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Microfluidics-based selection of red-fluorescent proteins with decreased rates of photobleaching
Author(s) -
Kevin M. Dean,
Jennifer L. Lubbeck,
Lloyd M. Davis,
Chola Regmi,
Prem P. Chapagain,
Bernard S. Gerstman,
Ralph Jimenez,
Amy E. Palmer
Publication year - 2014
Publication title -
integrative biology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.853
H-Index - 70
eISSN - 1757-9708
pISSN - 1757-9694
DOI - 10.1039/c4ib00251b
Subject(s) - mcherry , photobleaching , fluorescence , fluorescence recovery after photobleaching , fluorescent protein , green fluorescent protein , biophysics , microfluidics , microbiology and biotechnology , live cell imaging , chemistry , biology , biochemistry , cell , nanotechnology , materials science , physics , quantum mechanics , gene
Fluorescent proteins offer exceptional labeling specificity in living cells and organisms. Unfortunately, their photophysical properties remain far from ideal for long-term imaging of low-abundance cellular constituents, in large part because of their poor photostability. Despite widespread engineering efforts, improving the photostability of fluorescent proteins remains challenging due to lack of appropriate high-throughput selection methods. Here, we use molecular dynamics guided mutagenesis in conjunction with a recently developed microfluidic-based platform, which sorts cells based on their fluorescence photostability, to identify red fluorescent proteins with decreased photobleaching from a HeLa cell-based library. The identified mutant, named Kriek, has 2.5- and 4-fold higher photostability than its progenitor, mCherry, under widefield and confocal illumination, respectively. Furthermore, the results provide insight into mechanisms for enhancing photostability and their connections with other photophysical processes, thereby providing direction for ongoing development of fluorescent proteins with improved single-molecule and low-copy imaging capabilities.

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