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使用碳酸酐酶抑制法分析氯噻酮。

Chlorthalidone analysis using carbonic anhydrase inhibition.

作者信息

Johnston M M, Li H, Mufson D

出版信息

J Pharm Sci. 1977 Dec;66(12):1735-8. doi: 10.1002/jps.2600661220.

Abstract

Chlorthalidone was analyzed in the concentration range of 0.1-3.0 microgram/ml with a precision of +/- 0.05 microgram/ml. Chlorthalidone inhibition of the enzymatic hydrolysis rate of p-nitrophenyl acetate by bovine erythrocyte carbonic anhydrase was used as a basis for the determination. The amount of p-nitrophenol formed was measured by monitoring the absorbance at 400 nm, and its formation rate was proportional to the chlorthalidone concentration. The mixing of the enzyme, substrate, and sample, the incubation of the reaction mixture, and the recording of the absorbance were automated. A survey of urine samples from 26 normal human subjects did not reveal any endogenous substances that interfered with the assay. Analyses of urine samples from six subjects after oral administration of 100 mg of chlorthalidone indicated rapid absorption and a biphasic elimination. The alpha-phase half-life was 1.5 hr, and the beta-phase half-life was 35 hr.

摘要

氯噻酮在0.1 - 3.0微克/毫升的浓度范围内进行分析,精密度为±0.05微克/毫升。以氯噻酮对牛红细胞碳酸酐酶催化乙酸对硝基苯酯水解速率的抑制作用为测定基础。通过监测400纳米处的吸光度来测定对硝基苯酚的生成量,其生成速率与氯噻酮浓度成正比。酶、底物和样品的混合、反应混合物的孵育以及吸光度的记录均实现自动化。对26名正常人类受试者的尿液样本进行检测,未发现有任何内源性物质干扰该测定。对6名受试者口服100毫克氯噻酮后的尿液样本进行分析,结果表明吸收迅速且消除呈双相性。α相半衰期为1.5小时,β相半衰期为35小时。

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