Utility of porous graphitic carbon stationary phase in quantitative liquid chromatography/tandem mass spectrometry bioanalysis: quantitation of diastereomers in plasma

Xia, Yuanqing; Jemal, Mohammed; Zheng, Naiyu; Shen, Xiaohang

doi:10.1002/rcm.2517

Cited by 26 publications

(14 citation statements)

References 23 publications

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“…The ability of this graphitic material to retain small polar molecules is superior to that of silica-based sorbents (Gamelin et al, 1998;Fleming et al, 1993;Remaud et al, 2005;Ayrton et al, 1995;Gu and Lim, 1990;Cantu et al, 2001;Mazan et al, 2002;Gaudin et al, 2002;Jackson and Carr, 2002;Hanai, 2003;Antonio et al, 2007;Pereira et al, 2007;Merelli et al, 2007;Tachon et al, 2007;Xia et al, 2006;Roy et al, 2006;Bohnstedt et al, 2005;Reepmeyer et al, 2005;Xing et al, 2004;Thiebaut et al, 2006;Vial et al, 2001;Lepont et al, 2001;Holmgren et al, 2005). Moreover, porous graphitic carbon proved to be chemically and pH stable, and an inert stationary phase.…”

Section: Development Of a Pgc-hplc-ms/ms Methodsmentioning

confidence: 99%

A new, validated HPLC‐MS/MS method for the simultaneous determination of the anti‐cancer agent capecitabine and its metabolites: 5′‐deoxy‐5‐fluorocytidine, 5′‐deoxy‐5‐fluorouridine, 5‐fluorouracil and 5‐fluorodihydrouracil, in human plasma

Vainchtein

Rosing

Schellens

et al. 2009

Biomedical Chromatography

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A rapid and selective liquid chromatography/tandem mass spectrometric method was developed for the simultaneous determination of capecitabine and its metabolites 5'-deoxy-5-fluorocytidine (5'-DFCR), 5'-deoxy-5-fluorouracil (5'-DFUR), 5-fluorouracil (5-FU) and dihydro-5-fluorouracil (FUH(2)) in human plasma. A 200 microL human plasma aliquot was spiked with a mixture of internal standards fludarabine and 5-chlorouracil. A single-step protein precipitation method was employed using 10% (v/v) trichloroacetic acid in water to separate analytes from bio-matrices. Volumes of 20 microL of the supernatant were directly injected onto the HPLC system. Separation was achieved on a 30 x 2.1 mm Hypercarb (porous graphitic carbon) column using a gradient by mixing 10 mm ammonium acetate and acetonitrile-2-propanol-tetrahydrofuran (1 : 3 : 2.25, v/v/v). The detection was performed using a Finnigan TSQ Quantum Ultra equipped with the electrospray ion source operated in positive and negative mode. The assay quantifies a range from 10 to 1000 ng/mL for capecitabine, from 10 to 5000 ng/mL for 5'-DFCR and 5'-DFUR, and from 50 to 5000 ng/mL for 5-FU and FUH(2) using a plasma sample of 200 microL. Correlation coefficients (r(2)) of the calibration curves in human plasma were better than 0.99 for all compounds. At all concentration levels, deviations of measured concentrations from nominal concentration were between -4.41 and 3.65% with CV values less than 12.0% for capecitabine, between -7.00 and 6.59% with CV values less than 13.0 for 5'-DFUR, between -3.25 and 4.11% with CV values less than 9.34% for 5'-DFCR, between -5.54 and 5.91% with CV values less than 9.69% for 5-FU and between -4.26 and 6.86% with CV values less than 14.9% for FUH(2). The described method was successfully applied for the evaluation of the pharmacokinetic profile of capecitabine and its metabolites in plasma of treated cancer patients.

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Section: Development Of a Pgc-hplc-ms/ms Methodsmentioning

confidence: 99%

A new, validated HPLC‐MS/MS method for the simultaneous determination of the anti‐cancer agent capecitabine and its metabolites: 5′‐deoxy‐5‐fluorocytidine, 5′‐deoxy‐5‐fluorouridine, 5‐fluorouracil and 5‐fluorodihydrouracil, in human plasma

Vainchtein

Rosing

Schellens

et al. 2009

Biomedical Chromatography

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“…Moreover, it has shown a remarkable selectivity for structurally similar compounds, which is most likely caused by differences in analyte contact area with the planar carbon sheets (Xia et al, 2006). PGC has therefore been used to separate cytarabine (ara-C) and its MP from their endogenous stereoisomers cytidine and its MP (Gouy et al, 2006).…”

Section: Quantitative Nucleotide Analysis With Msmentioning

confidence: 99%

Mass spectrometry in the quantitative analysis of therapeutic intracellular nucleotide analogs

