Metabolic labeling and LC-MS/MS-based identification of interleukin-1α-induced secreted proteomes from epithelial cells in the presence or absence of serum

Jasmin Priester; Johanna Meier-Soelch; Hendrik Weiser; Daniel Heylmann; Axel Weber; Uwe Linne; Michael Kracht

doi:10.1016/j.xpro.2023.102195

Metabolic labeling and LC-MS/MS-based identification of interleukin-1α-induced secreted proteomes from epithelial cells in the presence or absence of serum

STAR Protoc. 2023 Mar 31;4(2):102195. doi: 10.1016/j.xpro.2023.102195. Online ahead of print.

Authors

Jasmin Priester¹, Johanna Meier-Soelch¹, Hendrik Weiser¹, Daniel Heylmann¹, Axel Weber¹, Uwe Linne², Michael Kracht³

Affiliations

¹ Rudolf Buchheim Institute of Pharmacology, Justus Liebig University, 35392 Giessen, Germany.
² Mass Spectrometry Facility of the Department of Chemistry, Philipps University, 35032 Marburg, Germany. Electronic address: [email protected].
³ Rudolf Buchheim Institute of Pharmacology, Justus Liebig University, 35392 Giessen, Germany; Universities of Giessen and Marburg Lung Center (UGMLC), Giessen, Germany; Cardio-Pulmonary Institute (CPI), Giessen, Germany. Electronic address: [email protected].

Abstract

The unbiased identification of cytokine-induced, secreted proteins from cells cultured in serum-containing medium is challenging. Here, we describe an experimental and bioinformatics workflow to label interleukin-1α-regulated proteins in living cells with the methionine analogue L-homopropargylglycine. We detail their purification and identification by means of CLICK-chemistry-based biotinylation followed by nanoHPLC-MS/MS. A side-by-side comparison of enriched proteins and their ontologies to serum-free conditions demonstrates the sensitivity and specificity of this approach to study the inducible secreted proteomes of epithelial cells.

Keywords: Cell Biology; Cell Culture; Flow Cytometry/Mass Cytometry; Immunology; Molecular/Chemical Probes; Protein Biochemistry; Protein Expression and Purification; Proteomics.