High‐Throughput Screening of Protein‐Detergent Complexes Using Fluorescence Polarization Spectroscopy
Author(s) -
Wolfe Aaron J.,
Parella Kyle J.,
Movileanu Liviu
Publication year - 2019
Publication title -
current protocols in protein science
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.409
H-Index - 32
eISSN - 1934-3663
pISSN - 1934-3655
DOI - 10.1002/cpps.96
Subject(s) - fluorescence spectroscopy , fluorescence , fluorescence anisotropy , chemistry , spectroscopy , throughput , high throughput screening , biophysics , biochemistry , biology , computer science , physics , optics , quantum mechanics , telecommunications , wireless
This article provides detailed protocols for a high‐throughput fluorescence polarization (FP) spectroscopy approach to disentangle the interactions of membrane proteins with solubilizing detergents. Existing techniques for examining the membrane protein‐detergent complex (PDC) interactions are low throughput and require high amounts of proteins. Here, we describe a 96‐well analytical approach, which facilitates a scalable analysis of the PDC interactions at low‐nanomolar concentrations of membrane proteins in native solutions. At detergent concentrations much greater than the equilibrium dissociation constant of the PDC, K d , the FP anisotropy reaches a saturated value, so it is independent of the detergent concentration. On the contrary, at detergent concentrations comparable with or lower than the K d , the FP anisotropy readout undergoes a time‐dependent decrease, exhibiting a sensitive and specific detergent‐dissociation signature. Our approach can also be used for determining the kinetic rate constants of association and dissociation. With further development, these protocols might be used in various arenas of membrane protein research that pertain to extraction, solubilization, and stabilization. © 2019 by John Wiley & Sons, Inc.
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