Simple protein complex purification and identification method for high-throughput mapping of protein interaction networks

被引：14

作者：

Markillie, LM ^{[1
]}

Lin, CT ^{[1
]}

Adkins, JN ^{[1
]}

Auberry, DL ^{[1
]}

Hill, EA ^{[1
]}

Hooker, BS ^{[1
]}

Moore, PA ^{[1
]}

Moore, RJ ^{[1
]}

Shi, L ^{[1
]}

Wiley, HS ^{[1
]}

Kery, V ^{[1
]}

机构：

[1] Pacific NW Natl Lab, Richland, WA 99354 USA

来源：

JOURNAL OF PROTEOME RESEARCH | 2005年 / 4卷 / 02期

关键词：

protein complex purification; identification; mass spectrometry; mapping protein interaction networks;

D O I：

10.1021/pr049847a

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

Most current methods for purification and identification of protein complexes use endogenous expression of affinity-tagged bait, tandem affinity tag purification of protein complexes followed by specific elution of complexes from beads, and gel separation and in-gel digestion prior to mass spectrometric analysis of protein interactors. We propose a single affinity tag in vitro pull-down assay with denaturing elution, trypsin digestion in organic solvent, and LC-ESI MS/MS protein identification using SEQUEST analysis. Our method is simple and easy to scale-up and automate, making it suitable for high-throughput mapping of protein interaction networks and functional proteomics.

引用

页码：268 / 274

页数：7

共 25 条

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