Protein quantification by selective isolation and fragmentation of isotopic pairs using FT-ICR MS

Johnson, Hannah; Wong, Stephen C. C.; Simpson, Deborah M.; Beynon, Robert J.; Gaskell, Simon J.

doi:10.1016/j.jasms.2008.03.012

Cited by 10 publications

(4 citation statements)

References 13 publications

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“…To circumvent many of the complications posed by large‐scale AQUA‐based quantification studies, we developed the QconCAT approach for multiplexed absolute quantification 22–26. In brief, synthetic genes, optimised for heterologous expression in Escherichia coli , encode a single ORF that is a concatenation of tryptic peptides, each of which acts as an internal standard (a quantotypic or Qpeptide) for a different protein (of course it is equally feasible, or even desirable, to encode two or more peptides to report on each analyte protein).…”

Section: Multiplexed Quantification By Internal Standard: Qconcatmentioning

confidence: 99%

Global absolute quantification of a proteome: Challenges in the deployment of a QconCAT strategy

et al. 2011

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In this paper, we discuss the challenge of large-scale quantification of a proteome, referring to our programme that aims to define the absolute quantity, in copies per cell, of at least 4000 proteins in the yeast Saccharomyces cerevisiae. We have based our strategy on the well-established method of stable isotope dilution, generating isotopically labelled peptides using QconCAT technology, in which artificial genes, encoding concatenations of tryptic fragments as surrogate quantification standards, are designed, synthesised de novo and expressed in bacteria using stable isotopically enriched media. A known quantity of QconCAT is then co-digested with analyte proteins and the heavy:light isotopologues are analysed by mass spectrometry to yield absolute quantification. This workflow brings issues of optimal selection of quantotypic peptides, their assembly into QconCATs, expression, purification and deployment.

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Section: Multiplexed Quantification By Internal Standard: Qconcatmentioning

confidence: 99%

Global absolute quantification of a proteome: Challenges in the deployment of a QconCAT strategy

et al. 2011

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“…Other MS2-based quantitative proteomics approach have been described that use peptide-specific fragment ions for quantification (27, 28, 39). However, in these approaches an enlarged precursor isolation window ( e.g.…”

Section: Discussionmentioning

confidence: 99%

Index-ion Triggered MS2 Ion Quantification: A Novel Proteomics Approach for Reproducible Detection and Quantification of Targeted Proteins in Complex Mixtures

Yan

Luo

Robinson

et al. 2011

Molecular & Cellular Proteomics

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Biomedical research requires protein detection technology that is not only sensitive and quantitative, but that can reproducibly measure any set of proteins in a biological system in a high throughput manner. Here we report the development and application of a targeted proteomics platform termed index-ion triggered MS2 ion quantification (iMSTIQ) that allows reproducible and accurate peptide quantification in complex mixtures. The key feature of iMSTIQ is an approach called index-ion triggered analysis (ITA) that permits the reproducible acquisition of full MS2 spectra of targeted peptides independent of their ion intensities. Accurate quantification is achieved by comparing the relative intensities of multiple pairs of fragment ions derived from isobaric targeted peptides during MS2 analysis. Importantly, the method takes advantage of the favorable performance characteristics of the LTQ-Orbitrap, which include high mass accuracy, resolution, and throughput. As such it provides an attractive targeted proteomics tool to meet the demands of systems biology research and biomarker studies.

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“…Internal protein standards can also be obtained by metabolic labeling of organisms, such as E. coli (Hanke et al 2008). Additionally, a single synthesized concatemer protein comprised of peptides from 20 proteins of interest (QconCAT) has been generated to quantify a mixture of proteins (Pratt et al 2006;Johnson et al 2008;Rivers et al 2007;. Taken together, these studies show that the absolute quantitation of peptides and proteins using mass spectrometry is feasible (Brun et al 2009).…”

Section: Using Stable Isotopes To Achieve Absolute Quantitationmentioning

confidence: 99%

Strategies and Challenges in Measuring Protein Abundance Using Stable Isotope Labeling and Tandem Mass Spectrometry

Kristjansdottir¹,

Takahashi²,

Volchenboum³

et al. 2012

Tandem Mass Spectrometry - Applications and Principles

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Protein quantification by selective isolation and fragmentation of isotopic pairs using FT-ICR MS

Cited by 10 publications

References 13 publications

Global absolute quantification of a proteome: Challenges in the deployment of a QconCAT strategy

Global absolute quantification of a proteome: Challenges in the deployment of a QconCAT strategy

Index-ion Triggered MS2 Ion Quantification: A Novel Proteomics Approach for Reproducible Detection and Quantification of Targeted Proteins in Complex Mixtures

Strategies and Challenges in Measuring Protein Abundance Using Stable Isotope Labeling and Tandem Mass Spectrometry

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