Fig. 2.
Fig. 2. Transcriptional activity of reporter constructs driven by Ig regulatory elements or the HSV-tk promoter. / (A) Namalwa, BJA-B, DG-75, Raji and Jok-1 cells (control B-cell lines), and L428 and KM-H2 cells (HD cell lines) were transfected with the wild type promoter-driven luciferase reporters (μET1) and the mutant promoter-driven reporters (μET1m). The activity of the mutant promoters was set to 1 for all cell lines and the specific activity of the wild-type promoter-driven reporter is shown as relative activity. All transfections were independently repeated minimally 3 times and in all cases a tk-driven renilla-luciferase reporter was co-transfected to correct for differences in transfection efficiencies. (B) Similar transfection as in A with luciferase reporters containing the intact tk-promoter (tk.luc, −109 to +52) or a truncated version of this promoter (pTATA, −38 to +52). The activity of the truncated promoter was set to 1 and tk.luc activity is shown relative to pTATA. (C) Schematic representation of the reporter constructs used in A and B. O = octamer motif (the mutated octamer motif is indicated by the crossed out symbol); T = TATA box. The enhancer fragment is not drawn to scale (the 1000 bp XbaI fragment of the enhancer was used).40

Transcriptional activity of reporter constructs driven by Ig regulatory elements or the HSV-tk promoter.

(A) Namalwa, BJA-B, DG-75, Raji and Jok-1 cells (control B-cell lines), and L428 and KM-H2 cells (HD cell lines) were transfected with the wild type promoter-driven luciferase reporters (μET1) and the mutant promoter-driven reporters (μET1m). The activity of the mutant promoters was set to 1 for all cell lines and the specific activity of the wild-type promoter-driven reporter is shown as relative activity. All transfections were independently repeated minimally 3 times and in all cases a tk-driven renilla-luciferase reporter was co-transfected to correct for differences in transfection efficiencies. (B) Similar transfection as in A with luciferase reporters containing the intact tk-promoter (tk.luc, −109 to +52) or a truncated version of this promoter (pTATA, −38 to +52). The activity of the truncated promoter was set to 1 and tk.luc activity is shown relative to pTATA. (C) Schematic representation of the reporter constructs used in A and B. O = octamer motif (the mutated octamer motif is indicated by the crossed out symbol); T = TATA box. The enhancer fragment is not drawn to scale (the 1000 bp XbaI fragment of the enhancer was used).40 

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