Quantifying phosphorylation dynamics in primary neuronal cultures using LC-MS/MS

Kristina Desch; Erin M. Schuman; Julian D. Langer

STAR Protocols (Mar 2022)

Quantifying phosphorylation dynamics in primary neuronal cultures using LC-MS/MS

Kristina Desch,
Erin M. Schuman,
Julian D. Langer

Affiliations

Kristina Desch: Max Planck Institute for Brain Research, Max von Laue Strasse 4, 60438 Frankfurt, Germany
Erin M. Schuman: Max Planck Institute for Brain Research, Max von Laue Strasse 4, 60438 Frankfurt, Germany; Corresponding author
Julian D. Langer: Max Planck Institute for Brain Research, Max von Laue Strasse 4, 60438 Frankfurt, Germany; Max Planck Institute of Biophysics, Max von Laue Strasse 3, 60438 Frankfurt, Germany; Corresponding author

Journal volume & issue: Vol. 3, no. 1
p. 101063

Abstract

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Summary: Cellular processes require tight and coordinated control of protein abundance, localization, and activity. One of the core mechanisms to achieve specific regulation of proteins is protein phosphorylation. Here we present a workflow to monitor protein abundance and phosphorylation in primary cultured neurons using liquid chromatography-coupled mass spectrometry. Our protocol provides a detailed guide on all steps for detection and label-free-quantification of phosphorylated and unmodified proteins of primary cortical neurons, including primary cell culture, phosphoproteomic sample preparation and data-processing, and evaluation.For complete details on the use and execution of this protocol, please refer to Desch et al. (2021).

Published in STAR Protocols

ISSN: 2666-1667 (Online)
Publisher: Elsevier
Country of publisher: United States
LCC subjects: Science: Science (General)
Website: https://star-protocols.cell.com/

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