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首页> 外文期刊>Journal of Pharmaceutical and Biomedical Analysis: An International Journal on All Drug-Related Topics in Pharmaceutical, Biomedical and Clinical Analysis >Optimization and validation of reverse phase HPLC method for qualitative and quantitative assessment of polyphenols in seaweed
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Optimization and validation of reverse phase HPLC method for qualitative and quantitative assessment of polyphenols in seaweed

机译:逆相HPLC方法的优化与验证海藻中多酚定性评估的定性和定量评估

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Graphical abstract Display Omitted Highlights ? Optimization and validation of RP-HPLC-DAD method for seaweed polyphenols. ? Validation was based on calibration curve, linearity, LOD, LOQ and precision. ? 7 polyphenols were identified by LC-DAD-ESI–MS/MS in Himanthalia elongata seaweed. ? Phloroglucinol was the major polyphenol followed by gallic acid in H. elongata. ? Purified fraction showed 146.9% higher antioxidant activity than the ascorbic acid. Abstract A simple reverse phase-high performance liquid chromatography (RP–HPLC) coupled to a diode array detector (DAD) and negative ion electrospray mass spectrometer (ESI–MS) method was developed for simultaneous identification and quantification of phenolic antioxidants in seaweed. The proposed method was validated in terms of linearity, limits of detection (LOD), limits of quantification (LOQ), recovery and intermediate precision. The calibration curves were linear with correlation coefficient ranging from 0.9909 to 0.9997 while the values of LOD (0.26–0.82mg/L), LOQ (0.77–2.50mg/L), recovery (≥97.2%) and precision in terms of retention time (%RSD ≤2.27) and peak area (% RSD ≤5.11) were satisfactory. Brown seaweed Himanthalia elongata used in this study was extracted with 60% methanol and the crude extract was cleaned with SPE (Solid Phase Extraction) cartridge. HPLC-DAD-MS/MS analysis of the SPE fraction allowed the identification of 7 phenolic compounds comprising phlorotannins, hydroxybenzoic acid, hydroxycinnamic acid and flavonols subclasses of polyphenols. Quantitative analysis of these compounds revealed the presence of phloroglucinol (394.1±4.33μg/g), gallic acid (96.3±3.12μg/g), chlorogenic acid (38.8±1.94μg/g), caffeic acid (44.4±2.72μg/g), ferulic acid (17.6±0.85μg/g), myricetin (8.6±0.85μg/g) and quercetin (4.2±0.15μg/g), in the extract. The SPE fraction were tested for antioxidant capacity which were significantly (P 50 ; 14.5±0.57mg/g) than the ascorbic acid (EC 50 ; 35.8±0.59mg/g) and the crude extract (EC 50 ; 46.3±0.48mg/g). The occurrence of all these phenolic antioxidant compounds in H. elongata extract suggested that the developed method is sensitive enough and reproducible and could be used for qualitative and quantitative assessment of polyphenols in seaweed.
机译:图形抽象显示省略了亮点?海藻多酚RP-HPLC-DAD方法的优化与验证。还是验证基于校准曲线,线性,LOD,LOQ和精度。还是通过LCANTHALIA ELONGATA海藻中的LC-DAD-ESI-MS / MS鉴定了7种多酚。还是甘油酸是主要的多酚,然后是H.Ilongata的Galic酸。还是纯化的级分显示​​比抗坏血酸更高的抗氧化活性较高的146.9%。摘要耦合到二极管阵列检测器(爸爸)和负离子电喷雾质谱仪(ESI-MS)方法的简单反相高效液相色谱(RP-HPLC)以同时鉴定和定量海藻中的酚类抗氧化剂。所提出的方法在线性,检测限(LOD),定量限制(LOQ),恢复和中间精度方面进行了验证。校准曲线具有线性,相关系数为0.9909至0.9997,而LOD值(0.26-0.82mg / L),LOQ(0.77-2.50mg / L),恢复(≥97.2%)和保留时间的精确度(%RSD≤2.27)和峰面积(%RSD≤5.11)令人满意。本研究中使用的棕色海藻Himanthalia Elongata用60%甲醇提取,用SPE(固相萃取)盒清洗粗提取物。 HPLC-DAD-MS / MS分析SPE级分允许鉴定鉴定包含氟丙蛋白,羟基苯甲酸,羟基氨基酸和黄酮酚的黄鼠亚类的7种酚类化合物。这些化合物的定量分析显示氟葡糖醇(394.1±4.33μg/ g)的存在,无碱酸(96.3±3.12μg/ g),绿原酸(38.8±1.94μg/ g),咖啡酸(44.4±2.72μg/ g ),在提取物中,乳突酸(17.6±0.85μg/ g),myricetin(8.6±0.85μg/ g)和槲皮素(4.2±0.15μg/ g)。测试SPE部分的抗氧化能力,显着(P 50; 14.5±0.57mg / g)比抗坏血酸(EC 50; 35.8±0.59mg / g)和粗提物(EC 50; 46.3±0.48mg / G)。 H. Elongata提取物中所有这些酚类抗氧化剂化合物的发生表明,发育方法足够敏感,可再现,可用于海藻中多酚的定性和定量评估。

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