Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay

Stable isotope-labeled standard (SIS) peptides are used as internal standards in targeted proteomics to provide robust protein quantification, which is required in clinical settings. However, SIS peptides are typically added post trypsin digestion and, as the digestion efficiency can vary significan...

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Autores principales: Hober, Andreas, Edfors, Fredrik, Ryaboshapkina, Maria, Malmqvist, Jonas, Rosengren, Louise, Percy, Andrew J., Lind, Lars, Forsström, Björn, Uhlén, Mathias, Oscarsson, Jan, Miliotis, Tasso
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The American Society for Biochemistry and Molecular Biology 2019
Materias:
Research
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6885709/
https://www.ncbi.nlm.nih.gov/pubmed/31591263
http://dx.doi.org/10.1074/mcp.RA119.001765
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author Hober, Andreas
Edfors, Fredrik
Ryaboshapkina, Maria
Malmqvist, Jonas
Rosengren, Louise
Percy, Andrew J.
Lind, Lars
Forsström, Björn
Uhlén, Mathias
Oscarsson, Jan
Miliotis, Tasso
author_facet Hober, Andreas
Edfors, Fredrik
Ryaboshapkina, Maria
Malmqvist, Jonas
Rosengren, Louise
Percy, Andrew J.
Lind, Lars
Forsström, Björn
Uhlén, Mathias
Oscarsson, Jan
Miliotis, Tasso
author_sort Hober, Andreas
collection PubMed
description Stable isotope-labeled standard (SIS) peptides are used as internal standards in targeted proteomics to provide robust protein quantification, which is required in clinical settings. However, SIS peptides are typically added post trypsin digestion and, as the digestion efficiency can vary significantly between peptides within a protein, the accuracy and precision of the assay may be compromised. These drawbacks can be remedied by a new class of internal standards introduced by the Human Protein Atlas project, which are based on SIS recombinant protein fragments called SIS PrESTs. SIS PrESTs are added initially to the sample and SIS peptides are released on trypsin digestion. The SIS PrEST technology is promising for absolute quantification of protein biomarkers but has not previously been evaluated in a clinical setting. An automated and scalable solid phase extraction workflow for desalting and enrichment of plasma digests was established enabling simultaneous preparation of up to 96 samples. Robust high-precision quantification of 13 apolipoproteins was achieved using a novel multiplex SIS PrEST-based LC-SRM/MS Tier 2 assay in non-depleted human plasma. The assay exhibited inter-day coefficients of variation between 1.5% and 14.5% (median = 3.5%) and was subsequently used to investigate the effects of omega-3 carboxylic acids (OM3-CA) and fenofibrate on these 13 apolipoproteins in human plasma samples from a randomized placebo-controlled trial, EFFECT I (NCT02354976). No significant changes were observed in the OM3-CA arm, whereas treatment with fenofibrate significantly increased apoAII and reduced apoB, apoCI, apoE and apoCIV levels. The reduction in apoCIV following fenofibrate treatment is a novel finding. The study demonstrates that SIS PrESTs can facilitate the generation of robust multiplexed biomarker Tier 2 assays for absolute quantification of proteins in clinical studies.
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spelling pubmed-68857092019-12-03 Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay Hober, Andreas Edfors, Fredrik Ryaboshapkina, Maria Malmqvist, Jonas Rosengren, Louise Percy, Andrew J. Lind, Lars Forsström, Björn Uhlén, Mathias Oscarsson, Jan Miliotis, Tasso Mol Cell Proteomics Research Stable isotope-labeled standard (SIS) peptides are used as internal standards in targeted proteomics to provide robust protein quantification, which is required in clinical settings. However, SIS peptides are typically added post trypsin digestion and, as the digestion efficiency can vary significantly between peptides within a protein, the accuracy and precision of the assay may be compromised. These drawbacks can be remedied by a new class of internal standards introduced by the Human Protein Atlas project, which are based on SIS recombinant protein fragments called SIS PrESTs. SIS PrESTs are added initially to the sample and SIS peptides are released on trypsin digestion. The SIS PrEST technology is promising for absolute quantification of protein biomarkers but has not previously been evaluated in a clinical setting. An automated and scalable solid phase extraction workflow for desalting and enrichment of plasma digests was established enabling simultaneous preparation of up to 96 samples. Robust high-precision quantification of 13 apolipoproteins was achieved using a novel multiplex SIS PrEST-based LC-SRM/MS Tier 2 assay in non-depleted human plasma. The assay exhibited inter-day coefficients of variation between 1.5% and 14.5% (median = 3.5%) and was subsequently used to investigate the effects of omega-3 carboxylic acids (OM3-CA) and fenofibrate on these 13 apolipoproteins in human plasma samples from a randomized placebo-controlled trial, EFFECT I (NCT02354976). No significant changes were observed in the OM3-CA arm, whereas treatment with fenofibrate significantly increased apoAII and reduced apoB, apoCI, apoE and apoCIV levels. The reduction in apoCIV following fenofibrate treatment is a novel finding. The study demonstrates that SIS PrESTs can facilitate the generation of robust multiplexed biomarker Tier 2 assays for absolute quantification of proteins in clinical studies. The American Society for Biochemistry and Molecular Biology 2019-12 2019-10-07 /pmc/articles/PMC6885709/ /pubmed/31591263 http://dx.doi.org/10.1074/mcp.RA119.001765 Text en © 2019 Hober et al. Published by The American Society for Biochemistry and Molecular Biology, Inc. https://creativecommons.org/licenses/by/4.0/Author's Choice—Final version open access under the terms of the Creative Commons CC-BY license (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Research
Hober, Andreas
Edfors, Fredrik
Ryaboshapkina, Maria
Malmqvist, Jonas
Rosengren, Louise
Percy, Andrew J.
Lind, Lars
Forsström, Björn
Uhlén, Mathias
Oscarsson, Jan
Miliotis, Tasso
Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay
title Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay
title_full Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay
title_fullStr Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay
title_full_unstemmed Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay
title_short Absolute Quantification of Apolipoproteins Following Treatment with Omega-3 Carboxylic Acids and Fenofibrate Using a High Precision Stable Isotope-labeled Recombinant Protein Fragments Based SRM Assay
title_sort absolute quantification of apolipoproteins following treatment with omega-3 carboxylic acids and fenofibrate using a high precision stable isotope-labeled recombinant protein fragments based srm assay
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6885709/
https://www.ncbi.nlm.nih.gov/pubmed/31591263
http://dx.doi.org/10.1074/mcp.RA119.001765
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