Cysteine tagging for MS‐based proteomics

Giron, Priscille; Dayon, Loı̈c; Sanchez, Jean‐Charles

doi:10.1002/mas.20285

Cited by 66 publications

(67 citation statements)

References 284 publications

(269 reference statements)

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“…For effective analysis of SNO and SOH selective labelling and enrichment are required [13]. A number of methods for analysis of cysteine oxidation exist, each with certain advantages and limitations, as reviewed in [2].…”

Section: Introductionmentioning

confidence: 99%

The SNO/SOH TMT strategy for combinatorial analysis of reversible cysteine oxidations

Wojdyła

Williamson

Roepstorff

et al. 2015

Journal of Proteomics

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SNO/SOH TMT strategy outperforms other available strategies for cysteine oxidation analysis. It provides quantitative profiling of S-nitrosylation and S-sulfenylation changes simultaneously in two experimental conditions. It allows correction of modification levels by protein abundance changes and determination of relative modification site occupancy - all in a single nLC-MSMS experiment based on commercially available reagents. The method has proven precise and sensitive enough to detect and quantify endogenous levels of oxidative stress on proteome-wide scale.

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Section: Introductionmentioning

confidence: 99%

The SNO/SOH TMT strategy for combinatorial analysis of reversible cysteine oxidations

Wojdyła

Williamson

Roepstorff

et al. 2015

Journal of Proteomics

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“…Numerous techniques have been developed because of the increasing interest and evidences of redox-regulated signaling networks (8,9). For a long time, the determination of the redox-regulated functional role of specific Cys sites has been performed using site-directed mutagenesis (10).…”

mentioning

confidence: 99%

A Novel Strategy for Global Analysis of the Dynamic Thiol Redox Proteome

Martínez-Acedo

Núñez

Gómez

et al. 2012

Molecular & Cellular Proteomics

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Nitroxidative stress in cells occurs mainly through the action of reactive nitrogen and oxygen species (RNOS) on protein thiol groups. Reactive nitrogen and oxygen species-mediated protein modifications are associated with pathophysiological states, but can also convey physiological signals. Identification of Cys residues that are modified by oxidative stimuli still poses technical challenges and these changes have never been statistically analyzed from a proteome-wide perspective. Here we show that GELSILOX, a method that combines a robust proteomics protocol with a new computational approach that analyzes variance at the peptide level, allows a simultaneous analysis of dynamic alterations in the redox state of Cys sites and of protein abundance. GELSILOX permits the characterization of the major endothelial redox targets of hydrogen peroxide in endothelial cells and reveals that hypoxia induces a significant increase in the status of oxidized thiols. GELSILOX also detected thiols that are redox-modified by ischemia-reperfusion in heart mitochondria and demonstrated that these alterations are abolished in ischemia-preconditioned animals.

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“…22 Specific photodissociation was also obtained for Tyr/His-containing peptides after derivatization with diazonium chromophore groups. 23 Detection specificity is also critical when tackling protein quantification in whole proteome by targeted mass spectrometry in selected reaction monitoring mode (SRM 25 Thus, photo-SRM showed similar or even improved detection performance compared to conventional CID-SRM for the analysis of a whole plasma hydrolysate.…”

Section: Collision-induced Dissociation (Cid) Remains the Widespread mentioning

confidence: 99%

Implementing visible 473 nm photodissociation in a Q-Exactive mass spectrometer: towards specific detection of cysteine-containing peptides

Girod

Biarc

Enjalbert

et al. 2014

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Cysteine tagging for MS‐based proteomics

Cited by 66 publications

References 284 publications

The SNO/SOH TMT strategy for combinatorial analysis of reversible cysteine oxidations

The SNO/SOH TMT strategy for combinatorial analysis of reversible cysteine oxidations

A Novel Strategy for Global Analysis of the Dynamic Thiol Redox Proteome

Implementing visible 473 nm photodissociation in a Q-Exactive mass spectrometer: towards specific detection of cysteine-containing peptides

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