首页> 外文期刊>Journal of the Brazilian Chemical Society >HPLC/DAD determination of rosmarinic acid in Salvia officinalis: Sample preparation optimization by factorial design
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HPLC/DAD determination of rosmarinic acid in Salvia officinalis: Sample preparation optimization by factorial design

机译:HPLC / DAD法测定丹参中迷迭香酸的含量:通过因子设计优化样品制备

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Sage (Salvia officinalis) contains high amounts of the biologically active rosmarinic acid (RA) and other polyphenolic compounds. RA is easily oxidized, and may undergo degradation during sample preparation for analysis. The objective of this work was to develop and validate an analytical procedure for determination of RA in sage, using factorial design of experiments for optimizing sample preparation. The statistically significant variables for improving RA extraction yield were determined initially and then used in the optimization step, using central composite design (CCD). The analytical method was then fully validated, and used for the analysis of commercial samples of sage. The optimized procedure involved extraction with aqueous methanol (40%) containing an antioxidant mixture (ascorbic acid and ethylenediaminetetraacetic acid (EDTA)), with sonication at 45 °C for 20 min. The samples were then injected in a system containing a C_(18) column, using methanol (A) and 0.1% phosphoric acid in water (B) in step gradient mode (45A:55B, 0-5 min; 80A:20B, 5-10 min) with flow rate of 1.0 mL min-1 and detection at 330 nm. Using this conditions, RA concentrations were 50% higher when compared to extractions without antioxidants (98.94 ± 1.07% recovery). Auto-oxidation of RA during sample extraction was prevented by the use of antioxidants resulting in more reliable analytical results. The method was then used for the analysis of commercial samples of sage.
机译:鼠尾草(Salvia officinalis)含有大量具有生物活性的迷迭香酸(RA)和其他多酚化合物。 RA很容易被氧化,可能会在样品制备过程中发生降解以进行分析。这项工作的目的是开发和验证用于确定鼠尾草中RA的分析方法,并使用用于优化样品制备的析因设计实验。首先使用中央复合设计(CCD)确定提高RA提取产量的统计学上显着的变量,然后将其用于优化步骤。然后,对分析方法进行了充分验证,并将其用于分析鼠尾草的商业样品。优化的过程包括用含有抗氧化剂混合物(抗坏血酸和乙二胺四乙酸(EDTA))的甲醇水溶液(40%)萃取,并在45°C下超声处理20分钟。然后将样品以逐步梯度模式(45A:55B,0-5 min; 80A:20B,5)注入包含C_(18)柱的系统中,使用甲醇(A)和0.1%磷酸在水中的溶液(B) -10分钟),流速为1.0 mL min-1,并在330 nm处检测。在这种条件下,与不含抗氧化剂的提取物相比,RA的浓度要高50%(回收率98.94±1.07%)。使用抗氧化剂可防止样品提取过程中RA的自氧化,从而获得更可靠的分析结果。然后将该方法用于鼠尾草商业样品的分析。

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