Real-time single-molecule coimmunoprecipitation of weak protein-protein interactions

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Coimmunoprecipitation (co-IP) analysis is a useful method for studying protein-protein interactions. It currently involves electrophoresis and western blotting, which are not optimized for detecting weak and transient interactions. In this protocol we describe an advanced version of co-IP analysis that uses real-time, single-molecule fluorescence imaging as its detection scheme. Bait proteins are pulled down onto the imaging plane of a total internal reflection (TIR) microscope. With unpurified cells or tissue extracts kept in reaction chambers, we observe single protein-protein interactions between the surface-immobilized bait and the fluorescent protein-labeled prey proteins in real time. Such direct recording provides an improvement of five orders of magnitude in the time resolution of co-IP analysis. With the single-molecule sensitivity and millisecond time resolution, which distinguish our method from other methods for measuring weak protein-protein interactions, it is possible to quantify the interaction kinetics and active fraction of native, unlabeled bait proteins. Real-time single-molecule co-IP analysis, which takes similar to 4 h to complete from lysate preparation to kinetic analysis, provides a general avenue for revealing the rich kinetic picture of target protein-protein interactions, and it can be used, for example, to investigate the molecular lesions that drive individual cancers at the level of protein-protein interactions.
Publisher
NATURE PUBLISHING GROUP
Issue Date
2013-10
Language
English
Article Type
Article
Keywords

PROXIMITY LIGATION; PULL-DOWN; IN-SITU; RAS; BINDING; RECEPTOR; DYNAMICS; KINASES; CANCER; DOMAIN

Citation

NATURE PROTOCOLS, v.8, no.10, pp.2045 - 2060

ISSN
1754-2189
DOI
10.1038/nprot.2013.116
URI
http://hdl.handle.net/10203/188532
Appears in Collection
PH-Journal Papers(저널논문)
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