Fig. 2.
Fig. 2. MNNG induces uPA transcription in C2C12 cells: requirement of an AP1 enhancer element. / (A) Transcriptional activity of uPA promoter constructs in response to MNNG in C2C12 and NIH3T3 cells. C2C12 and NIH3T3 cells were transiently transfected with p-8.2Luc and p-0.035Luc, containing 8.2 kb and 35 bp, respectively, of murine uPA 5′-flanking region ligated upstream of the luciferase reporter gene, and luciferase activity was determined after 8 hours stimulation with 70 μmol/L MNNG. Three independent experiments, showing less than 25% variability in luciferase activity, were performed. Luciferase activity corresponding to each plasmid in the absence of MNNG stimulation was arbitrarily assigned a value of 1. (B) Luciferase induction of uPA promoter-containing cell lines by MNNG. C2C12 cells were stably transfected with different uPA 5′-deletion mutants, containing −0.035 kb, −2.0 kb, −4.9 kb, −6.6 kb, and −8.2 kb, respectively. For each uPA-luciferase plasmid transfection, neomycin-resistant colonies were pooled and chimerical plasmid insertion was normalized by Southern blot analysis with a luciferase DNA probe, as described in Miralles et al,72 and the corresponding cell lines were treated or not with MNNG for 8 hours. Luciferase activities for each cell line are expressed relative to the activity found in the corresponding untreated cells, which was assigned a value of 1. Values are the mean value of 4 experiments. (C) The uPA AP1-enhancer is required for MNNG transcriptional induction. C2C12 cells stably transfected with different uPA promoter-luciferase constructs containing (as in panel B) or lacking the AP1-enhancer (p-8.2(ΔAP1)Luc, p-6.6(ΔAP1)Luc, p-4.9(ΔAP1)Luc,72were treated with MNNG as described in (A). Only results obtained with p-8.2Luc– and p-8.2(ΔAP1)Luc–containing cell lines are shown. Luciferase activity for each cell line is expressed relative to the activity found in the untreated cells, which was assigned a value of 1. All normalized activities represent a minimum of 4 experiments, showing less than 25% variability. (D) MNNG treatment induces AP1-binding activity to the uPA enhancer element. Left: Induction of uPA 5′-TRE- and 3′-TRE-binding activities by MNNG treatment. C2C12 cells were grown in 0.5% FBS for 16 hours and either treated (+) or not (−) with MNNG (70 μmol/L) for 2 hours. Nuclear extracts were prepared at 2 hours after treatment and incubated with 20 000 cpm of the indicated32P-labeled probes, corresponding to the 5′-TRE (AP1A) and 3′-TRE (AP1B) elements of the uPA promoter, respectively. Right: Specificity of the induced uPA AP1-binding activity. Two-hour–induced C2C12 nuclear extract was incubated with the labeled AP1A or AP1Boligonucleotide, respectively, in the absence or presence of 150-fold molar excess of unlabeled competitors (described in the “Materials and methods” section): cold AP1A and AP1Bwere used as specific competitors for the corresponding labeled oligonucleotides, whereas cold IgκB (κB site of the Igκ enhancer) was used as unrelated competitor. The filled arrowhead indicates specific TRE-binding complexes.

MNNG induces uPA transcription in C2C12 cells: requirement of an AP1 enhancer element.

(A) Transcriptional activity of uPA promoter constructs in response to MNNG in C2C12 and NIH3T3 cells. C2C12 and NIH3T3 cells were transiently transfected with p-8.2Luc and p-0.035Luc, containing 8.2 kb and 35 bp, respectively, of murine uPA 5′-flanking region ligated upstream of the luciferase reporter gene, and luciferase activity was determined after 8 hours stimulation with 70 μmol/L MNNG. Three independent experiments, showing less than 25% variability in luciferase activity, were performed. Luciferase activity corresponding to each plasmid in the absence of MNNG stimulation was arbitrarily assigned a value of 1. (B) Luciferase induction of uPA promoter-containing cell lines by MNNG. C2C12 cells were stably transfected with different uPA 5′-deletion mutants, containing −0.035 kb, −2.0 kb, −4.9 kb, −6.6 kb, and −8.2 kb, respectively. For each uPA-luciferase plasmid transfection, neomycin-resistant colonies were pooled and chimerical plasmid insertion was normalized by Southern blot analysis with a luciferase DNA probe, as described in Miralles et al,72 and the corresponding cell lines were treated or not with MNNG for 8 hours. Luciferase activities for each cell line are expressed relative to the activity found in the corresponding untreated cells, which was assigned a value of 1. Values are the mean value of 4 experiments. (C) The uPA AP1-enhancer is required for MNNG transcriptional induction. C2C12 cells stably transfected with different uPA promoter-luciferase constructs containing (as in panel B) or lacking the AP1-enhancer (p-8.2(ΔAP1)Luc, p-6.6(ΔAP1)Luc, p-4.9(ΔAP1)Luc,72were treated with MNNG as described in (A). Only results obtained with p-8.2Luc– and p-8.2(ΔAP1)Luc–containing cell lines are shown. Luciferase activity for each cell line is expressed relative to the activity found in the untreated cells, which was assigned a value of 1. All normalized activities represent a minimum of 4 experiments, showing less than 25% variability. (D) MNNG treatment induces AP1-binding activity to the uPA enhancer element. Left: Induction of uPA 5′-TRE- and 3′-TRE-binding activities by MNNG treatment. C2C12 cells were grown in 0.5% FBS for 16 hours and either treated (+) or not (−) with MNNG (70 μmol/L) for 2 hours. Nuclear extracts were prepared at 2 hours after treatment and incubated with 20 000 cpm of the indicated32P-labeled probes, corresponding to the 5′-TRE (AP1A) and 3′-TRE (AP1B) elements of the uPA promoter, respectively. Right: Specificity of the induced uPA AP1-binding activity. Two-hour–induced C2C12 nuclear extract was incubated with the labeled AP1A or AP1Boligonucleotide, respectively, in the absence or presence of 150-fold molar excess of unlabeled competitors (described in the “Materials and methods” section): cold AP1A and AP1Bwere used as specific competitors for the corresponding labeled oligonucleotides, whereas cold IgκB (κB site of the Igκ enhancer) was used as unrelated competitor. The filled arrowhead indicates specific TRE-binding complexes.

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