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  • Monitoring in vivo reversible cysteine oxidation in proteins using ICAT and mass spectrometry.

Monitoring in vivo reversible cysteine oxidation in proteins using ICAT and mass spectrometry.

Nature protocols (2014-04-20)
Sarela García-Santamarina, Susanna Boronat, Alba Domènech, José Ayté, Henrik Molina, Elena Hidalgo
摘要

Reversible thiol oxidation of cysteine residues occurs in many intracellular catalytic and signaling processes. Here we describe an optimized protocol, which can be completed in ∼5 d, to unambiguously identify specific cysteine residues that are transiently and reversibly oxidized by comparing two complex biological samples obtained from yeast cell cultures at the proteome level. After 'freezing' the in vivo thiol stage of cysteine residues by medium acidification, we first block reduced thiols in extracts with iodoacetamide (IAM), and then we sequentially reduce and label reversible oxidized thiols with the biotin-based heavy or light IAM derivatives, which are known as isotope-coded affinity tag (ICAT) reagents, so that the two samples can be compared at once after combination of the labeled extracts, trypsin digestion, streptavidin-affinity purification of peptides containing oxidized cysteines, and liquid chromatography-tandem mass spectrometry (LC-MS/MS) analysis. For the same protein extracts, before cysteine-containing peptide enrichment, individual relative protein concentrations are obtained by stable-isotope dimethyl labeling.

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Sigma-Aldrich
乙腈, HPLC Plus, ≥99.9%
Sigma-Aldrich
甲酸, ACS reagent, ≥96%
Sigma-Aldrich
乙二胺四乙酸 二钠盐 二水合物, suitable for electrophoresis, for molecular biology, 99.0-101.0% (titration)
Sigma-Aldrich
三乙基碳酸氢铵缓冲液, 1.0 M, pH 8.5±0.1