Dipolar Relaxation Dynamics at the Active Site of an ATPase Regulated by Membrane Lateral Pressure

Elisabeth Fischermeier; Petr Pospíšil; Ahmed Sayed; Martin Hof; Marc Solioz; Karim Fahmy

doi:10.1002/anie.201611582

Dipolar Relaxation Dynamics at the Active Site of an ATPase Regulated by Membrane Lateral Pressure

Angew Chem Int Ed Engl. 2017 Jan 24;56(5):1269-1272. doi: 10.1002/anie.201611582. Epub 2016 Dec 27.

Authors

Elisabeth Fischermeier^{1

2

3}, Petr Pospíšil⁴, Ahmed Sayed^{1

2

5}, Martin Hof⁴, Marc Solioz⁶, Karim Fahmy^{1

2}

Affiliations

¹ Helmholtz-Zentrum Dresden-Rossendorf, Institute of Resource Ecology, Bautzner Landstrasse 400, 01328, Dresden, Germany.
² Technische Universität Dresden, Biotechnology Center, Tatzberg 47-49, 01307, Dresden, Germany.
³ Nationales Zentrum für Tumorerkrankungen Heidelberg, Im Neuenheimer Feld 460, 69120, Heidelberg, Germany.
⁴ J. Heyrovský Inst. Physical Chemistry of the A.S.C.R. v.v.i., Prague, Czech Republic.
⁵ Institute for Experimental Physics I, Universität Leipzig, Linnéstrasse 5, 04103, Leipzig, Germany.
⁶ University of Bern, Dept. of Clinical Pharmacology, Murtenstrasse 35, 3008, Bern, Switzerland.

PMID: 28026092
DOI: 10.1002/anie.201611582

Abstract

The active transport of ions across biological membranes requires their hydration shell to interact with the interior of membrane proteins. However, the influence of the external lipid phase on internal dielectric dynamics is hard to access by experiment. Using the octahelical transmembrane architecture of the copper-transporting P_1B -type ATPase from Legionella pneumophila as a model structure, we have established the site-specific labeling of internal cysteines with a polarity-sensitive fluorophore. This enabled dipolar relaxation studies in a solubilized form of the protein and in its lipid-embedded state in nanodiscs. Time-dependent fluorescence shifts revealed the site-specific hydration and dipole mobility around the conserved ion-binding motif. The spatial distribution of both features is shaped significantly and independently of each other by membrane lateral pressure.

Keywords: fluorescence; ion pump; membrane proteins; nanodiscs; time-resolved emission.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

2-Naphthylamine / analogs & derivatives
2-Naphthylamine / chemistry
Bacterial Proteins / chemistry
Bacterial Proteins / metabolism*
Catalytic Domain
Circular Dichroism
Cysteine / chemistry
Fluorescent Dyes / chemistry
Legionella pneumophila / enzymology
Nanostructures / chemistry
Protein Structure, Secondary

Substances

6-bromoacetyl-2-dimethylaminonaphthalene
Bacterial Proteins
CopA protein, Bacteria
Fluorescent Dyes
2-Naphthylamine
Cysteine