首页> 美国卫生研究院文献>Sensors (Basel Switzerland) >Determination of DPPH Radical Oxidation Caused by Methanolic Extracts of Some Microalgal Species by Linear Regression Analysis of Spectrophotometric Measurements
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Determination of DPPH Radical Oxidation Caused by Methanolic Extracts of Some Microalgal Species by Linear Regression Analysis of Spectrophotometric Measurements

机译:分光光度法线性回归分析测定某些微藻种甲醇提取物引起的DPPH自由基氧化

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摘要

The demonstrated modified spectrophotometric method makes use of the 2,2-diphenyl-1-picrylhydrazyl (DPPH) radical and its specific absorbance properties. The absorbance decreases when the radical is reduced by antioxidants. In contrast to other investigations, the absorbance was measured at a wavelength of 550 nm. This wavelength enabled the measurements of the stable free DPPH radical without interference from microalgal pigments. This approach was applied to methanolic microalgae extracts for two different DPPH concentrations. The changes in absorbance measured vs. the concentration of the methanolic extract resulted in curves with a linear decrease ending in a saturation region. Linear regression analysis of the linear part of DPPH reduction versus extract concentration enabled the determination of the microalgae's methanolic extracts antioxidative potentials which was independent to the employed DPPH concentrations. The resulting slopes showed significant differences (6 - 34 μmol DPPH g−1 extract concentration) between the single different species of microalgae (Anabaena sp., Isochrysis galbana, Phaeodactylum tricornutum, Porphyridium purpureum, Synechocystis sp. PCC6803) in their ability to reduce the DPPH radical. The independency of the signal on the DPPH concentration is a valuable advantage over the determination of the EC50 value.
机译:证明了改进的分光光度法使用了2,2-二苯基-1-吡啶并肼基(DPPH)自由基及其比吸收特性。当自由基被抗氧化剂还原时,吸光度会降低。与其他研究相反,在550 nm波长处测量吸光度。该波长使得能够测量稳定的游离DPPH自由基,而不受微藻色素的干扰。该方法应用于两种不同DPPH浓度的甲醇微藻提取物。测得的吸光度相对于甲醇提取物浓度的变化导致曲线的线性下降终止于饱和区域。 DPPH减少的线性部分对提取物浓度的线性回归分析使得能够确定微藻的甲醇提取物的抗氧化电位,该电位与所采用的DPPH浓度无关。所得的斜率显示出单个不同种类的微藻(Anabaena sp。,Isochrysis galbana,Phaeodyylum tricornutum,Porphyridium purpureum,Synechochocystis sp。PCC6803)之间的显着差异(6-34μmolDPPH g −1 提取物浓度)。 )降低DPPH自由基的能力。信号对DPPH浓度的独立性是确定EC50值的宝贵优势。

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