Litcius/Paper detail

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

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

2021STAR Protocols10 citationsDOIOpen Access PDF

Abstract

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).

Topics & Concepts

PhosphorylationPrimary (astronomy)Protein phosphorylationChemistryWorkflowProtocol (science)ProteomicsComputational biologyCell biologyBiologyBiochemistryComputer scienceProtein kinase ADatabaseMedicineGeneAstronomyAlternative medicinePhysicsPathologyAdvanced Proteomics Techniques and ApplicationsMass Spectrometry Techniques and ApplicationsMetabolomics and Mass Spectrometry Studies