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Phenotyping of CYP450 in human liver microsomes using the cocktail approach

Publié dansAnalytical & bioanalytical chemistry, vol. 406, p. 4875-4887
Date de publication2014
Résumé

The cocktail approach is an advantageous strategy used to monitor the activities of several cytochromes P450 (CYPs) in a single test to increase the throughput of in vitro phenotyping studies. In this study, a cocktail mixture was developed with eight CYP-specific probe substrates to simultaneously evaluate the activity of the most important CYPs, namely, CYP1A2, CYP2A6, CYP2B6, CYP2C9, CYP2C19, CYP2D6, CYP2E1, and the CYP3A subfamily. After cocktail incubation in the presence of human liver microsomes (HLMs), the eight selected substrates and their specific metabolites were analyzed by ultra-high-pressure liquid chromatography and electrospray ionization quadrupole time-offlight mass spectrometry. Qualitative and quantitative data were simultaneously acquired to produce an overview of the extended phase I biotransformation routes for each probe substrate in the HLMs and to generate phenotypic profiles of various HLMs. A comparison of the cocktail strategy with an individual substrate assay for each CYP produced similar results. Moreover, the cocktail was tested on HLMs with different allelic variants and/or in the presence of selective inhibitors. The results were in agreement with the genetic polymorphisms of the CYPs and the expected effect of the alterations. All of these experiments confirmed the reliability of this cocktail assay for phenotyping of the microsomal CYPs.

Mots-clés
  • Cocktail approach
  • Ultra-high-pressure liquid
  • chromatography–quadrupole time-of-flight mass
  • spectrometry
  • Cytochrome P450 profile
  • Phenotyping
  • Genetic polymorphism
  • Human liver microsomes
Citation (format ISO)
SPAGGIARI, Dany et al. Phenotyping of CYP450 in human liver microsomes using the cocktail approach. In: Analytical & bioanalytical chemistry, 2014, vol. 406, p. 4875–4887. doi: 10.1007/s00216-014-7915-4
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Article (Published version)
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Identifiants
ISSN du journal1618-2642
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Création02/11/2016 15:17:00
Première validation02/11/2016 15:17:00
Heure de mise à jour15/03/2023 00:54:17
Changement de statut15/03/2023 00:54:17
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