TY - JOUR
T1 - Regulation of gene expression in human prostate cancer cells with artificially constructed promoters that are activated in response to ultrasound stimulation
AU - Ogawa, Ryohei
AU - Morii, Akihiro
AU - Watanabe, Akihiko
AU - Cui, Zheng Guo
AU - Kagiya, Go
AU - Kondo, Takashi
AU - Doi, Nobutaka
AU - Feril, Loreto B.
N1 - Funding Information:
This work was supported in part by Grants-in-Aid for Scientific Research (C) (21500403 to R.O.) and for Young Scientist (B) (20377253 to A.W.) and (23791746 to A.M.) from Japan Society for the Promotion of Science. In addition, this research was also supported in part by Research and Development Committee Program of The Japan Society of Ultrasonics in Medicine (to R.O.).
PY - 2013/1
Y1 - 2013/1
N2 - We chose promoters responsive to sonication in LNCap cells, a prostate cancer cell line, out of a library composed of DNA fragments constructed by linking the TATA box sequence to randomly combined cis-acting elements of transcription factors activated in response to radiation in prostate cancer cells. When a plasmid containing the luciferase gene under control of a promoter was transfected into LNCap cells and sonicated with 1 MHz ultrasound at 0.5 W/cm2, 10% DF for 60 s, 13 promoters showed more than 10-fold enhancement compared with their counterparts without sonication 12 h after sonication. As to their responsiveness to sonication, the best two promoters were then compared to clone 880-8, a derivative from clone 880 that was created by random introduction of point mutations and was shown to have an improved response to X-ray irradiation. We then took clone 880-8 for further analyses since it showed the highest enhancement to sonication, though not statistically significant from the others. Next, we employed a retrovirus vector and stably introduced the luciferase gene under control of clone 880-8 into LNCap cells to establish a cell line. When the cell line was sonicated with 1 MHz ultrasound at 0.5 W/cm2, 10% DF for 60 s, luciferase expression was enhanced up to 14.8-fold 12 h after sonication. We then established another cell line by replacing the luciferase gene with the fcy::fur gene, a suicide gene, and when the cell line was sonicated with 1 MHz ultrasound at 0.5 W/cm2, 10% DF for 60 s, expression of the gene was enhanced, showing the maximum expression 12-24 h after sonication. When the cells were incubated in medium containing 5-fluorocytosine, cell survival ratio decreased dose dependently with 5-fluorocytosine only after sonication treatment, suggesting this promoter could be utilized for gene expression control with ultrasound.
AB - We chose promoters responsive to sonication in LNCap cells, a prostate cancer cell line, out of a library composed of DNA fragments constructed by linking the TATA box sequence to randomly combined cis-acting elements of transcription factors activated in response to radiation in prostate cancer cells. When a plasmid containing the luciferase gene under control of a promoter was transfected into LNCap cells and sonicated with 1 MHz ultrasound at 0.5 W/cm2, 10% DF for 60 s, 13 promoters showed more than 10-fold enhancement compared with their counterparts without sonication 12 h after sonication. As to their responsiveness to sonication, the best two promoters were then compared to clone 880-8, a derivative from clone 880 that was created by random introduction of point mutations and was shown to have an improved response to X-ray irradiation. We then took clone 880-8 for further analyses since it showed the highest enhancement to sonication, though not statistically significant from the others. Next, we employed a retrovirus vector and stably introduced the luciferase gene under control of clone 880-8 into LNCap cells to establish a cell line. When the cell line was sonicated with 1 MHz ultrasound at 0.5 W/cm2, 10% DF for 60 s, luciferase expression was enhanced up to 14.8-fold 12 h after sonication. We then established another cell line by replacing the luciferase gene with the fcy::fur gene, a suicide gene, and when the cell line was sonicated with 1 MHz ultrasound at 0.5 W/cm2, 10% DF for 60 s, expression of the gene was enhanced, showing the maximum expression 12-24 h after sonication. When the cells were incubated in medium containing 5-fluorocytosine, cell survival ratio decreased dose dependently with 5-fluorocytosine only after sonication treatment, suggesting this promoter could be utilized for gene expression control with ultrasound.
KW - Gene expression
KW - Gene therapy
KW - Promoter
KW - Ultrasound
UR - http://www.scopus.com/inward/record.url?scp=84867742923&partnerID=8YFLogxK
U2 - 10.1016/j.ultsonch.2012.05.007
DO - 10.1016/j.ultsonch.2012.05.007
M3 - 学術論文
C2 - 22695309
AN - SCOPUS:84867742923
SN - 1350-4177
VL - 20
SP - 460
EP - 467
JO - Ultrasonics Sonochemistry
JF - Ultrasonics Sonochemistry
IS - 1
ER -