Targeted Precise Quantification of 12 Human Recombinant Uridine-Diphosphate Glucuronosyl Transferase 1A and 2B Isoforms Using Nano-Ultra-High-Performance Liquid Chromatography/Tandem Mass Spectrometry with Selected Reaction Monitoring

Fallon, John K.; Neubert, Hendrik; Goosen, Theunis C.; Smith, Philip C.

doi:10.1124/dmd.113.053801

Cited by 65 publications

(63 citation statements)

References 13 publications

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“…Expression and activity data suggest that UGT1A9 and UGT2B7 are the major UGT enzymes in human kidney, with UGT1A9 expressed at levels close to or higher than those measured in liver (91). These findings are in agreement with the majority of quantitative abundance data from commercially available pooled human kidney microsomes, acquired using targeted LC-MS/MS proteomic methods (14,92). Large variability in both mRNA (72-85% CV, n = 11) and protein abundance (76-159% CV, n = 10) has been noted for UGT1A6, 1A9 and 2B7 in kidney homogenates prepared from unspecified regions of healthy kidney (93).…”

Section: Amount Of Specific Drug Metabolising Enzymes In Kidneysupporting

confidence: 78%

“…High variability in abundance, not only between enzymes but also between batches for the same enzyme, has been reported for recombinantly expressed UGTs (e.g. 30.6% coefficient of variation for rUGT1A4), which may hinder IVIVE-based prediction of both hepatic and renal glucuronidation clearance (14). In addition, UGTs expressed in insect cells may have a substantial amount of inactive protein present that can be reduced by lowering the amount of baculovirus used to infect cells (21).…”

Section: Use Of In Vitro Systems To Understand Renal Drug Eliminationmentioning

confidence: 99%

“…It is evident from Table I that human kidney subcellular fractions (microsomes, S9) and recombinant enzyme expression systems are the most commonly applied sources of kidney drug-metabolising enzymes in in vitro assays (7,(14)(15)(16). Subcellular fractions require supplementation with appropriate cofactors lost during the preparation procedure and these are highlighted in Table I.…”

Section: Use Of In Vitro Systems To Understand Renal Drug Eliminationmentioning

confidence: 99%

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Key to Opening Kidney for In Vitro–In Vivo Extrapolation Entrance in Health and Disease: Part I: In Vitro Systems and Physiological Data

Scotcher

Jones²,

Posada

et al. 2016

AAPS J

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ABSTRACT.The programme for the 2015 AAPS Annual Meeting and Exhibition (Orlando, FL; 25-29 October 2015) included a sunrise session presenting an overview of the state-of-the-art tools for in vitro-in vivo extrapolation (IVIVE) and mechanistic prediction of renal drug disposition. These concepts are based on approaches developed for prediction of hepatic clearance, with consideration of scaling factors physiologically relevant to kidney and the unique and complex structural organisation of this organ. Physiologically relevant kidney models require a number of parameters for mechanistic description of processes, supported by quantitative information on renal physiology (system parameters) and in vitro/in silico drug-related data. This review expands upon the themes raised during the session and highlights the importance of high quality in vitro drug data generated in appropriate experimental setup and robust system-related information for successful IVIVE of renal drug disposition. The different in vitro systems available for studying renal drug metabolism and transport are summarised and recent developments involving state-of-the-art technologies highlighted. Current gaps and uncertainties associated with system parameters related to human kidney for the development of physiologically based pharmacokinetic (PBPK) model and quantitative prediction of renal drug disposition, excretion, and/or metabolism are identified.

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Section: Amount Of Specific Drug Metabolising Enzymes In Kidneysupporting

confidence: 78%

Section: Use Of In Vitro Systems To Understand Renal Drug Eliminationmentioning

confidence: 99%

Section: Use Of In Vitro Systems To Understand Renal Drug Eliminationmentioning

confidence: 99%

See 1 more Smart Citation

Key to Opening Kidney for In Vitro–In Vivo Extrapolation Entrance in Health and Disease: Part I: In Vitro Systems and Physiological Data

Scotcher

Jones²,

Posada

et al. 2016

AAPS J

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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%

