(A) Diagram of the TLR9 overexpression plasmid and insertion into the rosa26 locus. The plasmid contains 2 rosa26 homology arms flanking the expression vector. The vector is composed of a floxed region (demarcated by black triangles) containing eGFP, a Neo cassette, and a transcriptional stop sequence. This floxed sequence is followed by an HA-tagged Tlr9. PGK-DTA was used as a negative selection marker for ES cells; bPA represents the bovine growth hormone polyadenylation site. The top panels show the targeting plasmid and rosa26 locus, and the bottom 2 panels show the Rosa^Tlr9 locus before and after Cre-mediated excision. (B) qPCR analysis of TLR9 expression in sorted B cells from control (n = 7) and CD19-Cre Rosa^Tlr9 mice (n = 4) mice. (C) Representative Western blot showing TLR9-HA expression in CD19-Cre Rosa^Tlr9 mice but not control mice. Sorted B cells were immunoprecipitated (IP) with isotype control antibody (rat IgG1) or anti–HA antibody and immunoblotted with anti–HA antibody. Arrows depict the full-length (FL-TLR9) and cleaved (C-TLR9) forms of TLR9. (D) Sorted B cells from control and CD19-Cre Rosa^Tlr9 mice were stimulated with CpG ODN 1826 (at indicated concentrations) for 3 days and IgM secretion was measured by ELISA. Scatter plots display data from individual mice, with black lines showing means. (E) Left shows representative FACS plots showing GFP expression in CD19⁺ (red) and TCRβ⁺ cells derived from CD19-Cre Rosa^Tlr9 mice, with the right panel showing summary data from CD19-Cre⁺ and Cre-negative Rosa^Tlr9 mice (n = 42 and n = 46, respectively). For tabulated data, each dot denotes an individual mouse and horizontal lines represent the mean and standard deviation. *P < 0.05; **P < 0.01; ****P < 0.0001 using Student’s t test.