TY - JOUR
T1 - On the acquisition and analysis of microscale thermophoresis data
AU - Scheuermann, Thomas H.
AU - Padrick, Shae B.
AU - Gardner, Kevin H.
AU - Brautigam, Chad A.
N1 - Funding Information:
The authors thank Peter Schuck, Xian-Jin Xie, and Xuewu Zhang for helpful discussions. Chris Jao is thanked for suggestions on an early version of PALMIST. This work has been supported by grants from the Cancer Research and Prevention Institute of Texas ( RP-130513 to K.H.G.). S.B.P. was supported by grants to Michael K. Rosen from the Howard Hughes Medical Institute , the NIH ( GM56322 ), and the Welch Foundation ( I-1544 ). C.A.B. was also supported by GM56322 to M.K. Rosen.
Publisher Copyright:
© 2015 Elsevier Inc. All rights reserved.
PY - 2016/3/1
Y1 - 2016/3/1
N2 - A comprehensive understanding of the molecular mechanisms underpinning cellular functions is dependent on a detailed characterization of the energetics of macromolecular binding, often quantified by the equilibrium dissociation constant, KD. While many biophysical methods may be used to obtain KD, the focus of this report is a relatively new method called microscale thermophoresis (MST). In an MST experiment, a capillary tube filled with a solution containing a dye-labeled solute is illuminated with an infrared laser, rapidly creating a temperature gradient. Molecules will migrate along this gradient, causing changes in the observed fluorescence. Because the net migration of the labeled molecules will depend on their liganded state, a binding curve as a function of ligand concentration can be constructed from MST data and analyzed to determine KD. Herein, simulations demonstrate the limits of KD that can be measured in current instrumentation. They also show that binding kinetics is a major concern in planning and executing MST experiments. Additionally, studies of two protein-protein interactions illustrate challenges encountered in acquiring and analyzing MST data. Combined, these approaches indicate a set of best practices for performing and analyzing MST experiments. Software for rigorous data analysis is also introduced.
AB - A comprehensive understanding of the molecular mechanisms underpinning cellular functions is dependent on a detailed characterization of the energetics of macromolecular binding, often quantified by the equilibrium dissociation constant, KD. While many biophysical methods may be used to obtain KD, the focus of this report is a relatively new method called microscale thermophoresis (MST). In an MST experiment, a capillary tube filled with a solution containing a dye-labeled solute is illuminated with an infrared laser, rapidly creating a temperature gradient. Molecules will migrate along this gradient, causing changes in the observed fluorescence. Because the net migration of the labeled molecules will depend on their liganded state, a binding curve as a function of ligand concentration can be constructed from MST data and analyzed to determine KD. Herein, simulations demonstrate the limits of KD that can be measured in current instrumentation. They also show that binding kinetics is a major concern in planning and executing MST experiments. Additionally, studies of two protein-protein interactions illustrate challenges encountered in acquiring and analyzing MST data. Combined, these approaches indicate a set of best practices for performing and analyzing MST experiments. Software for rigorous data analysis is also introduced.
KW - Actin
KW - Hypoxia-inducible factor
KW - Isothermal titration calorimetry
KW - Microscale thermophoresis
KW - PALMIST
KW - Protein-protein interactions
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U2 - 10.1016/j.ab.2015.12.013
DO - 10.1016/j.ab.2015.12.013
M3 - Article
C2 - 26739938
AN - SCOPUS:84955247395
SN - 0003-2697
VL - 496
SP - 79
EP - 93
JO - Analytical Biochemistry
JF - Analytical Biochemistry
ER -