(A–C) DC2.4 cells were (A) treated with 1 μM T0901317 for the indicated times, (B) preincubated with actinomycin D, or (C) transfected with control siRNA (mock) or with siRNA specific for Nr1h3, Nr1h2, or both, then treated with T0901317. y axes denote fold change of Ccr7 mRNA relative to Ppia. *P < 0.05 versus respective 2-hour or mock control. (D) CCR7 promoter luciferase reporter constructs (left). HEK293T cells transfected with the indicated constructs and with Nr1h3 and Nr1h2 expression plasmids were incubated with DMSO (–) or 1 μM T0901317 for 24 hours. Shown is mean ± SD luciferase activity normalized to β-galactosidase (relative luciferase activity; RLU). (E) DC2.4 cells were incubated with vehicle or 5 μM T0901317 for 2 hours, and chromatin was prepared. Precipitated DNA was amplified using CCR7 primers located between –800 to –350 bp upstream of transcription start (LXR-responsive region; LXRR) and –3.8 kb (arrows), normalized to input chromatin. Results denote induction relative to vehicle-treated samples (set as 1). Shown is mean ± SD for a representative experiment assayed in triplicate. (F) Primary immature human DCs were incubated overnight with DMSO (vehicle only; VO) or 5 μM GW3965 and 1 μM 9-cis-retinoic acid (G+9). y axis denotes fold change of Ccr7 mRNA relative to Gapdh as mean ± SD (n = 6). *P = 0.001. (G) Primary immature human DCs were treated as in F and stained for CCR7 or with isotype-matched control antibody and analyzed by FACS. Representative results from 3 experiments are shown. (H) Primary immature human DCs were treated as in F, then placed in the top chamber of Transwell plates containing CCL21 in the bottom. 3 hours later, cells that migrated toward the lower chamber were counted and subtracted from cells that migrated in the absence of CCL21. Assays were performed in triplicate; shown is a representative experiment.