Technical report: Targeted proteomic analysis reveals enrichment of atypical ubiquitin chains in contractile murine tissues

Tiaan Heunis; Frederic Lamoliatte; José Luis Marín-Rubio; Abeer Dannoura; Matthias Trost

doi:10.1016/j.jprot.2020.103963

Technical report: Targeted proteomic analysis reveals enrichment of atypical ubiquitin chains in contractile murine tissues

J Proteomics. 2020 Oct 30:229:103963. doi: 10.1016/j.jprot.2020.103963. Epub 2020 Sep 6.

Authors

Tiaan Heunis¹, Frederic Lamoliatte¹, José Luis Marín-Rubio¹, Abeer Dannoura¹, Matthias Trost²

Affiliations

¹ Biosciences Institute, Newcastle University, NE2 4HH Newcastle upon Tyne, United Kingdom.
² Biosciences Institute, Newcastle University, NE2 4HH Newcastle upon Tyne, United Kingdom. Electronic address: matthias.trost@ncl.ac.uk.

Abstract

Ubiquitylation is an elaborate post-translational modification involved in all biological processes. Its pleotropic effect is driven by the ability to form complex polyubiquitin chain architectures that can influence biological functions. In this study, we optimised sample preparation and chromatographic separation of Ubiquitin peptides for Absolute Quantification by Parallel Reaction Monitoring (Ub-AQUA-PRM). Using this refined Ub-AQUA-PRM assay, we were able to quantify all ubiquitin chain types in 10-min LC-MS/MS runs. We used this method to determine the ubiquitin chain-linkage composition in murine bone marrow-derived macrophages and different mouse tissues. We could show tissue-specific differences in ubiquitin levels in murine tissues, with polyubiquitin chain types contributing a small proportion to the total pool of ubiquitin. Interestingly, we observed enrichment of atypical (K33) ubiquitin chains in heart and muscle. Our approach enabled high-throughput screening of ubiquitin chain-linkage composition in different murine tissues and highlighted a possible role for atypical ubiquitylation in contractile tissues. SIGNIFICANCE: Large knowledge gaps exist in our understanding of ubiquitin chain-linkage composition in mammalian tissues. Defining this in vivo ubiquitin chain-linkage landscape could reveal the functional importance of different ubiquitin chain types in tissues. In this study, we refined the previously described Ub-AQUA-PRM assay to enable quantification of all ubiquitin chain types in a high-throughput manner. Using this assay, we provided new data on the ubiquitin chain-linkage composition in primary murine macrophages and tissues, and revealed an enrichment of atypical ubiquitin chains in contractile tissues. Our approach should thus enable rapid, high-throughput screening of ubiquitin chain-linkage composition in different sample types, as demonstrated in murine primary cells and tissues.

Keywords: Absolute quantification; Atypical ubiquitin chain types; Murine; Parallel reaction monitoring; Primary murine macrophages; Tissues; Ubiquitin chain-linkage.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Chromatography, Liquid
Mice
Polyubiquitin / metabolism
Proteomics*
Tandem Mass Spectrometry
Ubiquitin* / metabolism
Ubiquitination

Substances

Ubiquitin
Polyubiquitin

Abstract

Publication types

MeSH terms

Substances

Grants and funding