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In vivo metabolic investigation of cetilistat in normal versus pseudo-germ-free rats using UPLC-QTOFMS/MS and in silico toxicological evaluation of its metabolites.

Abstract
Cetilistat (CET) is a pancreatic lipase inhibitor approved for management of obesity after the serious adverse effects exhibited by its analogue orlistat. Exhaustive literature review reveals lack of comprehensive reports on its biotransformation. With a view to study the same, the present study reports the identification and characterization of metabolites of CET in rats using UPLC-MS/MS. As the small intestine is the site of action for CET, it is important that the role of microbial flora in the metabolism of CET be explored. To achieve this, the metabolic profile of CET was compared between normal and pseudo-germ-free rats. The study involved the administration of a drug suspension to male Sprague-Dawley pseudo-germ-free and normal untreated rats followed by collection of urine, feces, and blood at specific intervals. Sample preparation was performed using liquid-liquid extraction and concentration of samples followed by analysis using LC-MS/MS. Finally, an in silico study was performed on the drug and metabolites to predict their toxicological properties using ADMET PredictorTM software. Four metabolites of CET were observed in in vivo matrices. As expected, significant changes were observed both qualitatively and quantitatively, implying that formation of metabolites was both CYP enzymes and gut microflora mediated.
AuthorsShristy S Tiwari, Sumit Mukesh, Abhay T Sangamwar, M V N Kumar Talluri
JournalBiomedical chromatography : BMC (Biomed Chromatogr) Vol. 34 Issue 8 Pg. e4860 (Aug 2020) ISSN: 1099-0801 [Electronic] England
PMID32311767 (Publication Type: Journal Article)
Copyright© 2020 John Wiley & Sons, Ltd.
Chemical References
  • Benzoxazines
  • cetilistat
Topics
  • Animals
  • Benzoxazines (blood, chemistry, pharmacokinetics, toxicity)
  • Chromatography, High Pressure Liquid (methods)
  • Germ-Free Life
  • Male
  • Rats
  • Rats, Sprague-Dawley
  • Tandem Mass Spectrometry (methods)

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