Volume 21, Issue 3, Pages (March 2013)

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Volume 21, Issue 3, Pages 394-401 (March 2013) Cell-free Expressed Bacteriorhodopsin in Different Soluble Membrane Mimetics: Biophysical Properties and NMR Accessibility  Manuel Etzkorn, Thomas Raschle, Franz Hagn, Vladimir Gelev, Amanda J. Rice, Thomas Walz, Gerhard Wagner  Structure  Volume 21, Issue 3, Pages 394-401 (March 2013) DOI: 10.1016/j.str.2013.01.005 Copyright © 2013 Elsevier Ltd Terms and Conditions

Structure 2013 21, 394-401DOI: (10.1016/j.str.2013.01.005) Copyright © 2013 Elsevier Ltd Terms and Conditions

Figure 1 The Role of Cell-free Expression for a Bias-free Analysis of the Environment This figure shows differences between bR in DDM micelles when extracted from the native purple membrane (Schubert et al., 2002) or when refolded after cell-free expression. Residues in the transmembrane region that experience chemical shift alterations due to the different sample preparation are highlighted in red (on the crystal structure; Luecke et al., 1999b). Blue residues do not display any significant difference. Lipids (fragments) as present in the crystal are shown in yellow. See Figure S1 for experimental data and more details. Structure 2013 21, 394-401DOI: (10.1016/j.str.2013.01.005) Copyright © 2013 Elsevier Ltd Terms and Conditions

Figure 2 Biophysical Properties of Cell-free Expressed bR Refolded into Different Soluble Membrane-Mimicking Environments (A) SEC of bR in DDM micelles (bR-DDM, black), in A8-35 amphipols (bR-APOL, red) and in DMPC lipid bilayer nanodiscs (bR-ND, blue). (B) Thermal denaturation curves of bR in the same environments, measured by fluorescence intensity of Sypro Orange (Sigma-Aldrich). First derivatives of fitting curves are shown (see Figure S2 for full experimental data). (C) Lifetimes of bR in different environments as measured by time-resolved absorption spectroscopy at a wavelength of 550 nm (indicative of intact tertiary structure) at 58°C. (D) Absorption profile of bR in the different environments. To enable a better comparison, data in (A)–(D) were normalized (also see Figure S2 for experimental data on light/dark adaptation). (E) NMR analysis of bR rotational correlation times τc as a function of proton resonance frequency in indicated environments and temperatures. Values were determined using the TRACT experiment (Lee et al., 2006). Error bars give an estimate of the error margin of calculating the shown correlation time from the experimental data. Starting from the root mean square error of the fitted relaxation rates in the TRACT data, the values for the error bars are calculated according to error propagation and by using the goodness-of-fit function in matlab (MathWorks). Structure 2013 21, 394-401DOI: (10.1016/j.str.2013.01.005) Copyright © 2013 Elsevier Ltd Terms and Conditions

Figure 3 Characterization of bR-ND (A) SEC of bR directly incorporated into nanodiscs during cell-free expression. (B and C) Representative negative-stained EM images of fraction A (B) and of fraction B (C). (D) Representative class averages obtained with fraction B (see Figure S3 for full set). (E and F) TROSY-HSQC NMR spectra of fraction A (E) and fraction B (F). (G–I) Set of 3D TROSY NMR data recorded on bR in DMPC nanodiscs after optimization of refolding conditions. (G) HNCA, (H) NOESY-HSQC, (I) HNcaCB). Strip plots for residues from the end of helix G toward the C terminus are shown. 3D spectra were recorded at 48°C. See supporting information Figure S3 for more details. Structure 2013 21, 394-401DOI: (10.1016/j.str.2013.01.005) Copyright © 2013 Elsevier Ltd Terms and Conditions

Figure 4 Effects Induced by Different Membrane-Mimetic Environments on Local bR Structure (A–C) Illustration of bR in the different environments and corresponding TROSY-HSQC NMR spectra. All spectra were recorded at 40°C on cell-free expressed and refolded bR. The illustration in (A) shows bR (red) in micelles with 126 detergent molecules. In (B), eight amphipol molecules are shown in different shading. The nanodisc shown in (C) comprises 100 DMPC molecules and two copies of MSP1D1 (green). (Note that the shown particles are drawn to scale to illustrate the different environments and are not energy minimized.) (D) Overall chemical-shift perturbations for assigned residues mapped on the structure of bR (green: no perturbation, purple: changes in at least one environment). Lipids as identified in the crystal structure (Luecke et al., 1999b) are shown in transparent gray. (See supporting information Figure S4 for complete residue-specific pairwise analysis). (E) Classification of regions interacting differently with the surrounding membrane mimetic. Only residues for which chemical-shift changes could be assigned in all environments (39 in total) are highlighted. Residues not present in the X-ray structure are indicated as ellipses in matching colors. (F) Example of selected peaks for all classes (colors of residue labels indicate the respective classes shown in (E); the color code for the NMR spectra is: black, bR-DDM; blue, bR-ND; red, bR-APOL). (G) Average chemical-shift perturbation per residue for the different classes. Numbers above bars indicate the amount of assigned/total residues per class. The pairwise differences between the three environments are shown separately. Structure 2013 21, 394-401DOI: (10.1016/j.str.2013.01.005) Copyright © 2013 Elsevier Ltd Terms and Conditions