4.8 Article

Unbiased Detection of Cysteine Sulfenic Acid by 473 nm Photodissociation Mass Spectrometry: Toward Facile In Vivo Oxidative Status of Plasma Proteins

Journal

ANALYTICAL CHEMISTRY
Volume 93, Issue 5, Pages 2907-2915

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acs.analchem.0c04484

Keywords

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Funding

  1. French Agence National de la Recherche [ANR-18-CE29-0002-01]
  2. Agence Nationale de la Recherche (ANR) [ANR-18-CE29-0002] Funding Source: Agence Nationale de la Recherche (ANR)

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Cysteine in proteins is prone to oxidation, and a visible laser-induced dissociation technique was used in a mass spectrometer to streamline the detection of oxidized proteins. By derivatizing cysteine with a chromophore tag, high fragmentation yield was achieved for detecting oxidized peptides. This method has the potential for clinical applications in large human cohorts.
Cysteine (Cys) is prone to diverse post translational modifications in proteins, including oxidation into sulfenic acid (CysSOH) by reactive oxygen species generated under oxidative stress. Detection of low-concentration and metastable Cys-SOH within complex biological matrices is challenging due to the dynamic concentration range of proteins in the samples. Herein, visible laser-induced dissociation (LID) implemented in a mass spectrometer was used for streamlining the detection of Cys oxidized proteins owing to proper derivatization of Cys-SOH with a chromophore tag functionalized with a cyclohexanedione group. Once grafted, peptides undergo a high fragmentation yield under LID, leading concomitantly to informative backbone ions and to a chromophore reporter ion. Seventy-nine percent of the Cys-containing tryptic peptides and serotransferrin tracked by parallel reaction monitoring (PRM) were detected as targets subjected to oxidation. These candidates as well as Cys-containing peptides predicted by in silico trypsin digestion of five other human plasma proteins were then tracked in real plasma samples to pinpoint the endogenous Cys-SOH subpopulation. Most of the targeted peptides were detected in all plasma samples by LID-PRM, with significant differences in their relative amounts. By eliminating the signal of interfering co-eluted compounds, LID-PRM surpasses conventional HCD (higher-energy collisional dissociation)-PRM in detecting grafted Cys-SOH-containing peptides and allows now to foresee clinical applications in large human cohorts.

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