DIP-MS: ultra-deep interaction proteomics for the deconvolution of protein complexes

Author:

Frommelt FabianORCID,Fossati Andrea,Uliana Federico,Wendt FabianORCID,Xue Peng,Heusel Moritz,Wollscheid BerndORCID,Aebersold RuediORCID,Ciuffa Rodolfo,Gstaiger MatthiasORCID

Abstract

AbstractMost proteins are organized in macromolecular assemblies, which represent key functional units regulating and catalyzing most cellular processes. Affinity purification of the protein of interest combined with liquid chromatography coupled to tandem mass spectrometry (AP–MS) represents the method of choice to identify interacting proteins. The composition of complex isoforms concurrently present in the AP sample can, however, not be resolved from a single AP–MS experiment but requires computational inference from multiple time- and resource-intensive reciprocal AP–MS experiments. Here we introduce deep interactome profiling by mass spectrometry (DIP-MS), which combines AP with blue-native-PAGE separation, data-independent acquisition with mass spectrometry and deep-learning-based signal processing to resolve complex isoforms sharing the same bait protein in a single experiment. We applied DIP-MS to probe the organization of the human prefoldin family of complexes, resolving distinct prefoldin holo- and subcomplex variants, complex–complex interactions and complex isoforms with new subunits that were experimentally validated. Our results demonstrate that DIP-MS can reveal proteome modularity at unprecedented depth and resolution.

Funder

Innovative Medicines Initiative

Publisher

Springer Science and Business Media LLC

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