色谱 ›› 2021, Vol. 39 ›› Issue (5): 526-533.DOI: 10.3724/SP.J.1123.2020.04028

• 技术与应用 • 上一篇    下一篇

固相萃取-超高效液相色谱-串联质谱法检测保健食品中9种人参皂苷

陈树东1,2,*(), 冯锐1, 林晓佳3, 梁土金1, 何秋婷2   

  1. 1.广东省中药研究所, 广东 广州 510640
    2.广东医科大学, 广东 东莞 523808
    3.广州检测认证集团有限公司, 广东 广州 511447
  • 收稿日期:2020-06-28 出版日期:2021-05-08 发布日期:2021-03-31
  • 通讯作者: 陈树东
  • 作者简介:Tel:(020)89285782,E-mail:uu3g@163.com.

Determination of nine ginsenosides in health foods by solid extraction phase-ultra performance liquid chromatography-tandem mass spectrometry

CHEN Shudong1,2,*(), FENG Rui1, LIN Xiaojia3, LIANG Tujin1, HE Qiuting2   

  1. 1. Guangdong Institute of Traditional Chinese Medicine, Guangzhou 510640, China
    2. Guangdong Medical University, Dongguan 523808, China
    3. Guangzhou Inspection Testing and Certification Group Co., Ltd., Guangzhou 511447, China
  • Received:2020-06-28 Online:2021-05-08 Published:2021-03-31
  • Contact: CHEN Shudong

摘要:

建立了以固相萃取结合超高效液相色谱-串联质谱(UPLC-MS/MS)同时检测保健食品中9种原人参二醇型和原人参三醇型人参皂苷的方法。保健食品中人参皂苷经过提取后,通过Alumina-N/XAD-2 SPE柱净化,在Hypersil Gold C18色谱柱(100 mm×2.1 mm, 1.9 μm)上分离,利用乙酸铵溶液(含0.1%甲酸)和乙腈作为流动相进行梯度洗脱,采用负离子扫描,多反应监测模式测定,外标法定量。研究通过对不同填料的固相萃取小柱的考察,最终选择了Alumina-N/XAD-2复合填料,其能对保健食品复杂基质中的人参皂苷进行有效富集和净化;通过考察人参皂苷的电离裂解过程,确定人参皂苷一级质谱准分子离子和相应的碎片离子,并经过色谱条件的优化,使质谱条件下一级质谱准分子离子和相应的碎片离子均一致的3种原人参二醇型人参皂苷Rb2、Rb3、Rc同分异构体实现完全分离。结果表明,9种人参皂苷在0.005~0.5 μg/mL范围内具有很好的线性关系,相关系数均大于0.9950。方法的加标回收率为81.1%~114.2%,相对标准偏差为0.4%~8.0%。所建立的方法采用XAD-2大孔吸附树脂和中性氧化铝的复合固相萃取材料,保健食品经过简单提取可直接作为固相萃取的上样溶液进行人参皂苷的富集和净化,通过超高效液相色谱-串联质谱不仅缩短了分析时间,也能对复杂基质样品中含量相对较低的人参皂苷进行准确定性和定量。该方法通量高,简单快速,重复性好,适用于保健食品中9种人参皂苷的定性和定量分析。

关键词: 超高效液相色谱-串联质谱, 固相萃取, 人参皂苷, 保健食品

Abstract:

Ginsenosides are the main active compounds of ginseng, American ginseng and Panax notoginseng. They have certain pharmacological effects on the cardiovascular, immune and central nervous systems. Most ginsenosides are naturally classified as protopanaxatriol (PPT), protopanaxadiol (PPD), and oleanolic acid (OA) according to their aglycone skeletons. The nine main ginsenosides are Rb1, Rb2, Rb3, Rc, Rd, Re, Rf, Rg1 and Rg2. Accurate quantification of ginsenosides is imperative because they are the characteristic components and quality evaluation indicators of health foods. A new method based on solid phase extraction-ultra performance liquid chromatography-tandem mass spectrometry (SPE-UPLC-MS/MS) was developed for the determination of the nine ginsenosides in health foods. First, the pretreatment conditions were optimized. With the aim of purifying the samples and removing impurities, SPE cartridges with different packing materials, such as Alumina-N/XAD-2 SPE Cartridge, C18 and HLB were investigated. Based on the purification efficiencies, recoveries and other factors, the Alumina-N/XAD-2 SPE cartridge composite SPE column was selected as the pretreatment purification column. The eluents were then optimized. When water was used as the eluent, the ginsenosides could remain adsorbed on the SPE column, and could not be eluted down with other water-soluble substances. By increasing the proportion of ethanol in the eluent, the ginsenoside adsorbed on the filler of the SPE column could be gradually eluted. When the proportion of ethanol in the eluent reached 70%, the ginsenosides could be completely eluted. The effects of different volumes of 70% ethanol elution solvent (5-30 mL) on the extraction efficiencies of ginsenosides were also investigated. The results showed that when the volume of the elution solvent reached 20 mL, the ginsenosides were completely eluted. Then, the chromatographic conditions and MS parameters were optimized. By examining the ionization cracking of ginsenosides, the quasi-molecular ions and corresponding fragment ions in ginsenoside primary MS were determined. After optimizing the chromatographic conditions and MS parameters, not only the sensitivity of the method was improved, but also the isomers Rb2, Rb3 and Rc with the same quasi-molecular ions and the corresponding fragment ions were completely separated. Good separation was achieved for the nine ginsenosides, thus meeting the requirements for accurate quantification. Finally, chromatographic separation was achieved on a Hypersil Gold C18 column (100 mm×2.1 mm, 1.9 μm) under linear gradient elution using a 5 mmol/L ammonium acetate solution (with 0.1% formic acid) and acetonitrile as the mobile phases. The nine ginsenosides were detected using a triple quadrupole MS detector under ESI - and multiple reaction monitoring (MRM) modes, and quantified by the external standard method. The nine ginsenosides showed a strong positive linear correlation (r 2>0.9950) in the range of 0.005-0.5 μg/mL. The sample recoveries and the corresponding relative standard deviations (RSDs) were 81.1%-114.2% and 0.4%-8.0% (n=6), respectively. Eleven batches of health foods on the market, among which six batches contained ginseng, American ginseng or Panax notoginseng ingredients, were analyzed by the developed method, and the ginsenosides were detected. The total ginsenosides contents were close to those mentioned on the label. However, the nine ginsenosides were detected in one batch of health food, whose label did not indicated ginseng, American ginseng or Panax notoginseng. The nine ginsenosides were not detected in the remaining batches of health foods.The health food extract was directly loaded and purified without any complex pretreatment. The UPLC⁃MS/MS method, not only helped shorten the analysis time, but also accurate quantification of low ginsenoside contents in complex matrix samples. The developed method is simple and rapid, with high throughput, thus being suitable for the quantitative analysis of the nine ginsenosides in health foods.

Key words: ultra performance liquid chromatography?tandem mass spectrometry (UPLC MS/MS), solid phase extraction (SPE), ginsenosides, health foods

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