An automated proximity proteomics pipeline for subcellular proteome and protein interaction mapping

Author:

Zhong Xiaofang,Li Qiongyu,Polacco Benjamin J.,Patil Trupti,DiBerto Jeffrey F.,Vartak Rasika,Xu Jiewei,Marley Aaron,Foussard Helene,Roth Bryan L.ORCID,Eckhardt ManonORCID,Zastrow Mark VonORCID,Krogan Nevan J.ORCID,Hüttenhain RuthORCID

Abstract

AbstractProximity labeling (PL) coupled with mass spectrometry has emerged as a powerful technique to map proximal protein interactions in living cells. Large-scale sample processing for proximity proteomics necessitates a high-throughput workflow to reduce hands-on time and increase quantitative reproducibility. To address this issue, we developed a scalable and automated PL pipeline, including generation and characterization of monoclonal cell lines, automated enrichment of biotinylated proteins in a 96-well format, and optimization of the quantitative mass spectrometry (MS) acquisition method. Combined with data-independent acquisition (DIA) MS, our pipeline outperforms manual enrichment and data-dependent acquisition (DDA) MS regarding reproducibility of protein identification and quantification. We apply the pipeline to map subcellular proteomes for endosomes, late endosomes/lysosomes, the Golgi apparatus, and the plasma membrane. Moreover, using serotonin receptor (5HT2A) as a model, we investigated agonist-induced dynamics in protein-protein interactions. Importantly, the approach presented here is universally applicable for PL proteomics using all biotinylation-based PL enzymes, increasing both throughput and reproducibility of standard protocols.

Publisher

Cold Spring Harbor Laboratory

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