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Using Protein Dimers to Maximize the Protein Hybridization Efficiency with Multisite DNA Origami Scaffolds
Author(s) -
Vikash Verma,
Leena Mallik,
Rizal F. Hariadi,
Sivaraj Sivaramakrishnan,
Georgios Skiniotis,
Ajit P. Joglekar
Publication year - 2015
Publication title -
plos one
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.99
H-Index - 332
ISSN - 1932-6203
DOI - 10.1371/journal.pone.0137125
Subject(s) - dna origami , scaffold protein , scaffold , function (biology) , multiplex , protein engineering , computational biology , population , dna–dna hybridization , dna , nanotechnology , chemistry , biology , computer science , bioinformatics , materials science , genetics , biochemistry , enzyme , database , sociology , signal transduction , demography
DNA origami provides a versatile platform for conducting ‘architecture-function’ analysis to determine how the nanoscale organization of multiple copies of a protein component within a multi-protein machine affects its overall function. Such analysis requires that the copy number of protein molecules bound to the origami scaffold exactly matches the desired number, and that it is uniform over an entire scaffold population. This requirement is challenging to satisfy for origami scaffolds with many protein hybridization sites, because it requires the successful completion of multiple, independent hybridization reactions. Here, we show that a cleavable dimerization domain on the hybridizing protein can be used to multiplex hybridization reactions on an origami scaffold. This strategy yields nearly 100% hybridization efficiency on a 6-site scaffold even when using low protein concentration and short incubation time. It can also be developed further to enable reliable patterning of a large number of molecules on DNA origami for architecture-function analysis.

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