![Figure 1. Regulation of NF-κB distribution and activity by 5F11 and bortezomib. Detection of the NF-κB subunit p65 with anti-p65 and a secondary FITC-labeled antibody (green) in untreated L540 cells (A), after stimulation with cross-linked 5F11 for 6 and 8 hours (B-C), and after stimulation with bortezomib (D-E). The cell nuclei are stained with 4′6-diamidino-2-phenylindole (DAPI). Imaging medium was Vectashield (Vector Laboratories, Burlingame, CA). Pictures were taken using the digital Nikon Eclipse E800 microscope with the LuciaG/F program (Nikon, Düsseldorf, Germany). (A) 10 ×/0.17 NA objective; (B-E) 40 ×/0.11-0.23 NA objective. (F) L428 cells were transfected with either reporter construct pCMV-luc (transfection control) or pNF-κB-luc (bars 2-4) or pNF-κB-luc together with the expression vector IkBαM (bars 5-7) and exposed to PBS (basal), 5F11, or bortezomib for 24 hours. The luciferase activity (relative light units [RLU]) of the cell lysates is indicated. Error bars indicate mean and SD of 2 independent experiments. (G) EMSA to detect DNA binding of NF-κB in nuclear extracts of L540 and L428 cells after 6-hour incubation with no antibody, cross-linked 5F11, and cross-linked Ber-H2 (BH2) antibody. Ber-H2 as a control anti-CD30 antibody is unable to mediate CD30 signaling10 and fails to activate NF-κB. (H) Western blotting of whole L540 cell extracts to detect c-flip, bcl-2, and bax in untreated cells after 16-hour incubation (n.t. indicates no treatment) and following treatment with either 5F11 or 5F11 + bortezomib after 6-, 8-, and 16-hour incubation.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/106/5/10.1182_blood-2005-01-0427/6/zh80170583230001.jpeg?Expires=1723461550&Signature=mOK-GGNuxiiuM5L2a2BTLrdNypfS4ElWchOL07m1NEUsa2zlI7FVh4WeQ7A5JopKIhaNM0xUYET9rL8vFz3yqFj5Y4R5H0XqfWJoTnAgACcWHdEH4MIC6OVE9u-ikWuMZyMc-HBqs1xFCCvRXaI~0gooxQDHfT3RpbM5qbwj5MErWJyDYXwRUVcf4q08r8EzrutH05dm16p5PKCJupKLni2xQeNGZNpA6rG9Bn~zvIV6Jz8-Lp4DFowm14xoCx5ve63uSmMq~uYxcSxzSzfvKpESRUCNGV25mAU7YIgAlB68JLyp4ubvDIcPp8HS89FkGqozD15k3cbyDyC19Qra6Q__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Regulation of NF-κB distribution and activity by 5F11 and bortezomib. Detection of the NF-κB subunit p65 with anti-p65 and a secondary FITC-labeled antibody (green) in untreated L540 cells (A), after stimulation with cross-linked 5F11 for 6 and 8 hours (B-C), and after stimulation with bortezomib (D-E). The cell nuclei are stained with 4′6-diamidino-2-phenylindole (DAPI). Imaging medium was Vectashield (Vector Laboratories, Burlingame, CA). Pictures were taken using the digital Nikon Eclipse E800 microscope with the LuciaG/F program (Nikon, Düsseldorf, Germany). (A) 10 ×/0.17 NA objective; (B-E) 40 ×/0.11-0.23 NA objective. (F) L428 cells were transfected with either reporter construct pCMV-luc (transfection control) or pNF-κB-luc (bars 2-4) or pNF-κB-luc together with the expression vector IkBαM (bars 5-7) and exposed to PBS (basal), 5F11, or bortezomib for 24 hours. The luciferase activity (relative light units [RLU]) of the cell lysates is indicated. Error bars indicate mean and SD of 2 independent experiments. (G) EMSA to detect DNA binding of NF-κB in nuclear extracts of L540 and L428 cells after 6-hour incubation with no antibody, cross-linked 5F11, and cross-linked Ber-H2 (BH2) antibody. Ber-H2 as a control anti-CD30 antibody is unable to mediate CD30 signaling10 and fails to activate NF-κB. (H) Western blotting of whole L540 cell extracts to detect c-flip, bcl-2, and bax in untreated cells after 16-hour incubation (n.t. indicates no treatment) and following treatment with either 5F11 or 5F11 + bortezomib after 6-, 8-, and 16-hour incubation.
