Figure 3. Endophilin A2 is required for peripheral B‐cell development and GC responses.

1. CRISPR‐targeted bone marrow chimera workflow, showing flow cytometry detection of donor‐derived (GFP⁺), sgRNA‐containing (mCherry⁺) cells.
2. Development of B‐cell populations in chimeras' bone marrow and spleen from Cd4‐ or Sh3gl1‐targeted HSCs. Percentage of mCherry⁺ cells at each stage is normalized to initial infection rate of transferred lineage^‐ cells, and shown as mean + SEM. N = 11–12 mice. *P = 0.0286, ***P < 0.0001 using two‐way ANOVA.
3. MZ development in mCherry⁺ B‐cell compartment.
4. Representative stain of surface CD86 and CD69 on adoptively transferred HEL‐specific follicular B cells 24 h post‐SRBC‐HEL immunization.
5. Quantification of surface CD86 and CD69 mean fluorescence intensity (MFI). Data show mean and SEM from six mice across two experiments.
6. Fractions of mCherry⁺ cells in GC, PC, IgG1⁺ class‐switched and follicular B cells at 4‐, 8‐, and 14 days post‐SRBC‐HEL immunization. N = 8–10 mice; data shows mean and SEM. *P < 0.05; ***P < 0.001; ****P < 0.0001 using 2‐way ANOVA with multiple comparisons.