Figure 3.
Figure 3. Ebf1 and the Batf/IRF4 complex cooperatively promote the expression of Aicda and Ezh2. (A-B) Ebf1 transduction in B1-8hi splenic B cells. Cells were transduced with control retroviral vector or retroviral vector expressing Ebf1 on day 1 after differentiation stimuli and sorted on the basis of green fluorescent protein (GFP) expression on day 3. One experiment was performed using 3 mice. (A) RT-PCR analysis of Ebf1 and Ezh2 transcripts. (B) Flow cytometry analysis of intracellular IRF4, CD138, and IgG1. Numbers adjacent to outlined areas indicate percent IRF4loCD138nega cells (top lower), IRF4hiCD138nega cells (top upper left), IRF4hiCD138posi cells (top upper right), IRF4loIgG1posi cells (bottom lower), or IRF4hiIgG1posi cells (bottom upper). (C-D) Knockdown of Batf and/or Ebf1 in B1-8hi splenic B cells. Cells were transduced with a control vector or vector targeting Batf (shBatf) and vector targeting Ebf1 (shEbf1) on day 1 after differentiation stimuli. On day 3, cells were sorted on the basis of GFP expression for control, and GFP (shBatf) and/or dsRed (shEbf1) expression for shBatf and/or shEbf1. One experiment was performed using 3 mice. (C) RT-PCR analysis of transcripts of indicated genes. (D) Flow cytometry analysis of surface CD138 and IgG1. For panels A and C, results are presented relative to the abundance of transcripts encoding Β2m, and shown with box-and-whisker plot. *P < .05; **P < .01; ***P < .001. For panels B and D, data are representative of 3 mice, and shown with the means and standard deviation (SD), respectively.

Ebf1 and the Batf/IRF4 complex cooperatively promote the expression of Aicda and Ezh2. (A-B) Ebf1 transduction in B1-8hi splenic B cells. Cells were transduced with control retroviral vector or retroviral vector expressing Ebf1 on day 1 after differentiation stimuli and sorted on the basis of green fluorescent protein (GFP) expression on day 3. One experiment was performed using 3 mice. (A) RT-PCR analysis of Ebf1 and Ezh2 transcripts. (B) Flow cytometry analysis of intracellular IRF4, CD138, and IgG1. Numbers adjacent to outlined areas indicate percent IRF4loCD138nega cells (top lower), IRF4hiCD138nega cells (top upper left), IRF4hiCD138posi cells (top upper right), IRF4loIgG1posi cells (bottom lower), or IRF4hiIgG1posi cells (bottom upper). (C-D) Knockdown of Batf and/or Ebf1 in B1-8hi splenic B cells. Cells were transduced with a control vector or vector targeting Batf (shBatf) and vector targeting Ebf1 (shEbf1) on day 1 after differentiation stimuli. On day 3, cells were sorted on the basis of GFP expression for control, and GFP (shBatf) and/or dsRed (shEbf1) expression for shBatf and/or shEbf1. One experiment was performed using 3 mice. (C) RT-PCR analysis of transcripts of indicated genes. (D) Flow cytometry analysis of surface CD138 and IgG1. For panels A and C, results are presented relative to the abundance of transcripts encoding Β2m, and shown with box-and-whisker plot. *P < .05; **P < .01; ***P < .001. For panels B and D, data are representative of 3 mice, and shown with the means and standard deviation (SD), respectively.

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