Figure 8.
Transcriptional activation of CXCR4 by PGE2. (A) HMECs were stimulated with physiologic PGE2 levels for 1 hour. Thereafter, CXCR4 mRNA expression was determined. (B) HMECs were stimulated with 10–9 M of PGE2 at indicated time points and CXCR4 mRNA expression was analyzed. Glyceraldehyde-3-phosphate dehydrogenase (GADPH) was used as control. A representative experiment of 2 is shown. (C) A schematic representation of reporter gene constructs containing the CXCR4 promoter region –691 bp up to +87 bp is provided, which shows the presence of consensus DNA-binding elements for several transcription factors. Controls consisted of the basic PGL3 vector containing the appropriate construct transfected into primary HMECs, in the presence or absence of PGE2, VEGF, or bFGF. The promoter activity for each construct after different stimulus is shown as normalized dual luciferase activity. The largest construct (pGL3-777) exhibited very little activity in response to different stimuli. The construct –191 to +87 (pGL3 279) yielded a 4-to 5-fold increase in activity after stimulation with VEGF, bFGF, and PGE2. (D) Sp1-binding sites are essential for induction of CXCR4 by VEGF, bFGF, and PGE2. Deletion studies were performed using the pGL3 279 construct as template; a construct with the NF-κB DNA-binding element deleted (pGL3 248) but containing the 3 Sp1-binding sites exhibited very similar responses to the construct pGl3 279. The smallest construct –50 to +83 (pGL3 142), which lacks the 3 Sp1-binding sites, showed virtually no response to any stimuli. The experiments depicted in this figure were performed several times. The bars represent SEM of 3 experiments, in which samples were run in triplicate.