Jansen

Rosing

Schellens

et al. 2011

Mass Spectrometry Reviews

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Nucleoside analogs are widely used in anti-cancer, anti-(retro)viral, and immunosuppressive therapy. Nucleosides are prodrugs that require intracellular activation to mono-, di-, and finally triphosphates. Monitoring of these intracellular nucleotides is important to understand their pharmacology. The relatively involatile salts and ion-pairing agents traditionally used for the separation of these ionic analytes limit the applicability of mass spectrometry (MS) for detection. Both indirect and direct methods have been developed to circumvent this apparent incompatibility. Indirect methods consist of de-phosphorylation of the nucleotides into nucleosides before the actual analysis. Various direct approaches have been developed, ranging from the use of relatively volatile or very low levels of regular ion-pairing agents, hydrophilic interaction chromatography (HILIC), weak anion-exchange, or porous graphitic carbon columns to capillary electrophoresis and matrix-assisted light desorption--time of flight (MALDI-TOF) MS. In this review we present an overview of the publications describing the quantitative analysis of therapeutic intracellular nucleotide analogs using MS. The focus is on the different approaches for their direct analysis. We conclude that despite the technical hurdles, several useful MS-compatible chromatographic approaches have been developed, enabling the use of the excellent selectivity and sensitivity of MS for the quantitative analysis of intracellular nucleotides.

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“…Epimeric, diastereomeric and enantiomeric metabolites (Testa et al, 1993;Xia et al, 2006a) also cause the same kind of interference since such metabolites would obviously interfere with the SRM transition used for the quantitation of the drug.…”

Section: Metabolite Mass Spectrometric Interference In the Absence Ofmentioning

confidence: 99%

“…The purpose of using the modifi ed chromatographic conditions is to test if an additional peak would appear in the drug SRM channel, which would indicate the presence of a metabolite which is not separated from the drug under the initially used chromatographic conditions. With isomeric metabolites such as diastereomers, epimers and E/Z isomers, unlike metabolites that undergo in-source conversion to produce the drug molecular ion, there are no additional SRM channels that can distinguish the metabolites from the drug and hence chromatographic separation is essential (Xia et al, , 2006aTesta et al, 1993). It is impossible to know the chromatographic conditions or chromatographic run times required to achieve the chromatographic separation of the drug from such metabolites in the absence of authentic reference standards.…”

Section: Rationale and Strategy For The Use Of Incurred Sample For Mementioning

confidence: 99%

Systematic LC‐MS/MS bioanalytical method development that incorporates plasma phospholipids risk avoidance, usage of incurred sample and well thought‐out chromatography

Jemal

Ouyang

Xia

2009

Biomedical Chromatography

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181

124

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This treatise summarizes the underlying principle and the road map for systematic LC-MS/MS bioanalytical method development. The three themes that have recently emerged as central to building quality during method development-phospholipids, incurred sample and sound chromatographic considerations-are the main focus of this article. In order to reduce the bioanalytical risk associated with plasma phospholipids, a dual approach involving extraction and chromatography is recommended. The use of incurred sample during method development is essential to avoid interference arising from drug-related components. This is different from the current practice of incurred sample reanalysis, which tests reproducibility during method application. LC column/mobile phase optimization is needed to achieve appropriate peak shape, sensitivity and the separation of the analyte from interfering metabolites and phospholipids. Related to sound chromatographic considerations, we lay out facts and myths related to UPLC, vis-à-vis HPLC. Incorporation of quality during method development avoids the costly experience of finding out by chance about the invalidity of a method after it has been used in support of a number of pivotal clinical and non-clinical studies. To this end, we put forth an outline of a protocol for a systematic LC-MS/MS bioanalytical method development.

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Utility of porous graphitic carbon stationary phase in quantitative liquid chromatography/tandem mass spectrometry bioanalysis: quantitation of diastereomers in plasma

Cited by 26 publications

References 23 publications

A new, validated HPLC‐MS/MS method for the simultaneous determination of the anti‐cancer agent capecitabine and its metabolites: 5′‐deoxy‐5‐fluorocytidine, 5′‐deoxy‐5‐fluorouridine, 5‐fluorouracil and 5‐fluorodihydrouracil, in human plasma

A new, validated HPLC‐MS/MS method for the simultaneous determination of the anti‐cancer agent capecitabine and its metabolites: 5′‐deoxy‐5‐fluorocytidine, 5′‐deoxy‐5‐fluorouridine, 5‐fluorouracil and 5‐fluorodihydrouracil, in human plasma

Mass spectrometry in the quantitative analysis of therapeutic intracellular nucleotide analogs

Systematic LC‐MS/MS bioanalytical method development that incorporates plasma phospholipids risk avoidance, usage of incurred sample and well thought‐out chromatography

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