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Journal article

A rapid methods development workflow for high-throughput quantitative proteomic applications

In Plos One 2019, Volume 14, Issue 2, pp. e0211582

Edited by Jacobs, Jon M.

From

Lawrence Berkeley National Laboratory1

Novo Nordisk Foundation Center for Biosustainability, Technical University of Denmark2

Synthetic Biology Tools for Yeast, Novo Nordisk Foundation Center for Biosustainability, Technical University of Denmark3

Recent improvements in the speed and sensitivity of liquid chromatography-mass spectrometry systems have driven significant progress toward system-wide characterization of the proteome of many species. These efforts create large proteomic datasets that provide insight into biological processes and identify diagnostic proteins whose abundance changes significantly under different experimental conditions.

Yet, these system-wide experiments are typically the starting point for hypothesis-driven, follow-up experiments to elucidate the extent of the phenomenon or the utility of the diagnostic marker, wherein many samples must be analyzed. Transitioning from a few discovery experiments to quantitative analyses on hundreds of samples requires significant resources both to develop sensitive and specific methods as well as analyze them in a high-throughput manner.

To aid these efforts, we developed a workflow using data acquired from discovery proteomic experiments, retention time prediction, and standard-flow chromatography to rapidly develop targeted proteomic assays. We demonstrated this workflow by developing MRM assays to quantify proteins of multiple metabolic pathways from multiple microbes under different experimental conditions.

With this workflow, one can also target peptides in scheduled/dynamic acquisition methods from a shotgun proteomic dataset downloaded from online repositories, validate with appropriate control samples or standard peptides, and begin analyzing hundreds of samples in only a few minutes.

Language: English
Publisher: Public Library of Science
Year: 2019
Pages: e0211582
ISSN: 19326203
Types: Journal article
DOI: 10.1371/journal.pone.0211582
ORCIDs: 0000-0002-4950-7967 and 0000-0002-8270-5228

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