A simple isotopic labeling method to study cysteine oxidation in Alzheimer’s disease: oxidized cysteine-selective dimethylation (OxcysDML)

A simple isotopic labeling method to study cysteine oxidation in Alzheimer’s disease: oxidized cysteine-selective dimethylation (OxcysDML)

Cysteine is widely involved in redox signaling pathways through a number of reversible and irreversible modifications. Reversible modifications (e.g., S-glutathionylation, S-nitrosylation, disulfide bonds, and sulfenic acid) are used to protect proteins from oxidative attack and maintain cellular ho...

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Veröffentlicht in:Analytical and bioanalytical chemistry 2016-04, Vol.408 (11), p.2993-3004
Hauptverfasser: Gu, Liqing, Robinson, Renã A. S.
Format: Artikel
Sprache:eng
Schlagworte:
Alzheimer Disease - metabolism
Alzheimer's disease
Amino acids
Analytical Chemistry
Animals
Biochemistry
Characterization and Evaluation of Materials
Chemical bonds
Chemistry
Chemistry and Materials Science
Chromatography, Liquid
Cysteine
Cysteine - chemistry
Enrichment
Food Science
Health aspects
Homeostasis
Humans
Isotope analysis
Isotope Labeling
Isotopic labeling
Labeling
Laboratory Medicine
Methods
Methylation
Mice
Mice, Transgenic
Monitoring/Environmental Analysis
Observations
Oxidation
Oxidation-Reduction
Oxidation-reduction reactions
Oxidative stress
Peptides
Physiological aspects
Proteins
Proteomics
Reagents
Research Paper
Tandem Mass Spectrometry
Young Investigators in Analytical and Bioanalytical Science
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Zusammenfassung:Cysteine is widely involved in redox signaling pathways through a number of reversible and irreversible modifications. Reversible modifications (e.g., S-glutathionylation, S-nitrosylation, disulfide bonds, and sulfenic acid) are used to protect proteins from oxidative attack and maintain cellular homeostasis, while irreversible oxidations (e.g., sulfinic acid and sulfonic acid) serve as hallmarks of oxidative stress. Proteomic analysis of cysteine-enriched peptides coupled with reduction of oxidized thiols can be used to measure the oxidation states of cysteine, which is helpful for elucidating the role that oxidative stress plays in biology and disease. As an extension of our previously reported cysDML method, we have developed oxidized cysteine-selective dimethylation (OxcysDML), to investigate the site-specific total oxidation of cysteine residues in biologically relevant samples. OxcysDML employs (1) blocking of free thiols by a cysteine-reactive reagent, (2) enrichment of peptides containing reversibly oxidized cysteine by a solid phase resin, and (3) isotopic labeling of peptide amino groups to quantify cysteine modifications arising from different biological conditions. On-resin enrichment and labeling minimizes sample handing time and improves efficiency in comparison with other redox proteomic methods. OxcysDML is also inexpensive and flexible, as it can accommodate the exploration of various cysteine modifications. Here, we applied the method to liver tissues from a late-stage Alzheimer’s disease (AD) mouse model and wild-type (WT) controls. Because we have previously characterized this proteome using the cysDML approach, we are able here to probe deeper into the redox status of cysteine in AD. OxcysDML identified 1129 cysteine sites (from 527 proteins), among which 828 cysteine sites underwent oxidative modifications. Nineteen oxidized cysteine sites had significant alteration levels in AD and represent proteins involved in metabolic processes. Overall, we have demonstrated OxcysDML as a simple, rapid, robust, and inexpensive redox proteomic approach that is useful for gaining deeper insight into the proteome of AD. Graphical abstract OxcysDML enables the proteome comparision of cysteine reversible oxidations from two biological conditions
ISSN:1618-2642
1618-2650
DOI:10.1007/s00216-016-9307-4