2008
DOI: 10.2174/187231208785425764
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Absolute Quantification of Human Uridine-Diphosphate Glucuronosyl Transferase (UGT) Enzyme Isoforms 1A1 and 1A6 By Tandem LC-MS

Abstract: UGT enzymes catalyze the formation of glucuronic acid conjugates. Specifically selected representative stable isotope (C(13), N(15)) labeled peptide internal standards of each enzyme were employed to quantify UGTs 1A1 and 1A6 by LC-MS/MS using isotope dilution techniques. Inter day variability (n=5) for human liver microsomes was Show more

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Cited by 42 publications
(71 citation statements)
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“…In-solution sample preparation was performed as reported previously (Fallon et al, 2008(Fallon et al, , 2013a. Briefly, sample protein content was assessed using bicinchoninic acid assay and samples (n = 60) were diluted 1:20 in 50 mM ammonium bicarbonate.…”
Section: Quantification Of Ugt Enzymes Using Stable Isotope-labeled Pmentioning
confidence: 99%
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“…In-solution sample preparation was performed as reported previously (Fallon et al, 2008(Fallon et al, , 2013a. Briefly, sample protein content was assessed using bicinchoninic acid assay and samples (n = 60) were diluted 1:20 in 50 mM ammonium bicarbonate.…”
Section: Quantification Of Ugt Enzymes Using Stable Isotope-labeled Pmentioning
confidence: 99%
“…Selection of proteotypic peptides was carried out as previously reported (Fallon et al, 2008(Fallon et al, , 2013aKamiie et al, 2008). The peptides were tryptic, as well as proteotypic, and contained no linkers or added moieties, such that they could be used directly as standards for quantification.…”
Section: Quantification Of Ugt Enzymes Using Stable Isotope-labeled Pmentioning
confidence: 99%
See 2 more Smart Citations
“…Targeted isotope dilution techniques with tandem mass spectrometry have recently been used to quantify a wide range of bioactive proteins including UGTs, cytochrome P450s, and transporters (Li et al, 2009;Harbourt et al, 2012;Ohtsuki et al, 2012;Picotti et al, 2013). The specificity and broad dynamic range of the methods are advantageous when compared with often semiquantitative, nonspecific, and expensive traditional immunometric methods (Seppen et al, 1994;Ritter et al, 1999;Paine and Fisher, 2000;Fallon et al, 2008). In this study we present application of a previously described capillary liquid chromatography-tandem mass spectrometry isotope dilution method (Fallon et al, 2013) for the targeted quantification of up to 14 UGT isoforms to a series of commercially produced recUGT samples (BD Supersomes [baculovirus-infected insect-cell microsomes]) (12 isoforms; n = 49 samples).…”
mentioning
confidence: 99%