![Figure 6. Enforced CREB and ATF-2 expression trans-activates Gγ-promoter activity. (A) Western blot analysis showed increased phosphorylated and total CREB1 and ATF-2 protein levels after enforced expression for 12 and 24 hours after transfection. (B) The effect of increasing concentrations of pCMV-CREB on Gγ-promoter transcription was analyzed. Maximal trans-activation was observed at the 50-μg concentration at 24 hours. The base vector was transfected to control for nonspecific trans-activation. The bracket and star above the graph (comparison between the untransfected K562 cells [0] versus those treated with pCMV-CREB) represent significance at the P < .05 level. Data are shown as the mean ± SEM. (C) The effects of enforced ATF-2 (pDNA3.1ATF-2) expression on Gγ-promoter activity were tested. A robust concentration-dependent increase in luciferase activity was observed for both expression vectors. (D) The -1500GγLuc, -1350GγLuc, -1180GγLuc, and -1500AγLuc reporter plasmids (10 μg) were cotransfected into K562 cells with the constitutively active pCMV-CREB expression vector; luciferase activity was analyzed after 24 hours. A pattern of luciferase activity similar to that obtained with the HDACIs was observed. The star above the graph (comparison between untreated and pCMV-CREB-transfected cells) represents significance at the P < .05 level.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/108/10/10.1182_blood-2006-01-023713/4/zh80220603790006.jpeg?Expires=1722711384&Signature=oiciVXGl6vGADkM78k08dwtCd2gbsEAaJK6vumXXuhQNknSpiFd8DZJVdsNZ-lK3u1EU1M2RJTyfqy3RvCgCW6F6~lgiVIIKh9ulXUtL7UPi18gV6MeEOc8N38mfejGIDmVIaHvO0XyCdiWmnPPIUtbL0Rfifj7HsQB27Ruey96cBG~1GdyWJGCIbv2O6GvFIi2oVWZp1Y94-mag1truHGJGfg-x9WnQd-ZySr04vOT184s9wYUYCev40-gEMOvaN-8j~7evQhxWh8~zD3H1G7c6oGKJC6huKK7bNnOVvVWm5olQkugSeF3YXWPV6QNwPrLKFzP28r9XQEvDtaNNsw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Enforced CREB and ATF-2 expression trans-activates Gγ-promoter activity. (A) Western blot analysis showed increased phosphorylated and total CREB1 and ATF-2 protein levels after enforced expression for 12 and 24 hours after transfection. (B) The effect of increasing concentrations of pCMV-CREB on Gγ-promoter transcription was analyzed. Maximal trans-activation was observed at the 50-μg concentration at 24 hours. The base vector was transfected to control for nonspecific trans-activation. The bracket and star above the graph (comparison between the untransfected K562 cells [0] versus those treated with pCMV-CREB) represent significance at the P < .05 level. Data are shown as the mean ± SEM. (C) The effects of enforced ATF-2 (pDNA3.1ATF-2) expression on Gγ-promoter activity were tested. A robust concentration-dependent increase in luciferase activity was observed for both expression vectors. (D) The -1500GγLuc, -1350GγLuc, -1180GγLuc, and -1500AγLuc reporter plasmids (10 μg) were cotransfected into K562 cells with the constitutively active pCMV-CREB expression vector; luciferase activity was analyzed after 24 hours. A pattern of luciferase activity similar to that obtained with the HDACIs was observed. The star above the graph (comparison between untreated and pCMV-CREB-transfected cells) represents significance at the P < .05 level.
