Figure 1
Figure 1. DOX HIF-1αP402A/P564A/N803A transgene induction and target gene up-regulation. (A) Real-time reverse-transcribed polymerase chain reaction analysis of rapid and sustained elevations of transgene and “canonical” HIF-1 target gene mRNAs represented by glucose transporter-1 (Glut1) and CAIX in TetON-HIF-1 transgenic (denoted as “DTG” double transgenic) compared with NTG mice during continuous DOX induction. Prior analysis demonstrated no difference between NTG and DOX day 0 TetON-HIF-1 controls. (B) Transgene protein expression from Western blots of ear nuclear extracts on DOX day 14 in DTG, single TRE-HIF-1αP402/P464A/N803A transgenic mice (NTGTG), or NTG controls. Each dot in scatter plots represents one mouse. Horizontal bars represent the mean. Gene expression measurements for HIF-1α, Glut1, and CAIX were from the same samples. DTG data at each DOX day were compared with NTG or TetON-HIF-1 day 0 data (data not shown), using unpaired Student t test: **P < .01; ***P < .001. (C) Representative HIF-1α transgene and dual VEGF-keratin-14 immunofluorescence, showing expression localization in the interfollicular and hair follicle basal cell compartment after 3 and 14 days of DOX induction. Arrowheads indicate the basolateral VEGF localization within the basal cells. Bar represents 50 μm.

DOX HIF-1αP402A/P564A/N803A transgene induction and target gene up-regulation. (A) Real-time reverse-transcribed polymerase chain reaction analysis of rapid and sustained elevations of transgene and “canonical” HIF-1 target gene mRNAs represented by glucose transporter-1 (Glut1) and CAIX in TetON-HIF-1 transgenic (denoted as “DTG” double transgenic) compared with NTG mice during continuous DOX induction. Prior analysis demonstrated no difference between NTG and DOX day 0 TetON-HIF-1 controls. (B) Transgene protein expression from Western blots of ear nuclear extracts on DOX day 14 in DTG, single TRE-HIF-1αP402/P464A/N803A transgenic mice (NTGTG), or NTG controls. Each dot in scatter plots represents one mouse. Horizontal bars represent the mean. Gene expression measurements for HIF-1α, Glut1, and CAIX were from the same samples. DTG data at each DOX day were compared with NTG or TetON-HIF-1 day 0 data (data not shown), using unpaired Student t test: **P < .01; ***P < .001. (C) Representative HIF-1α transgene and dual VEGF-keratin-14 immunofluorescence, showing expression localization in the interfollicular and hair follicle basal cell compartment after 3 and 14 days of DOX induction. Arrowheads indicate the basolateral VEGF localization within the basal cells. Bar represents 50 μm.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal