OCL formation in cocultures of normal OCL precursors with p62−/− stromal cells treated with TNF-α. (A) CFU-GM cells (104 cells/well) from spleens of p62+/− mice were cultured with stromal cells from p62+/− and p62−/− mice for 7 days in the presence of TNF-α. The cells were then stained for TRAP, a marker enzyme of OCLs, and the number of TRAP+ multinucleated cells determined. Results represent the mean (± SEM) for 4 determinations. *P < .01 compared with cells cocultured with p62+/− cultures. (B) RANKL production by p62+/− and p62−/− mouse stromal cells. Stromal cells from long-term mouse marrow cultures were treated with media alone or TNF-α. Conditioned media were harvested 4 days after the start of the cultures. The concentration of soluble RANKL present was determined using an ELISA kit for mouse RANKL. Results are reported as RANKL concentration (pg/mL) and are the mean (± SEM) of 4 samples. *P < .01, compared with p62+/− stromal cell cultures. Similar results were seen in 3 independent experiments.