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2'-2'-二氟脱氧胞苷和2'-2'-二氟脱氧尿苷核苷及核苷酸在多孔石墨化碳上的保留研究:液相色谱-串联质谱法的开发

Retention studies of 2'-2'-difluorodeoxycytidine and 2'-2'-difluorodeoxyuridine nucleosides and nucleotides on porous graphitic carbon: development of a liquid chromatography-tandem mass spectrometry method.

作者信息

Jansen Robert S, Rosing Hilde, Schellens Jan H M, Beijnen Jos H

机构信息

Department of Pharmacy & Pharmacology, Slotervaart Hospital/The Netherlands Cancer Institute, Amsterdam, The Netherlands.

出版信息

J Chromatogr A. 2009 Apr 10;1216(15):3168-74. doi: 10.1016/j.chroma.2009.02.002. Epub 2009 Feb 10.

DOI:10.1016/j.chroma.2009.02.002
PMID:19237159
Abstract

The development of a method for the separation of 2'-2'-difluorodeoxycytidine (gemcitabine, dFdC), 2'-2'-difluorodeoxyuridine (dFdU) and their mono-, di- and triphosphates using a porous graphitic carbon column (Hypercarb), without ion-pairing agent, is described. The retention of dFdC and dFdU could be controlled with an organic modifier (acetonitrile, CH(3)CN) and the retention of the anionic nucleotides with an eluting ion (bicarbonate). Separation of all analytes was achieved using a 0-25 mM ammonium bicarbonate gradient in CH(3)CN-H(2)O (15:85, v/v). Under these conditions, however, very long re-equilibration times were required. Injection of an acidic solution (100 microL 10% formic acid in H(2)O, v/v; 2.65 M) after running a gradient directly restored the separation capabilities of the column. Still, separation between the analytes slowly deteriorated over a period of months. These problems were solved by preconditioning the column with a pH buffered hydrogen peroxide (H(2)O(2)) solution (0.05% H(2)O(2) in CH(3)CN-H(2)O (15:85, v/v), pH 4) before starting an analytical run. The oxidation of the stationary phase with H(2)O(2) prevented its slow reduction, which most likely caused the decreasing retention times. The analytes were detected using tandem mass spectrometry.

摘要

描述了一种使用多孔石墨化碳柱(Hypercarb)分离2'-2'-二氟脱氧胞苷(吉西他滨,dFdC)、2'-2'-二氟脱氧尿苷(dFdU)及其单磷酸、二磷酸和三磷酸酯的方法,该方法无需离子对试剂。dFdC和dFdU的保留可通过有机改性剂(乙腈,CH(3)CN)控制,而阴离子核苷酸的保留则通过洗脱离子(碳酸氢盐)控制。使用CH(3)CN-H(2)O(15:85,v/v)中的0-25 mM碳酸氢铵梯度实现了所有分析物的分离。然而,在这些条件下,需要很长的重新平衡时间。在运行梯度后直接注入酸性溶液(100 μL H(2)O中10%的甲酸,v/v;2.65 M)可直接恢复柱的分离能力。尽管如此,分析物之间的分离在几个月内仍会缓慢恶化。通过在开始分析运行前用pH缓冲的过氧化氢(H(2)O(2))溶液(CH(3)CN-H(2)O(15:85,v/v)中0.05%的H(2)O(2),pH 4)对柱进行预处理,解决了这些问题。用H(2)O(2)氧化固定相可防止其缓慢还原,这很可能导致保留时间缩短。使用串联质谱法检测分析物。

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