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基于无需萃取的样品制备方法和液相色谱/(大气压化学电离)质谱联用技术同时测定人血浆中的二甲双胍和格列本脲。

Simultaneous assay of metformin and glibenclamide in human plasma based on extraction-less sample preparation procedure and LC/(APCI)MS.

作者信息

Georgita Cristina, Albu Florin, David Victor, Medvedovici Andrei

机构信息

S.C. Labormed Pharma S.A., Splaiul Independentei No. 319E, Bucharest 060044, Romania.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2007 Jul 1;854(1-2):211-8. doi: 10.1016/j.jchromb.2007.04.032. Epub 2007 May 1.

DOI:10.1016/j.jchromb.2007.04.032
PMID:17500048
Abstract

Separation of metformin and glibenclamide was achieved within a single chromatographic run on a Zorbax CN column, under isocratic conditions, using acetonitrile and aqueous component (0.01 moles/L ammonium acetate adjusted at pH 3.5 with acetic acid) in volumetric ratio 1/1. Plasma sample preparation is based on protein precipitation by means of organic solvent addition. 1,3,5-Triazine-2,4,6-triamine (IS1) was used as internal standard for metformin, while gliquidone (IS2) played the same role for glibenclamide. Detection was performed with an ion trap mass analyzer, using atmospheric pressure chemical ionization (APCI). A single MS stage was used for detection of metformin and IS1, by extracting ion chromatograms corresponding to molecular ions. MS/MS detection in the SRM mode was used for glibenclamide (m/z transition from 494 to 369 Da) and IS2 (m/z transition from 528 to 403 Da). The method produces linear responses up to 2000 ng/mL for metformin and 400 ng/mL for glibenclamide, respectively. Low limits of quantification were found in the 40 ng/mL range for metformin and at the 4 ng/mL level for glibenclamide. Precision was characterized by relative standard deviations (RSD%) below 9%. The analytical method was successfully applied to a single dose, open-label, randomized, two-period, two-sequence, crossover bioequivalence study of two commercially available anti-diabetic combinations containing 400 mg metformin and 2.5 mg of glibenclamide per coated tablet.

摘要

在Zorbax CN柱上,采用等度洗脱条件,以体积比1/1的乙腈和水性组分(0.01摩尔/升用乙酸调节至pH 3.5的醋酸铵),在一次色谱运行中实现了二甲双胍和格列本脲的分离。血浆样品制备基于通过添加有机溶剂进行蛋白质沉淀。1,3,5 - 三嗪 - 2,4,6 - 三胺(IS1)用作二甲双胍的内标,而格列喹酮(IS2)对格列本脲起相同作用。使用大气压化学电离(APCI)的离子阱质谱仪进行检测。通过提取对应于分子离子的离子色谱图,使用单级质谱检测二甲双胍和IS1。在SRM模式下进行MS/MS检测用于格列本脲(m/z从494到369 Da的转变)和IS2(m/z从528到403 Da的转变)。该方法对二甲双胍和格列本脲分别产生高达2000 ng/mL和400 ng/mL的线性响应。二甲双胍的低定量限在40 ng/mL范围内,格列本脲在4 ng/mL水平。精密度以低于9%的相对标准偏差(RSD%)为特征。该分析方法成功应用于一项单剂量、开放标签、随机、两周期、两序列、交叉生物等效性研究,该研究涉及两种市售抗糖尿病组合,每片包衣片中含有400 mg二甲双胍和2.5 mg格列本脲。

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