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使用改良的 HPLC/DAD 方法对大麻中的大麻素进行定性和定量测量。

Qualitative and quantitative measurement of cannabinoids in cannabis using modified HPLC/DAD method.

机构信息

Chemical Terrorism, Biomonitoring and Food Testing Program, Public Health & Environmental Laboratories, New Jersey Department of Health, Ewing, NJ 08628, United States.

Chemical Terrorism, Biomonitoring and Food Testing Program, Public Health & Environmental Laboratories, New Jersey Department of Health, Ewing, NJ 08628, United States.

出版信息

J Pharm Biomed Anal. 2017 Nov 30;146:15-23. doi: 10.1016/j.jpba.2017.07.021. Epub 2017 Aug 10.

Abstract

This study presents an accurate and high throughput method for the quantitative determination of various cannabinoids in cannabis plant material using high pressure liquid chromatography (HPLC) with a diode array detector (DAD). Sample extraction and chromatographic analysis conditions for the measurement of cannabinoids in the complex cannabis plant material matrix were optimized. The Agilent Poroshell 120 SB-C18 column provided high resolution for all target analytes with a short run time (10minutes) given the core shell technology. The aqueous buffer mobile phase was optimized with ammonium acetate at pH 4.75. The change in the mobile phase and the new column ensured a separation between cannabidiol (CBD and cannabigerol (CBG) along with cannabigerol and tetrahydrocannabinolic acid (THCA), which were not well separated by previous publications, improved buffering capacity, and provided analytical performance stability. Moreover, baseline drifting was significantly minimized by the use of a low concentration buffer solution (25mM ammonium acetate). In addition, evaporation and reconstitution of the sample residue with a methanol-organic pure (OP) water solution (65:35) significantly reduced the matrix interference. The modified extraction produced good recoveries (>91%) for each of the eight cannabinoids. The optimized method was validated for specificity, linearity, sensitivity, precision, accuracy, and stability. The combined relative standard deviation (%RSD) for intra-day and inter-day precision for all eight analytes varied from 2.5% to 5.2% and 0.28% to 5.5%, respectively. The %RSD for the repeatability study varied from 1.1% to 5.5%. The recoveries from spiked cannabis matrix samples were greater than 90% for all analytes, except delta-8-tetrahydrocannabinol (Δ-THC), which was 80%. The recoveries varied from 81% to 107% with a precision of 0.7-8.1%RSD. Delta-9-tetrahydrocannabinol (Δ-THC) in all of the cannabis samples (n=635) was less than 10%, which is in compliance with the NJ Medicinal Marijuana regulation. Analysis of samples from two cultivars, which included ten individual samples, four composite samples, seven calibration standards, and four quality control standards, can be performed within 24hours by this high throughput method.

摘要

本研究提出了一种准确、高通量的方法,用于使用带有二极管阵列检测器 (DAD) 的高效液相色谱 (HPLC) 定量测定大麻植物材料中的各种大麻素。优化了用于测量复杂大麻植物材料基质中大麻素的样品提取和色谱分析条件。Agilent Poroshell 120 SB-C18 柱采用核壳技术,可在短运行时间(10 分钟)内为所有目标分析物提供高分辨率。优化了含有 pH 值为 4.75 的乙酸铵的水性缓冲移动相。流动相的变化和新的色谱柱确保了大麻二酚 (CBD) 和大麻萜酚 (CBG) 以及大麻萜酚和四氢大麻酚酸 (THCA) 之间的分离,这在以前的出版物中没有得到很好的分离,提高了缓冲能力,并提供了分析性能稳定性。此外,通过使用低浓度缓冲溶液 (25mM 乙酸铵),显著减少了基线漂移。此外,使用甲醇-有机纯 (OP) 水溶液 (65:35) 对样品残留物进行蒸发和再溶解,显著减少了基质干扰。改进的提取方法使八种大麻素的回收率均达到 91%以上。对该方法进行了特异性、线性、灵敏度、精密度、准确度和稳定性验证。所有八种分析物的日内和日间精密度的总相对标准偏差 (%RSD) 分别为 2.5%至 5.2%和 0.28%至 5.5%。重复性研究的 %RSD 变化范围为 1.1%至 5.5%。除了 δ-8-四氢大麻酚 (Δ-THC) 外,添加到大麻基质样品中的所有分析物的回收率均大于 90%,δ-8-THC 的回收率为 80%。回收率变化范围为 81%至 107%,精密度为 0.7-8.1%RSD。所有 635 个大麻样品中的 δ-9-四氢大麻酚 (Δ-THC) 均小于 10%,符合新泽西药用大麻法规的要求。通过这种高通量方法,可以在 24 小时内分析两个品种的十个单独样品、四个复合样品、七个校准标准品和四个质量控制标准品的样品。

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