Literature DB >> 17993485

In silico protein fragmentation reveals the importance of critical nuclei on domain reassembly.

Lydia M Contreras Martínez1, Ernesto E Borrero Quintana, Fernando A Escobedo, Matthew P DeLisa.   

Abstract

Protein complementation assays (PCAs) based on split protein fragments have become powerful tools that facilitate the study and engineering of intracellular protein-protein interactions. These assays are based on the observation that a given protein can be split into two inactive fragments and these fragments can reassemble into the original properly folded and functional structure. However, one experimentally observed limitation of PCA systems is that the folding of a protein from its fragments is dramatically slower relative to that of the unsplit parent protein. This is due in part to a poor understanding of how PCA design parameters such as split site position in the primary sequence and size of the resulting fragments contribute to the efficiency of protein reassembly. We used a minimalist on-lattice model to analyze how the dynamics of the reassembly process for two model proteins was affected by the location of the split site. Our results demonstrate that the balanced distribution of the "folding nucleus," a subset of residues that are critical to the formation of the transition state leading to productive folding, between protein fragments is key to their reassembly.

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Year:  2007        PMID: 17993485      PMCID: PMC2242749          DOI: 10.1529/biophysj.107.119651

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  43 in total

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  2 in total

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

Authors:  Ernesto E Borrero; Lydia M Contreras Martínez; Matthew P DeLisa; Fernando A Escobedo
Journal:  Biophys J       Date:  2010-05-19       Impact factor: 4.033

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  2 in total

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