Optimization of a method to quantify S-acylation
Ontology highlight
ABSTRACT: HeLa cells were lysed and free cysteines were alkylated with an alkyne-tagged light probe (IAA-BnL or IAA-PrL). S-acylation was hydrolysed with hydroxylamine and newly revealed Cys allowed to react with the heavy probe (IAA-BnL or IAA-PrL). Proteins were clicked with azido-biotin, Adadps-biotin, AazoB or ARB, enriched on neutravidin beads, digested with trypsin and desalted. Different optimisations of the protocol were tested: -8 sets of probes / capture reagent -LC-MS/MS optimisation (gradient, FAIMS, etc) Finally, S-acylation was quantified for a biological replicate of HeLa cells.
INSTRUMENT(S):
ORGANISM(S): Homo Sapiens (human)
TISSUE(S): Hela Cell
SUBMITTER:
EMMANUELLE THINON
LAB HEAD: Emmanuelle Thinon
PROVIDER: PXD063994 | Pride | 2026-06-29
REPOSITORIES: Pride
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