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Optimization of a DNA Nicking Assay to Evaluate Oenocarpus bataua and Camellia sinensis Antioxidant Capacity

机译:DNA切刻法评价巴掌果和山茶抗氧化能力的优化

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摘要

This study was aimed at assessing the DNA damage protective activity of different types of extracts (aqueous, methanolic and acetonic) using an in vitro DNA nicking assay. Several parameters were optimized using the pUC18 plasmid, especially FeSO4, EDTA, solvent concentrations and incubation time. Special attention has been paid to removing the protective and damaging effect of the solvent and FeSO4 respectively, as well as to identifying the relevant positive and negative controls. For each solvent, the optimal conditions were determined: (i) for aqueous extracts, 0.33 mM of FeSO4 and 0.62 mM of EDTA were incubated for 20 min at 37 °C; (ii) for acetone extracts, 1.16% solvent were incubated for 15 min at 37 °C with 1.3 mM of FeSO4 and 2.5 mM of EDTA and (iii) for methanol extracts, 0.16% solvent, were incubated for 1.5 h at 37 °C with 0.33 mM of FeSO4 and 0.62 mM of EDTA. Using the optimized conditions, the DNA damage protective activity of aqueous, methanolic and acetonic extracts of an Amazonian palm berry (Oenocarpus bataua) and green tea (Camellia sinensis) was assessed. Aqueous and acetonic Oenocarpus bataua extracts were protective against DNA damage, whereas aqueous, methanolic and acetonic extracts of Camellia sinensis extracts induced DNA damage.
机译:这项研究旨在使用体外DNA切口测定法评估不同类型提取物(水性,甲醇和丙酮)的DNA损伤保护活性。使用pUC18质粒优化了几个参数,尤其是FeSO4,EDTA,溶剂浓度和孵育时间。特别注意分别去除溶剂和FeSO4的保护作用和破坏作用,以及确定相关的阳性和阴性对照。对于每种溶剂,确定了最佳条件:(i)对于水性提取液,将0.33 mM的FeSO4和0.62 mM的EDTA在37°C下孵育20分钟; (ii)对于丙酮提取物,将1.16%的溶剂与1.3 mM的FeSO4和2.5 mM的EDTA在37°C下孵育15分钟;(iii)对于0.16%的甲醇提取物,在37°C孵育1.5 h含0.33 mM的FeSO4和0.62 mM的EDTA。使用优化的条件,评估了亚马逊棕榈浆果(Oenocarpus bataua)和绿茶(Camellia sinensis)的水提取物,甲醇提取物和丙酮提取物的DNA损伤保护活性。水和丙酮酸巴氏荚果提取物对DNA损伤具有保护作用,而山茶提取物的水,甲醇和丙酮酸提取物可引起DNA损伤。

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