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Hemolysis Assessment and Antioxidant Activity Evaluation Modified in an Oxidized Erythrocyte Model

机译:氧化红细胞模型中的溶血评估和抗氧化活性评估

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Hydrogen peroxide (H2O2)-induced hemolysis is a commonly used model for antioxidant activity evaluation, and the hemolysis index is often presented as the absorbance of supernatant hemoglobin (Hb), which releases from injured cells. However, in previous studies, as an oxidation-sensitive protein, it has been recognized that Hb easily forms other types or substances, such as metHb, Heinz, and some fluorescent products. This study concerns whether Hb oxidation participated in H2O2-induced hemolysis and confirmed that the destruction of Hb under oxidizing condition had been a novel interfering factor that could reduce the absorbance in Hb quantitative detection. To correct the lower absorbance, the stable fluorescent products found in Hb degradation were selected, and the absorbance correction factor of 6.436 was drawn on the basis of the absorbance and fluorescent intensity. This correction factor obviously altered the results of both dose-dependent hemolysis of H2O2 and antioxidant activity. In addition, the assessment difference was innovatively discussed by altering the sequences of adding antioxidant and oxidant. These different sequences caused variations in hemolysis, indicating that multiple evaluations may be related to the antioxidant pathways which are necessary for more accurate bioactivity data. Khemolysis;; indices correction;; fluorescence;; adding order
机译:过氧化氢(H2O2)诱导的溶血是抗氧化剂活性评估的常用模型,溶血指数通常表示为从受损细胞释放的上清血红蛋白(Hb)的吸光度。但是,在以前的研究中,人们已经认识到Hb作为一种对氧化敏感的蛋白质,很容易形成其他类型或物质,例如metHb,Heinz和某些荧光产物。这项研究关注Hb氧化是否参与H2O2诱导的溶血,并证实在氧化条件下Hb的破坏已成为一种新的干扰因素,可以降低Hb定量​​检测的吸光度。为了校正较低的吸光度,选择了在Hb降解中发现的稳定的荧光产物,并根据吸光度和荧光强度得出了吸光度校正因子6.436。该校正因子明显改变了H2O2剂量依赖性溶血和抗氧化活性的结果。此外,通过改变添加抗氧化剂和氧化剂的顺序创新性地讨论了评估差异。这些不同的序列导致溶血变化,表明多重评估可能与抗氧化剂途径有关,这对于更准确的生物活性数据是必需的。 K溶血;;指数修正;荧光;添加订单

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