Protocol

Assessing Ubiquitylation of Individual Proteins Using Xenopus Extract Systems

  1. Anna Philpott3,4,5
  1. 1Future of Research, Abington, Massachusetts 02351
  2. 2Manylabs, San Francisco, California 94103
  3. 3Department of Oncology, MRC/Hutchison Research Centre, Cambridge CB21XZ, United Kingdom
  4. 4Wellcome Trust-Medical Research Centre Cambridge Stem Cell Institute, University of Cambridge, Cambridge CB21QR, United Kingdom
  1. 5Correspondence: ap113{at}cam.ac.uk; garymcdow{at}gmail.com

Abstract

Xenopus extract systems have been used to study ubiquitylation of proteins, and to uncover some of the fundamental processes of the ubiquitylation pathway itself. They provide a simple, quick, and robust method for studying ubiquitylation. In this protocol, methods are provided for studying protein ubiquitylation using Xenopus egg or embryo extracts and in vitro radiolabeled proteins. These methods also enable examination of whether proteins undergo noncanonical ubiquitylation, through modification of the protein by covalent linkage to ubiquitin through residues other than lysine, such as cysteine, serine, and threonine.

Footnotes

  • From the Xenopus collection, edited by Hazel L. Sive.

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  1. Published in Advance May 16, 2018, doi: 10.1101/pdb.prot104513 Cold Spring Harb Protoc © 2019 Cold Spring Harbor Laboratory Press
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  1. Profile for McDowell, G. S.http://orcid.org/0000-0002-9470-3799

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