Protocol to Assess Substrate Dephosphorylation by Serine/threonine Phosphoprotein Phosphatases In vitro

Overview

Journal STAR Protoc

Publisher Cell Press

Specialties Biology
Biomedical Engineering
Science

Date 2023 Apr 19

PMID 37074907

Authors

Jason S Wasserman

Felicity Feiser

Seren Palacio

Kishan Patel

Joy Gonzalez

Holly Fowle

Xavier Grana

Affiliations

Soon will be listed here.

Abstract

Serine/threonine protein phosphatase 2 (PP2A) forms heterotrimeric holoenzymes, where a scaffold subunit bridges the PP2A catalytic subunit to a B regulatory subunit, e.g., B55α. The PP2A/B55α holoenzyme plays key roles in signaling and cell-cycle control targeting multiple substrates. Here, we describe semiquantitative approaches to determine PP2A/B55α substrate specificity. Parts I and II detail approaches to assess PP2A/B55α-mediated dephosphorylation of immobilized substrate peptide variants. Parts III and IV detail methods to assess PP2A/B55α-substrate-binding specificity. These approaches are adaptable to other serine/threonine phosphatases. For complete details on the use and execution of this protocol, please refer to Fowle et al...

Citing Articles

FAM122A ensures cell cycle interphase progression and checkpoint control by inhibiting B55α/PP2A through helical motifs.

Wasserman J, Faezov B, Patel K, Kurimchak A, Palacio S, Glass D Nat Commun. 2024; 15(1):5776.

PMID: 38982062 PMC: 11233601. DOI: 10.1038/s41467-024-50015-7.

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