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采用高压液相色谱法和气相色谱法对生物体液中的Δ⁹-四氢大麻酚进行分离与分析。

Separation and analysis of delta 9-tetrahydrocannabinol in biological fluids by high-pressure liquid chromatography and GLC.

作者信息

Garrett E R, Hunt C A

出版信息

J Pharm Sci. 1977 Jan;66(1):20-6. doi: 10.1002/jps.2600660105.

DOI:10.1002/jps.2600660105
PMID:833737
Abstract

High-pressure liquid chromatographic (HPLC) systems were developed to separate quantitatively delta 9-tetrahydrocannabinol from heptane-extractable lipoidal and other endogenous substances in biological fluids. These substances interfered with the quantitation by flame-ionization GLC of the unmodified compound and by electron-capture GLC of the pentafluorobenzoyl derivative. Reversed-phase HPLC elution, with 47% acetonitrile in water, and normal-phase HPLC with 25% chloroform in heptane separated delta 9-tetrahydrocannabinol from 11-hydroxy-delta 9-tetrahydrocannabinol and other monohydroxylated tetrahydrocannabinols. These systems also purified stock solutions of delta 9-tetrahydrocannabinol from accompanying contaminants. The various monohydroxylated tetrahydrocannabinols were resolved from each other in the normal phase, 80% chloroform in heptane. The delta 8- and delta 9-tetrahydrocannabinols were separable in the normal phase with 5% tetrahydrofuran in hexane. The GLC analysis of pentafluorobenzoylated delta 9-tetrahydrocannabinol had a sensitivity of 1 ng/ml of plasma, with an estimated 5% standard error with the developed extraction and GLC procedures. Radiochemical analysis of the HPLC-separated fraction had a sensitivity of 0.2 ng/ml of plasma, with an estimated 2% standard error. There was no significant difference between the liquid scintillation and electron-capture GLC assays of the HPLC-separated delta 9-tetrahydrocannabinol obtained from the plasma of dogs administered the drug. Radiolabeled compounds can be added to plasma samples as internal standards to determine the recovery efficiencies of the several procedures in the analysis of unlabeled tetrahydrocannabinol.

摘要

高压液相色谱(HPLC)系统被开发用于从生物流体中的庚烷可提取类脂及其他内源性物质中定量分离出δ9 - 四氢大麻酚。这些物质干扰了未修饰化合物通过火焰离子化气相色谱(GLC)以及五氟苯甲酰衍生物通过电子捕获气相色谱进行的定量分析。在水中含47%乙腈的反相HPLC洗脱以及在庚烷中含25%氯仿的正相HPLC,可将δ9 - 四氢大麻酚与11 - 羟基 - δ9 - 四氢大麻酚及其他单羟基化四氢大麻酚分离。这些系统还能从伴随的污染物中纯化δ9 - 四氢大麻酚储备溶液。各种单羟基化四氢大麻酚在正相(庚烷中80%氯仿)中可相互分离。δ8 - 和δ9 - 四氢大麻酚在正相(己烷中5%四氢呋喃)中可分离。五氟苯甲酰化δ9 - 四氢大麻酚的气相色谱分析对血浆的检测灵敏度为1 ng/ml,采用所开发的提取和气相色谱方法估计标准误差为5%。对HPLC分离组分的放射化学分析对血浆的检测灵敏度为0.2 ng/ml,估计标准误差为2%。对给予该药物的犬血浆中通过HPLC分离得到的δ9 - 四氢大麻酚进行液体闪烁测定和电子捕获气相色谱测定,两者之间无显著差异。可将放射性标记化合物作为内标添加到血浆样品中,以确定在分析未标记四氢大麻酚时几种方法的回收率。

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引用本文的文献

1
Evidence that cannabidiol does not significantly alter the pharmacokinetics of tetrahydrocannabinol in man.有证据表明,大麻二酚不会显著改变人体内四氢大麻酚的药代动力学。
J Pharmacokinet Biopharm. 1981 Jun;9(3):245-60. doi: 10.1007/BF01059266.