Literature DB >> 15631464

Detecting protein-protein interactions with a green fluorescent protein fragment reassembly trap: scope and mechanism.

Thomas J Magliery1, Christopher G M Wilson, Weilan Pan, Dennis Mishler, Indraneel Ghosh, Andrew D Hamilton, Lynne Regan.   

Abstract

Identification of protein binding partners is one of the key challenges of proteomics. We recently introduced a screen for detecting protein-protein interactions based on reassembly of dissected fragments of green fluorescent protein fused to interacting peptides. Here, we present a set of comaintained Escherichia coli plasmids for the facile subcloning of fusions to the green fluorescent protein fragments. Using a library of antiparallel leucine zippers, we have shown that the screen can detect very weak interactions (K(D) approximately 1 mM). In vitro kinetics show that the reassembly reaction is essentially irreversible, suggesting that the screen may be useful for detecting transient interactions. Finally, we used the screen to discriminate cognate from noncognate protein-ligand interactions for tetratricopeptide repeat domains. These experiments demonstrate the general utility of the screen for larger proteins and elucidate mechanistic details to guide the further use of this screen in proteomic analysis. Additionally, this work gives insight into the positional inequivalence of stabilizing interactions in antiparallel coiled coils.

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Year:  2005        PMID: 15631464     DOI: 10.1021/ja046699g

Source DB:  PubMed          Journal:  J Am Chem Soc        ISSN: 0002-7863            Impact factor:   15.419


  165 in total

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6.  Kinetics and reaction coordinates of the reassembly of protein fragments via forward flux sampling.

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9.  In vivo protein stabilization based on fragment complementation and a split GFP system.

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10.  Use of fluorescence microscopy to probe intracellular lipolysis.

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Journal:  Methods Enzymol       Date:  2014       Impact factor: 1.600

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