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一种用于食品补充剂中β-胡萝卜素样品制备和测定的快速 HPLC 柱切换方法。

A rapid HPLC column switching method for sample preparation and determination of β-carotene in food supplements.

机构信息

Department of Analytical Chemistry, Faculty of Pharmacy, Charles University, Heyrovského 1203, Hradec Králové 500 05, Czech Republic.

出版信息

Food Chem. 2013 Nov 15;141(2):1433-7. doi: 10.1016/j.foodchem.2013.04.063. Epub 2013 Apr 30.

DOI:10.1016/j.foodchem.2013.04.063
PMID:23790935
Abstract

A simple and automated HPLC column-switching method with rapid sample pretreatment has been developed for quantitative determination of β-carotene in food supplements. Commercially samples of food supplements were dissolved in chloroform with help of saponification with 1M solution of sodium hydroxide in ultrasound bath. A 20-min sample dissolution/extraction step was necessary before chromatography analysis to transfer β-carotene from solid state of food supplements preparations (capsules,tablets) to chloroform solution. Sample volume - 3μL of chloroform phase was directly injected into the HPLC system. Next on-line sample clean-up was achieved on the pretreatment precolumn Chromolith Guard Cartridge RP-18e (Merck), 10×4.6mm, with a washing mobile phase (methanol:water, 92:8, (v/v)) at a flow rate of 1.5mL/min. Valve switch to analytical column was set at 2.5min in a back-flush mode. After column switching to the analytical column Ascentis Express C-18, 30×4.6mm, particle size 2.7μm (Sigma Aldrich), the separation and determination of β-carotene in food supplements was performed using a mobile phase consisting of 100% methanol, column temperature at 60°C and flow rate 1.5mL/min. The detector was set at 450nm. Under the optimum chromatographic conditions standard calibration curve was measured with good linearity - correlation coefficient for β-carotene (r(2)=0.999014; n=6) between the peak areas and concentration of β-carotene 20-200μg/mL. Accuracy of the method defined as a mean recovery was in the range 96.66-102.40%. The intraday method precision was satisfactory at three concentration levels 20, 125 and 200μg/mL and relative standard deviations were in the range 0.90-1.02%. The chromatography method has shown high sample throughput during column-switching pretreatment process and analysis in one step in short time (6min) of the whole chromatographic analysis.

摘要

已经开发出一种简单且自动化的 HPLC 柱切换方法,该方法具有快速的样品预处理功能,可用于定量测定食品补充剂中的β-胡萝卜素。通过在超声浴中用 1M 氢氧化钠溶液皂化,将市售的食品补充剂样品溶解于氯仿中。在色谱分析之前,需要进行 20 分钟的样品溶解/提取步骤,以便将β-胡萝卜素从食品补充剂制剂(胶囊,片剂)的固态转移到氯仿溶液中。将 3μL 的氯仿相直接注入 HPLC 系统中。接下来,通过在线预处理预柱 Chromolith Guard Cartridge RP-18e(默克),10×4.6mm,以 1.5mL/min 的流速用洗涤流动相(甲醇:水,92:8,(v/v))进行样品的在线清洗。在反冲洗模式下,将阀切换到分析柱的时间设置为 2.5 分钟。在切换到分析柱 Ascentis Express C-18,30×4.6mm,粒径 2.7μm(西格玛奥德里奇)之后,使用由 100%甲醇组成的流动相在 60°C 的柱温下以 1.5mL/min 的流速进行食品补充剂中β-胡萝卜素的分离和测定。将检测器设置为 450nm。在最佳色谱条件下,标准校准曲线的线性良好-β-胡萝卜素的峰面积与浓度之间的相关系数(r(2)=0.999014;n=6)为 20-200μg/mL。方法的准确度定义为平均回收率,在 20、125 和 200μg/mL 三个浓度水平的回收率范围为 96.66-102.40%。日内方法精密度在三个浓度水平 20、125 和 200μg/mL 下令人满意,相对标准偏差在 0.90-1.02%范围内。该色谱方法在柱切换预处理过程中具有较高的样品通量,并且在 6 分钟的短时间内即可完成整个色谱分析的一步分析。

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