Quantitative Characterization of Major Hepatic UDP-Glucuronosyltransferase Enzymes in Human Liver Microsomes: Comparison of Two Proteomic Methods and Correlation with Catalytic Activity

et al. 2017

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Quantitative characterization of UDP-glucuronosyltransferase (UGT) enzymes is valuable in glucuronidation reaction phenotyping, predicting metabolic clearance and drug-drug interactions using extrapolation exercises based on pharmacokinetic modeling. Different quantitative proteomic workflows have been employed to quantify UGT enzymes in various systems, with reports indicating large variability in expression, which cannot be explained by interindividual variability alone. To evaluate the effect of methodological differences on end-point UGT abundance quantification, eight UGT enzymes were quantified in 24 matched liver microsomal samples by two laboratories using stable isotope-labeled (SIL) peptides or quantitative concatemer (QconCAT) standard, and measurements were assessed against catalytic activity in seven enzymes (n = 59). There was little agreement between individual abundance levels reported by the two methods; only UGT1A1 showed strong correlation [Spearman rank order correlation (Rs) = 0.73, P < 0.0001; R 2 = 0.30; n = 24]. SIL-based abundance measurements correlated well with enzyme activities, with correlations ranging from moderate for UGTs 1A6, 1A9, and 2B15 (Rs = 0.52-0.59, P < 0.0001; R 2 = 0.34-0.58; n = 59) to strong correlations for UGTs 1A1, 1A3, 1A4, and 2B7 (Rs = 0.79-0.90, P < 0.0001; R 2 = 0.69-0.79). QconCAT-based data revealed generally poor correlation with activity, whereas moderate correlations were shown for UGTs 1A1, 1A3, and 2B7. Spurious abundance-activity correlations were identified in the cases of UGT1A4/2B4 and UGT2B7/2B15, which could be explained by correlations of protein expression between these enzymes. Consistent correlation of UGT abundance with catalytic activity, demonstrated by the SIL-based dataset, suggests that quantitative proteomic data should be validated against catalytic activity whenever possible. In addition, metabolic reaction phenotyping exercises should consider spurious abundance-activity correlations to avoid misleading conclusions.

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“…Enzyme abundances were found to be between 7-and 11-fold and 19-and 43-fold higher in recombinant expression systems than in human kidney microsomes for uridine diphosphate glucuronosyltransferase (UGT) 1A9 and UGT2B7, respectively (17,27,28). These data suggest that for calculation of the appropriate REF values for IVIVE, enzyme abundance data should be collected for every batch of recombinantly expressed UGT.…”

Section: Prediction Of Renal Drug Metabolism Within Pbpk Paradigmmentioning

confidence: 99%

Key to Opening Kidney for In Vitro-In Vivo Extrapolation Entrance in Health and Disease: Part II: Mechanistic Models and In Vitro-In Vivo Extrapolation

Scotcher

Jones²,

Posada

et al. 2016

AAPS J

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Abstract.It is envisaged that application of mechanistic models will improve prediction of changes in renal disposition due to drug-drug interactions, genetic polymorphism in enzymes and transporters and/or renal impairment. However, developing and validating mechanistic kidney models is challenging due to the number of processes that may occur (filtration, secretion, reabsorption and metabolism) in this complex organ. Prediction of human renal drug disposition from preclinical species may be hampered by species differences in the expression and activity of drug metabolising enzymes and transporters. A proposed solution is bottom-up prediction of pharmacokinetic parameters based on in vitro-in vivo extrapolation (IVIVE), mediated by recent advances in in vitro experimental techniques and application of relevant scaling factors. This review is a follow-up to the Part I of the report from the 2015 AAPS Annual Meeting and Exhibition (Orlando, FL; 25th-29th October 2015) which focuses on IVIVE and mechanistic prediction of renal drug disposition. It describes the various mechanistic kidney models that may be used to investigate renal drug disposition. Particular attention is given to efforts that have attempted to incorporate elements of IVIVE. In addition, the use of mechanistic models in prediction of renal drugdrug interactions and potential for application in determining suitable adjustment of dose in kidney disease are discussed. The need for suitable clinical pharmacokinetics data for the purposes of delineating mechanistic aspects of kidney models in various scenarios is highlighted.KEY WORDS: active renal excretion; human kidney transporters; human renal drug clearance; kidney disease; non-hepatic drug metabolism.

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Targeted Precise Quantification of 12 Human Recombinant Uridine-Diphosphate Glucuronosyl Transferase 1A and 2B Isoforms Using Nano-Ultra-High-Performance Liquid Chromatography/Tandem Mass Spectrometry with Selected Reaction Monitoring

Cited by 65 publications

References 13 publications

Key to Opening Kidney for In Vitro–In Vivo Extrapolation Entrance in Health and Disease: Part I: In Vitro Systems and Physiological Data

Key to Opening Kidney for In Vitro–In Vivo Extrapolation Entrance in Health and Disease: Part I: In Vitro Systems and Physiological Data

Quantitative Characterization of Major Hepatic UDP-Glucuronosyltransferase Enzymes in Human Liver Microsomes: Comparison of Two Proteomic Methods and Correlation with Catalytic Activity

Key to Opening Kidney for In Vitro-In Vivo Extrapolation Entrance in Health and Disease: Part II: Mechanistic Models and In Vitro-In Vivo Extrapolation

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