Figure 1. Development and characterization of nCOX-2 cKOs. A, Diagram shows the mating scheme used to generate progeny with COX-2 coding sequence disrupted in all principal neurons of the hippocampus. Synapsin 1-driven cre recombinase mice were crossed with mice that had 34 bp loxP elements inserted into introns 5 and 8 of the COX-2 gene. B1–B4, Immunostaining for COX-2 demonstrates that COX-2 is expressed constitutively in CA3 pyramidal neurons in WT mice (B1), but not in the cKOs (B2). One day after pilocarpine-induced SE, COX-2 induction is observed in WT pyramidal neurons (B3), but not in cKO (B4). In all four panels, a pattern of nonneuronal COX-2 staining is preserved in the nCOX-2 cKO. C, Real time PCR demonstrates that only COX-2 expression from WT mice is enhanced 1 d after SE [Saline WT, n = 5; Pilocarpine (Pilo) WT, n = 6; Saline cKO, n = 5; Pilo cKO, n = 8; **p < 0.001, one-way ANOVA with Bonferroni post-tests]. Saline-treated WTs and nCOX-2 cKOs were not different (p > 0.05), but pilocarpine-treated WTs and nCOX-2 cKOs were significantly different (p < 0.001). D, PCR from DNA extracted from tail demonstrates that WT and cKO mice retain the 2 kb band reflecting the COX-2 gene in the periphery (primer locations shown in A). Scale bar, 10 μm. Error bars indicate SEM.