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Literature DB >> 18563728

Discrimination between stable and dynamic components of protein complexes by means of quantitative proteomics.

Keiji Kito¹, Noriko Kawaguchi, Satoshi Okada, Takashi Ito.

Abstract

To discriminate between stable and dynamic protein-protein interactions, we propose a strategy in which cells with and without tagged bait are differentially labeled with stable isotope and combined prior to complex purification. Mass-spectrometric analysis of the purified complexes identifies stable and dynamic components as those derived exclusively from the tagged cells and those from both cells, respectively. We successfully applied this strategy to analyze two yeast protein complexes, eIF2B-eIF2 and cyclin-Cdc28.

Entities: Gene Species

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Year: 2008 PMID： 18563728 DOI： 10.1002/pmic.200800182

Source DB: PubMed Journal: Proteomics ISSN： 1615-9853 Impact factor: 3.984

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Cited

4 in total

Review 1. Profiling of protein interaction networks of protein complexes using affinity purification and quantitative mass spectrometry.

Authors: Robyn M Kaake; Xiaorong Wang; Lan Huang
Journal: Mol Cell Proteomics Date: 2010-05-05 Impact factor: 5.911

Discrimination between stable and dynamic components of protein complexes by means of quantitative proteomics.

Review 1. Profiling of protein interaction networks of protein complexes using affinity purification and quantitative mass spectrometry.

2. Proteomic investigations of complex I composition: how to define a subunit?

Review 3. Studying macromolecular complex stoichiometries by peptide-based mass spectrometry.

4. Multisite phosphorylation networks as signal processors for Cdk1.