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通过柱前衍生化和柱切换高效液相色谱-荧光检测法对新型抗缺血药物埃利罗地及其葡萄糖醛酸共轭物在人血浆和尿液中的立体选择性测定。

Stereoselective determination of unchanged and glucuroconjugated eliprodil, a new anti-ischaemic drug, in human plasma and urine by precolumn derivatization and column-switching high-performance liquid chromatography with fluorescence detection.

作者信息

Malavasi B, Ripamonti M, Rouchouse A, Ascalone V

机构信息

Synthélabo Recherche, Department of Chemical and Pharmaceutical Development, Limito, MI, Italy.

出版信息

J Chromatogr A. 1996 Apr 5;729(1-2):323-33. doi: 10.1016/0021-9673(95)00893-4.

DOI:10.1016/0021-9673(95)00893-4
PMID:9004957
Abstract

An HPLC method was developed and validated for the determination in human plasma and urine of the enantiomers of eliprodil, (+/-)-alpha-(4-chlorophenyl)-4[(4-fluorophenyl) methyl]piperidine-1-ethanol hydrochloride, a new anti-ischaemic agent administered as a racemate. Both enantiomers are present in human plasma in unchanged and glucuroconjugated form, whereas only the glucuroconjugated form is excreted into urine; as a consequence, such metabolites in human plasma and urine should be submitted to enzymatic deconjugation with beta-glucuronidase (Escherichia coli) before being extracted. The general method involves a liquid-liquid extraction of eliprodil and internal standard from alkalinized plasma or urine with n-hexane, evaporation of the organic phase and derivatization with (S)-(+)-naphthylethyl isocyanate to give carbamate diastereoisomeric derivatives of (S)-(+)- and (R)-(-)-eliprodil and internal standard; after evaporation of the derivatizing mixture and dissolution of the residue in a small volume of phosphate buffer-acetonitrile (60:40, v/v), an aliquot is injected into a column-switching HPLC system. The derivatized sample extract is purified on a precolumn filled with C8-bonded silica material, which is flushed with acetonitrile-water, then diastereoisomers of eliprodil and the internal standard are automatically transferred by the mobile phase to the analytical column. The analytical column is a C8 type, specially deactivated for basic compounds, the mobile phase is 0.025 M phosphate buffer (pH 2.6)-methanol-acetonitrile (42:2:56) at a flow-rate of 1.2 ml min-1 and fluorimetric detector operating at lambda ex = 275 nm and lambda em = 336 nm is used. The retention times, under these conditions, are about 16 and 17 min for (S)-(+)- and (R)-(-)-eliprodil diastereoisomers, respectively, and about 19 min for the first-eluted diastereoisomer of the internal standard. During the analysis time, the precolumn, reset in a different path from that of the analytical column, is back-flushed with different solvents, then re-equilibrated with acetonitrile-water before the next injection. Linearity in plasma, for unchanged eliprodil enantiomers, was assessed in the range 0.15-10 ng ml-1 and for total eliprodil enantiomers (unchanged + conjugated) in the range 0.75-500 ng ml-1; the limit of quantitation (LOQ) is 0.15 ng ml-1 for each unchanged enantiomer and 0.75 ng ml-1 for each total enantiomer. Linearity was also assessed in urine for total (conjugated) eliprodil enantiomers in the range 50-25 000 ng ml-1; the LOQ is 50 ng ml-1 for each enantiomer. The intra- and inter-day precision and accuracy of the method were investigated in plasma and urine and found to be satisfactory for pharmacokinetic studies. The method has been extensively used in pharamcokinetic studies in man treated with a 20-mg dose of eliprodil racemate and some results of this application are reported.

摘要

已开发并验证了一种高效液相色谱(HPLC)方法,用于测定人体血浆和尿液中依立普地尔对映体,即(±)-α-(4-氯苯基)-4-[(4-氟苯基)甲基]哌啶-1-乙醇盐酸盐,一种作为外消旋体给药的新型抗缺血药物。两种对映体在人体血浆中以未变化形式和葡萄糖醛酸结合形式存在,而只有葡萄糖醛酸结合形式排泄到尿液中;因此,人体血浆和尿液中的此类代谢物在提取前应使用β-葡萄糖醛酸酶(大肠杆菌)进行酶解结合。一般方法包括用正己烷从碱化的血浆或尿液中液-液萃取依立普地尔和内标,蒸发有机相并用(S)-(+)-萘基异氰酸酯进行衍生化,得到(S)-(+)-和(R)-(-)-依立普地尔及内标的氨基甲酸酯非对映体衍生物;蒸发衍生化混合物并将残渣溶解在少量磷酸盐缓冲液-乙腈(60:40,v/v)中后,取一份注入柱切换HPLC系统。衍生化的样品提取物在填充有C8键合硅胶材料的预柱上进行纯化,先用乙腈-水冲洗,然后依立普地尔和内标的非对映体由流动相自动转移至分析柱。分析柱为C8型,专为碱性化合物进行了特殊去活处理,流动相为0.025M磷酸盐缓冲液(pH 2.6)-甲醇-乙腈(42:2:56),流速为1.2 ml min-1,使用荧光检测器,激发波长λex = 275 nm,发射波长λem = 336 nm。在这些条件下,(S)-(+)-和(R)-(-)-依立普地尔非对映体的保留时间分别约为16和17分钟,内标第一个洗脱的非对映体保留时间约为19分钟。在分析过程中,预柱在与分析柱不同的路径中重新设置,先用不同溶剂反冲,然后在下一次进样前用乙腈-水重新平衡。对于未变化的依立普地尔对映体,血浆中的线性范围为0.15 - 10 ng ml-1,对于总依立普地尔对映体(未变化的 + 结合的),线性范围为0.75 - 500 ng ml-;每种未变化对映体的定量限(LOQ)为0.15 ng ml-1,每种总对映体的定量限为0.75 ng ml-1。尿液中总(结合的)依立普地尔对映体的线性范围为50 - 25 000 ng ml-1;每种对映体的定量限为50 ng ml-1。该方法在血浆和尿液中的日内和日间精密度及准确度进行了研究,发现对于药代动力学研究而言是令人满意的。该方法已广泛应用于接受20 mg剂量依立普地尔外消旋体治疗的人体药代动力学研究,并报告了此应用的一些结果。

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引用本文的文献

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Br J Pharmacol. 2004 Sep;143(1):152-8. doi: 10.1038/sj.bjp.0705901. Epub 2004 Aug 9.