A biosensor generated via high-throughput screening quantifies cell edge Src dynamics
A biosensor generated via high-throughput screening quantifies cell edge Src dynamics
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Date
2011-01-01
Authors
Gulyani, Akash
Vitriol, Eric
Allen, Richard
Wu, Jianrong
Gremyachinskiy, Dmitriy
Lewis, Steven
Dewar, Brian
Graves, Lee M.
Kay, Brian K.
Kuhlman, Brian
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Abstract
Fluorescent biosensors for living cells currently require laborious optimization and a unique design for each target. They are limited by the availability of naturally occurring ligands with appropriate target specificity. Here we describe a biosensor based on an engineered fibronectin monobody scaffold that can be tailored to bind different targets via high-throughput screening. We made this Src-family kinase (SFK) biosensor by derivatizing a monobody specific for activated SFKs with a bright dye whose fluorescence increases upon target binding. We identified sites for dye attachment and changes to eliminate vesiculation in living cells, providing a generalizable scaffold for biosensor production. This approach minimizes cell perturbation because it senses endogenous, unmodified target, and because sensitivity is enhanced by direct dye excitation. Automated correlation of cell velocities and SFK activity revealed that SFKs are activated specifically during protrusion. Activity correlates with velocity, and peaks 1-2 μm from the leading edge. © 2011 Nature America, Inc. All rights reserved.
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Nature Chemical Biology. v.7(7)