Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling

BACKGROUND: Quantitative measurements of specific protein phosphorylation sites, as presented here, can be used to investigate signal transduction pathways, which is an important aspect of cell dynamics. The presented method quantitatively compares peptide abundances from experiments using (18)O/(16...

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Autores principales: Andersen, Claus A, Gotta, Stefano, Magnoni, Letizia, Raggiaschi, Roberto, Kremer, Andreas, Terstappen, Georg C
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2009
Materias:
Methodology Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2693437/
https://www.ncbi.nlm.nih.gov/pubmed/19432989
http://dx.doi.org/10.1186/1471-2105-10-141
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author Andersen, Claus A
Gotta, Stefano
Magnoni, Letizia
Raggiaschi, Roberto
Kremer, Andreas
Terstappen, Georg C
author_facet Andersen, Claus A
Gotta, Stefano
Magnoni, Letizia
Raggiaschi, Roberto
Kremer, Andreas
Terstappen, Georg C
author_sort Andersen, Claus A
collection PubMed
description BACKGROUND: Quantitative measurements of specific protein phosphorylation sites, as presented here, can be used to investigate signal transduction pathways, which is an important aspect of cell dynamics. The presented method quantitatively compares peptide abundances from experiments using (18)O/(16)O labeling starting from elaborated MS spectra. It was originally developed to study signaling cascades activated by amyloid-β treatment of neurons used as a cellular model system with relevance to Alzheimer's disease, but is generally applicable. RESULTS: The presented method assesses, in complete cell lysates, the degree of phosphorylation of specific peptide residues from MS spectra using (18)O/(16)O labeling. The abundance of each observed phospho-peptide from two cell states was estimated from three overlapping isotope contours. The influence of peptide-specific labeling efficiency was removed by performing a label swapped experiment and assuming that the labeling efficiency was unchanged upon label swapping. Different degrees of phosphorylation were reported using the fold change measure which was extended with a confidence interval found to reflect the quality of the underlying spectra. Furthermore a new way of method assessment using simulated data is presented. Using simulated data generated in a manner mimicking real data it was possible to show the method's robustness both with increasing noise levels and with decreasing labeling efficiency. CONCLUSION: The fold change error assessable on simulated data was on average 0.16 (median 0.10) with an error-to-signal ratio and labeling efficiency distributions similar to the ones found in the experimentally observed spectra. Applied to experimentally observed spectra a very good match was found to the model (<10% error for 85% of spectra) with a high degree of robustness, as assessed by data removal. This new method can thus be used for quantitative signal cascade analysis of total cell extracts in a high throughput mode.
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spelling pubmed-26934372009-06-08 Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling Andersen, Claus A Gotta, Stefano Magnoni, Letizia Raggiaschi, Roberto Kremer, Andreas Terstappen, Georg C BMC Bioinformatics Methodology Article BACKGROUND: Quantitative measurements of specific protein phosphorylation sites, as presented here, can be used to investigate signal transduction pathways, which is an important aspect of cell dynamics. The presented method quantitatively compares peptide abundances from experiments using (18)O/(16)O labeling starting from elaborated MS spectra. It was originally developed to study signaling cascades activated by amyloid-β treatment of neurons used as a cellular model system with relevance to Alzheimer's disease, but is generally applicable. RESULTS: The presented method assesses, in complete cell lysates, the degree of phosphorylation of specific peptide residues from MS spectra using (18)O/(16)O labeling. The abundance of each observed phospho-peptide from two cell states was estimated from three overlapping isotope contours. The influence of peptide-specific labeling efficiency was removed by performing a label swapped experiment and assuming that the labeling efficiency was unchanged upon label swapping. Different degrees of phosphorylation were reported using the fold change measure which was extended with a confidence interval found to reflect the quality of the underlying spectra. Furthermore a new way of method assessment using simulated data is presented. Using simulated data generated in a manner mimicking real data it was possible to show the method's robustness both with increasing noise levels and with decreasing labeling efficiency. CONCLUSION: The fold change error assessable on simulated data was on average 0.16 (median 0.10) with an error-to-signal ratio and labeling efficiency distributions similar to the ones found in the experimentally observed spectra. Applied to experimentally observed spectra a very good match was found to the model (<10% error for 85% of spectra) with a high degree of robustness, as assessed by data removal. This new method can thus be used for quantitative signal cascade analysis of total cell extracts in a high throughput mode. BioMed Central 2009-05-11 /pmc/articles/PMC2693437/ /pubmed/19432989 http://dx.doi.org/10.1186/1471-2105-10-141 Text en Copyright © 2009 Andersen et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( (http://creativecommons.org/licenses/by/2.0) ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methodology Article
Andersen, Claus A
Gotta, Stefano
Magnoni, Letizia
Raggiaschi, Roberto
Kremer, Andreas
Terstappen, Georg C
Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling
title Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling
title_full Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling
title_fullStr Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling
title_full_unstemmed Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling
title_short Robust MS quantification method for phospho-peptides using (18)O/(16)O labeling
title_sort robust ms quantification method for phospho-peptides using (18)o/(16)o labeling
topic Methodology Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2693437/
https://www.ncbi.nlm.nih.gov/pubmed/19432989
http://dx.doi.org/10.1186/1471-2105-10-141
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