A targeted ultra performance liquid chromatography – Tandem mass spectrometric assay for tyrosine and metabolites in urine and plasma: Application to the effects of antibiotics on mice

•A rapid microbore RP-UHPLC-MS assay for tyrosine and 11 metabolites is described.•A “fit-for-purpose” approach was applied to method validation.•The assay was applied to mouse urine and plasma after feeding a high tyrosine diet.•Antibiotics revealed the contribution of the gut microbiota to tyrosin...

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Veröffentlicht in:Journal of chromatography. B, Analytical technologies in the biomedical and life sciences Analytical technologies in the biomedical and life sciences, 2021-02, Vol.1164, p.122511-122511, Article 122511
Hauptverfasser: Letertre, Marine P.M., Myridakis, Antonis, Whiley, Luke, Camuzeaux, Stéphane, Lewis, Matthew R., Chappell, Katie E., Thaikkatil, Annie, Dumas, Marc-Emmanuel, Nicholson, Jeremy K., Swann, Jonathan R., Wilson, Ian D.
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Sprache:eng
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Zusammenfassung:•A rapid microbore RP-UHPLC-MS assay for tyrosine and 11 metabolites is described.•A “fit-for-purpose” approach was applied to method validation.•The assay was applied to mouse urine and plasma after feeding a high tyrosine diet.•Antibiotics revealed the contribution of the gut microbiota to tyrosine metabolism. Tyrosine plays a key role in mammalian biochemistry and defects in its metabolism (e.g., tyrosinemia, alkaptonuria etc.) have significant adverse consequences for those affected if left untreated. In addition, gut bacterially-derived p-cresol and its metabolites are of interest as a result of various effects on host xenobiotic metabolism. A fit-for-purpose quantitative ultra-performance liquid chromatography tandem mass spectrometry (UPLC-MS/MS) assay was developed to target and quantify tyrosine and eleven metabolites in urine and plasma. Dansylation, using dansyl chloride, was used to improve chromatographic and mass spectral properties for tyrosine and nine phenolic metabolites, with detection using positive electrospray ionisation (ESI). The sulfate and glucuronide conjugates of p-cresol, where the phenol group was blocked, were quantified intact, using negative ESI via polarity switching during the same run. Sample preparation for urine and plasma involved deproteinization by solvent precipitation (of acetonitrile:isopropyl alcohol (1:1 v/v)) followed by in situ dansylation in 96 well plates. To minimize sample and solvent usage, and maximize sensitivity, analysis was performed using microbore reversed-phase gradient UPLC on a C8 phase with a 7.5 min. cycle time. The coefficients of variation obtained were
ISSN:1570-0232
1873-376X
DOI:10.1016/j.jchromb.2020.122511