with a control vector or vector targeting Ikaros (shIkzf1) or Aiolos (shIkzf3) on day 1 after differentiation stimuli, then sorted on the basis of GFP expression on day 3. One experiment using 3 mice. (A) RT-PCR analysis of Ikzf1 and Ikzf3 transcripts. Results are presented relative to the abundance of transcripts encoding Β2m, and shown with box-and-whisker plot. (B) Flow cytometry analysis of intracellular IRF4 and CD138 and IgG1. Numbers adjacent to outlined areas indicate percent IRF4loCD138nega cells (top lower), IRF4hiCD138nega cells (top upper left), IRF4hiCD138posi cells (top upper right), or IgG1posi cells (bottom). Data are representative of 3 mice, and shown with the mean and SD, respectively. (C) The binding of IRF4 or Ikaros to their regulatory regions at the Ebf1, Haao, and Setd2 loci. B1-8hi splenic B cells were stimulated for 48 hours, and ChIP assay was performed using control IgG, α-IRF4, or α-Ikaros, followed by quantitative PCR analysis. Binding enrichments is presented relative to input DNA. The average enrichment and SD is from 3 independent experiments for α-IRF4, and 2 independent experiments with technical duplicate for α-Ikaros. For panels A and C, *P < .05; **P < .01; ***P < .001.