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Antiproliferative and Antimigratory Activity of Poly-gallic Acid in Cancer Cell Lines

活力测定 MTT法 分子生物学 细胞培养 癌细胞 真皮成纤维细胞 化学 细胞生长 没食子酸 生物化学 细胞 成纤维细胞 生物 体外 癌症 抗氧化剂 遗传学
作者
Carmen G. Hernández-Valencia,Griselda Rodríguez‐Martínez,ANDRES M. CARRILES-PEREZ,DANIEL GONZALEZ-PEREZ,Carmina Ortega-Sánchez,Marco A. Andonegui-Elguera,Yessica Zamudio‐Cuevas,Javier Fernández‐Torres,Miguel A. Hernández-Valdepeña,Miquel Gimeno,Roberto Sánchez‐Sánchez
出处
期刊:Anticancer Research [International Institute of Anticancer Research (IIAR) Conferences 1997. Athens, Greece. Abstracts]
卷期号:44 (3): 1201-1208 被引量:1
标识
DOI:10.21873/anticanres.16915
摘要

Background/Aim: Enzyme-mediated grafting of poly (gallic acid) (PGAL) and L-arginine and a-L-lysine onto PGAL produces reactive oxygen species (ROS)-suppressor multiradical molecules with low cytotoxicity, high thermostability and water solubility with cancer treatment potential. This study examined the anticancer effects of these molecules in hepatic (HepG2, ATCC HB-8065), breast (MCF7, ATCC HTB-22), and prostate (PC-3, ATCC CRL-1435 and DU 145, ATCC HTB-81) cancer cell lines, as well as in fibroblasts from healthy human skin as control cells. Materials and Methods: PGAL was synthesized by the oxidative polymerization of the naturally abundant GA using laccase from Trametes versicolor. Insertions of amino acids L-arginine and α-L-lysine on the PGAL chain were carried out by microwave. The cells of dermal fibroblast (Fb) were obtained from primary skin cultures and isolated from skin biopsies. The cancer cells lines of hepatic (HepG2), breast (MCF7), and prostate (PC-3, DU 145) were obtained from ATCC. The viability of the cancer cells and the primary culture was obtained by the MTT assay. Proliferation was demonstrated by crystal violet assay. Cell migration was determined by Wound healing assay. Finally, cell cycle analysis was carried out with cells. Results: The results show that 200 μg/ml of PGAL cultured in vitro with prostate cancer cells decreased viability, proliferation, and migration, as well as arrested cells in the G1 and S phases of the cell cycle. In contrast, the dermal fibroblasts and the hepatic line remained unaffected. The random grafting of L-Arg and a-L-Lys onto the PGAL chain also decreased the viability of prostate cancer cells. Conclusion: PGAL and PGAL-grafted amino acids are potential adjuvants for prostate cancer treatment, with improved physicochemical characteristics compared to GA.

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