4.7 Article

Ultrafast and Reproducible Proteomics from Small Amounts of Heart Tissue Enabled by Azo and timsTOF Pro

JOURNAL OF PROTEOME RESEARCH (2021)

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Journal

JOURNAL OF PROTEOME RESEARCH
Volume 20, Issue 8, Pages 4203-4211

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acs.jproteome.1c00446

Keywords

photocleavable surfactant; human heart proteomics; quantitative proteomics; sample preparation; bottom-up proteomics

Categories

Biochemical Research Methods

Funding

  1. National Institutes of Health (NIH) [R01 HL096971, R01 GM117058, GM125085, HL109810, S10 OD018475]
  2. Training Program in Molecular and Cellular Pharmacology [T32 GM008688-20]
  3. American Heart Association Predoctoral Fellowship [832615/David S. Roberts/2021]
  4. Training Program in Translational Cardiovascular Science [T32 HL007936-20]
  5. Cardiovascular Research Center Training Program in Translational Cardiovascular Science [T32 HL007936-19]
  6. Vascular Surgery Research Training Program Grant [T32HL110853]

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This study developed an ultrafast bottom-up proteomics method using Azo surfactant and timsTOF Pro mass spectrometer for rapid, robust, and reproducible protein identification and quantification, successfully applied to analyze the human cardiac proteome with high coverage and reproducibility in a single run.
Global bottom-up mass spectrometry (MS)-based proteomics is widely used for protein identification and quantification to achieve a comprehensive understanding of the composition, structure, and function of the proteome. However, traditional sample preparation methods are timeconsuming, typically including overnight tryptic digestion, extensive sample cleanup to remove MS-incompatible surfactants, and offline sample fractionation to reduce proteome complexity prior to online liquid chromatography-tandem mass spectrometry (LC-MS/MS) analysis. Thus, there is a need for a fast, robust, and reproducible method for protein identification and quantification from complex proteomes. Herein, we developed an ultrafast bottom-up proteomics method enabled by Azo, a photocleavable, MS-compatible surfactant that effectively solubilizes proteins and promotes rapid tryptic digestion, combined with the Bruker timsTOF Pro, which enables deeper proteome coverage through trapped ion mobility spectrometry (TIMS) and parallel accumulation-serial fragmentation (PASEF) of peptides. We applied this method to analyze the complex human cardiac proteome and identified nearly 4000 protein groups from as little as 1 mg of human heart tissue in a single one-dimensional LC-TIMS-MS/MS run with high reproducibility. Overall, we anticipate this ultrafast, robust, and reproducible bottom-up method empowered by both Azo and the timsTOF Pro will be generally applicable and greatly accelerate the throughput of large-scale quantitative proteomic studies. Raw data are available via the MassIVE repository with identifier MSV000087476.

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