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血浆醋硝香豆素水平的葡萄糖氧化酶法测定

GLC determination of plasma acenocoumarol levels.

作者信息

Midha K K, Cooper J K

出版信息

J Pharm Sci. 1977 Jun;66(6):799-802. doi: 10.1002/jps.2600660614.

Abstract

A method for the quantitative estimation of acenocoumarol in plasma is described. Plasma containing acenocoumarol, to which a known amount of gamma-oxo derivative of phenylbutazone is added as an internal standard, is acidified and extracted with ethylene dichloride. The drug and the internal standard are then back-extracted into alkali, which, in turn, is acidified and reextracted with ethylene dichloride. The organic extract is evaporated and treated with an ethereal solution of diazomethane (100 microliter). The reacted mixture is evaporated, and the residue is dissolved in 25 microliter of carbon disulfide. Aliquots (2-3 microliter) are injected into a gas chromatograph equipped with a flame-ionization detector. The methyl derivatives of acenocoumarol and the internal standard give sharp, well-separated, symmetrical peaks. The method is of sufficient sensitivity to determine 0.25 microgram/ml of the drug in plasma with a relative standard deviation of 4%.

摘要

本文描述了一种定量测定血浆中醋硝香豆素的方法。向含有醋硝香豆素的血浆中加入已知量的保泰松γ-氧代衍生物作为内标,将血浆酸化后用二氯乙烷萃取。然后将药物和内标反萃取到碱液中,碱液再酸化并用二氯乙烷重新萃取。将有机萃取液蒸发,并用重氮甲烷的乙醚溶液(100微升)处理。反应后的混合物蒸发,残留物溶解于25微升二硫化碳中。取等分试样(2 - 3微升)注入配有火焰离子化检测器的气相色谱仪中。醋硝香豆素和内标的甲基衍生物给出尖锐、分离良好且对称的峰。该方法灵敏度足够高,能够测定血浆中0.25微克/毫升的药物,相对标准偏差为4%。

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