The induction of activating transcription factor 3 (ATF3) contributes to anti-cancer activity of Abeliophyllum distichum Nakai in human colorectal cancer cells

被引:16
作者
Park, Gwang Hun [1 ]
Park, Jae Ho [2 ]
Eo, Hyun Ji [1 ]
Song, Hun Min [1 ]
Woo, So Hee [1 ]
Kim, Mi Kyoung [1 ]
Lee, Jin Wook [1 ]
Lee, Man Hyo [3 ]
Lee, Jeong Rak [3 ]
Koo, Jin Suk [4 ]
Jeong, Jin Boo [1 ,4 ,5 ]
机构
[1] Andong Natl Univ, Dept Bioresource Sci, Andong 760749, South Korea
[2] Jungwon Univ, Dept Med Plant Sci, Goesan 367805, South Korea
[3] Gyeongbuk Inst Bioind, Andong 760380, South Korea
[4] Andong Natl Univ, Ins Agr Sci & Technol, Andong 760749, South Korea
[5] Andong Natl Univ, Dept Med Plant Resources, Andong 760749, South Korea
来源
BMC COMPLEMENTARY AND ALTERNATIVE MEDICINE | 2014年 / 14卷
关键词
Abeliophyllum distichum Nakai; Activating transcription factor 3; Apoptosis; Cancer chemoprevention; Colorectal cancer; EXPRESSION; KINASE; PROMOTER; STRESS; NAG-1; GENE;
D O I
10.1186/1472-6882-14-487
中图分类号
R [医药、卫生];
学科分类号
10 ;
摘要
Background: Recently, Abeliophyllum distichum Nakai (A. distichum) has been reported to exert the inhibitory effect on angiotensin converting enzyme. However, no specific pharmacological effects from A. distichum have been described. We performed in vitro study to evaluate anti-cancer properties of A. distichum and then elucidate the potential mechanisms. Methods: Cell viability was measured by MTT assay. ATF3 expression level was evaluated by Western blot or RT-PCR and ATF3 transcriptional activity was determined using a dual-luciferase assay kit after the transfection of ATF3 promoter constructs. In addition, ATF3-dependent apoptosis was evaluated by Western blot after ATF3 knockdown using ATF3 siRNA. Results: Exposure of ethyl acetate fraction from the parts of A. distichum including flower, leaf and branch to human colorectal cancer cells, breast cancer cells and hepatocellular carcinoma reduced the cell viability. The branch extracts from A. distichum (EAFAD-B) increased the expression of activating transcription factor 3 (ATF3) and promoter activity, indicating transcriptional activation of ATF3 gene by EAFAD-B. In addition, our data showed that EAFAD-B-responsible sites might be between -147 and -85 region of the ATF3 promoter. EAFAD-B-induced ATF3 promoter activity was significantly decreased when the CREB site was deleted. However, the deletion of Ftz sites did not affect ATF3 promoter activity by EAFAD-B. We also observed that inhibition of p38MAPK and GSK3 beta attenuated EAFAD-B-mediated ATF3 promoter activation. Also, EAFAD-B contributes at least in part to increase of ATF3 accumulation. Conclusion: These findings suggest that the anti-cancer activity of EAFAD-B may be a result of ATF3 promoter activation and subsequent increase of ATF3 expression.
引用
收藏
页数:9
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