Literature DB >> 16479536

Relative and absolute quantitative expression profiling of cytochromes P450 using isotope-coded affinity tags.

Rosalind E Jenkins1, Neil R Kitteringham, Christie L Hunter, Sally Webb, Tony J Hunt, Robert Elsby, Rod B Watson, Dominic Williams, Stephen R Pennington, B Kevin Park.   

Abstract

The development of a novel method for absolute quantification of proteins based on isotope-coded affinity tagging using ICAT reagents is described. The method exploits synthetic peptide standards to determine protein content at the femtomole level in biological samples. The approach is generally applicable to any subset of proteins, but is particularly appropriate for quantitative analysis of multiple, closely related isoforms, and for hydrophobic proteins that are poorly represented in 2-D gels. Relative and absolute quantification techniques are applied to an important group of microsomal metabolic enzymes, the cytochromes P450 (P450), which are critical in determining the disposition, safety and efficacy of drugs in man. Measurement of the P450 induction profile in response to chemicals is a fundamental aspect of drug safety evaluation and is currently achieved by low-throughput methods employing poorly discriminatory antibodies or substrates. Tagging technology is shown to supersede conventional methods for P450 profiling in terms of discriminatory power and throughput, exemplified by the simultaneous detection of distinct induction profiles for cyp2c subfamily members in response to phenobarbitone: cyp2c29 expression, but not cyp2c40 or cyp2c50, was induced threefold by treatment. This technology should abbreviate the drug development pathway, and provide a widely applicable, rapid means of quantifying proteins.

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Year:  2006        PMID: 16479536     DOI: 10.1002/pmic.200500432

Source DB:  PubMed          Journal:  Proteomics        ISSN: 1615-9853            Impact factor:   3.984


  11 in total

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Authors:  Ben C Collins; Christine A Miller; Alexandra Sposny; Phillip Hewitt; Martin Wells; William M Gallagher; Stephen R Pennington
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5.  Multiple-approaches to the identification and quantification of cytochromes P450 in human liver tissue by mass spectrometry.

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Review 6.  Targeted proteomics for biomarker discovery and validation of hepatocellular carcinoma in hepatitis C infected patients.

Authors:  Gul M Mustafa; Denner Larry; John R Petersen; Cornelis J Elferink
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7.  Quantitation of human cytochrome P450 2D6 protein with immunoblot and mass spectrometry analysis.

Authors:  Ai-Ming Yu; Jun Qu; Melanie A Felmlee; Jin Cao; Xi-Ling Jiang
Journal:  Drug Metab Dispos       Date:  2008-10-02       Impact factor: 3.922

Review 8.  Thematic Review Series: Proteomics. An integrated omics analysis of eicosanoid biology.

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Journal:  J Lipid Res       Date:  2009-02-24       Impact factor: 5.922

9.  Downregulation of mouse hepatic CYP3A protein by 3-methylcholanthrene does not require cytochrome P450-dependent metabolism.

Authors:  Chunja Lee; Xinxin Ding; David S Riddick
Journal:  Drug Metab Dispos       Date:  2013-07-11       Impact factor: 3.922

10.  Comparative cytochrome P450 proteomics in the livers of immunodeficient mice using 18O stable isotope labeling.

Authors:  Catherine S Lane; Yuqin Wang; Richard Betts; William J Griffiths; Laurence H Patterson
Journal:  Mol Cell Proteomics       Date:  2007-02-11       Impact factor: 5.911

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