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Preferentially enhanced gene expression from a synthetic human telomerase reverse transcriptase promoter in human cancer cells

Authors
Kim, Sung JinLee, Han SaemShin, June HoKim, Chul GeunJeong, SunjooPark, KeerangChoe, HanLee, Heuiran
Issue Date
Nov-2006
Publisher
Demetrios A. Spandidos Ed. & Pub.
Keywords
hTERT promoter; c-Myc; Sp1; gene regulatory element; TPL sequence; cancer gene therapy
Citation
Oncology Reports, v.16, no.5, pp 975 - 979
Pages
5
Indexed
SCIE
SCOPUS
Journal Title
Oncology Reports
Volume
16
Number
5
Start Page
975
End Page
979
URI
https://scholarworks.bwise.kr/hanyang/handle/2021.sw.hanyang/180771
DOI
10.3892/or.16.5.975
ISSN
1021-335X
1791-2431
Abstract
Although the human telomerase reverse transcriptase (hTERT) promoter can regulate cancer-specific genes, it is generally too weak to be effective. We therefore attempted to improve the potency of synthetic hTERT promoters by fusing the core element (E) of the hTERT promoter (H) and the tripartite leader sequence (T) from human adenovirus 5 in a combinatorial manner. To determine the potential as cancer-specific promoters, we measured luciferase activity driven by the chimeric hTERT promoters in human cancer cells. Among various constructs, the E3-H-T promoter induced the strongest luciferase activity in all the tested cancer cells. SK-Hep1 and Hela cells experienced 1000- and 11-fold higher expression than the basic hTERT promoter, respectively. Relative to the SV40 universal promoter, the E3-H-T promoter led to higher levels of gene expression. Using EMSA, we found that the hTERT enhancer region was specifically bound to c-Myc and Sp1. Thus, the data suggest that the E3-H-T promoter with up-regulated cancer-specific gene expression could be useful in cancer gene therapy.
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