Analysis of high-affinity assembly for AMPA receptor amino-terminal domains

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Analytical ultracentrifugation (AUC) and steady-state fluorescence anisotropy were used to measure the equilibrium dissociation constant (K(d)) for formation of dimers by the amino-terminal domains (ATDs) of the GluA2 and GluA3 subtypes of AMPA receptor. Previous reports on GluA2 dimerization differ...

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Detalles Bibliográficos
Autores principales: Zhao, Huaying, Berger, Anthony J., Brown, Patrick H., Kumar, Janesh, Balbo, Andrea, May, Carrie A., Casillas, Ernesto, Laue, Thomas M., Patterson, George H., Mayer, Mark L., Schuck, Peter
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The Rockefeller University Press 2012
Materias:
Tutorial Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3343374/
https://www.ncbi.nlm.nih.gov/pubmed/22508847
http://dx.doi.org/10.1085/jgp.201210770
Descripción
Sumario:Analytical ultracentrifugation (AUC) and steady-state fluorescence anisotropy were used to measure the equilibrium dissociation constant (K(d)) for formation of dimers by the amino-terminal domains (ATDs) of the GluA2 and GluA3 subtypes of AMPA receptor. Previous reports on GluA2 dimerization differed in their estimate of the monomer–dimer K(d) by a 2,400-fold range, with no consensus on whether the ATD forms tetramers in solution. We find by sedimentation velocity (SV) analysis performed using absorbance detection a narrow range of monomer–dimer K(d) values for GluA2, from 5 to 11 nM for six independent experiments, with no detectable formation of tetramers and no effect of glycosylation or the polypeptide linker connecting the ATD and ligand-binding domains; for GluA3, the monomer–dimer K(d) was 5.6 µM, again with no detectable tetramer formation. For sedimentation equilibrium (SE) experiments, a wide range of K(d) values was obtained for GluA2, from 13 to 284 nM, whereas for GluA3, the K(d) of 3.1 µM was less than twofold different from the SV value. Analysis of cell contents after the ∼1-week centrifuge run by silver-stained gels revealed low molecular weight GluA2 breakdown products. Simulated data for SE runs demonstrate that the apparent K(d) for GluA2 varies with the extent of proteolysis, leading to artificially high K(d) values. SV experiments with fluorescence detection for GluA2 labeled with 5,6-carboxyfluorescein, and fluorescence anisotropy measurements for GluA2 labeled with DyLight405, yielded K(d) values of 5 and 11 nM, consistent with those from SV with absorbance detection. However, the sedimentation coefficients measured by AUC using absorbance and fluorescence systems were strikingly different, and for the latter are not consistent with hydrodynamic protein models. Thus, for unknown reasons, the concentration dependence of sedimentation coefficients obtained with fluorescence detection SV may be unreliable, limiting the usefulness of this technique for quantitative analysis.

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