2013
DOI: 10.1021/pr4004213
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Targeted Quantitative Proteomics for the Analysis of 14 UGT1As and -2Bs in Human Liver Using NanoUPLC–MS/MS with Selected Reaction Monitoring

Abstract: Targeted quantitative proteomics using heavy isotope dilution techniques is increasingly being utilized to quantify proteins, including UGT enzymes, in biological matrices. Here we present a multiplexed method using nanoLC-MS/MS and multiple reaction monitoring (MRM) to quantify 14 UGT1As and UGT2Bs in liver matrices. Where feasible, we employ two or more proteotypic peptides per protein, with only four proteins quantified with only one proteotypic peptide. We apply the method to analysis of a library of 60 hu… Show more

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Cited by 111 publications
(165 citation statements)
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“…Followed by the selection of quantitative targeted peptides, the optimization of SRM, the selection of internal standards, and sample digestions, sample analysis can be conducted on a triple quadrupole mass spectrometer such as API 4000 or 6500 coupled to an LC, ultra performance LC (UPLC), or nano-UPLC system (22,23,37). The LC separation can be achieved in a reverse phase column (e.g., 100× 3.0 mm particle size 2.6 μm Kinetex® C18 column) with a gradient elution of water with 0.1% formic acid (solvent A) and acetonitrile with 0.1% formic acid (solvent B) as mobile phases.…”
Section: Lc-ms Methods Development Including Optimization and Validatimentioning
confidence: 99%
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“…Followed by the selection of quantitative targeted peptides, the optimization of SRM, the selection of internal standards, and sample digestions, sample analysis can be conducted on a triple quadrupole mass spectrometer such as API 4000 or 6500 coupled to an LC, ultra performance LC (UPLC), or nano-UPLC system (22,23,37). The LC separation can be achieved in a reverse phase column (e.g., 100× 3.0 mm particle size 2.6 μm Kinetex® C18 column) with a gradient elution of water with 0.1% formic acid (solvent A) and acetonitrile with 0.1% formic acid (solvent B) as mobile phases.…”
Section: Lc-ms Methods Development Including Optimization and Validatimentioning
confidence: 99%
“…To monitor multiple proteins in a single run, scheduled MRM acquisition method could be constructed using manually optimized declustering potentials, collision energies, as well as collision cell entrance and exit potentials. Three MRMs can be monitored simultaneously for each peptide (22,23). The quality control (QC) should also be conducted for the parameters of bioanalytical method validation guidelines suggested by regulatory agency for peptide stability, selectivity, linearity, reproducibility, and intra-/ interday variability (55).…”
Section: Lc-ms Methods Development Including Optimization and Validatimentioning
confidence: 99%
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“…All other reagents and solvents used were from standard suppliers and were of reagent or HPLC grade with all purities as defined by the manufacturer. Materials and chemicals used for the quantification of UGT abundances were as described previously (Fallon et al, 2013b;Achour et al, 2014a).…”
Section: Materials and Reagentsmentioning
confidence: 99%
“…Shi and coworkers applied the PRISM targeted proteomics to quantitate AGR2 in human urine at serum at concentrations of approximately 130 pg/ml and 10 pg per 100 ug of total protein mass in urine, respectively, and found in a proof‐of‐concept study of 37 urine samples that AGR2/PSA concentration ratios can distinguish noncancer and cancer 85. Fallon and coworkers developed assays for 14 UGT1As and UGT2Bs across 60 human liver microsomes and matching S9 samples to evaluate metabolism in drug development 86.…”
Section: Clinical Applicationsmentioning
confidence: 99%