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Probing the structure of membrane proteins with electron spin echo envelope modulation spectroscopy

✍ Scribed by Daniel Mayo; Andy Zhou; Indra Sahu; Robert McCarrick; Parker Walton; Adam Ring; Kaylee Troxel; Aaron Coey; Jaclyn Hawn; Abdul-Hamid Emwas; Gary A. Lorigan


Publisher
Cold Spring Harbor Laboratory Press
Year
2011
Tongue
English
Weight
178 KB
Volume
20
Category
Article
ISSN
0961-8368

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✦ Synopsis


Abstract

A new approach has been developed to probe the structural properties of membrane peptides and proteins using the pulsed electron paramagnetic resonance technique of electron spin echo envelope modulation (ESEEM) spectroscopy and the α‐helical M2Ξ΄ subunit of the acetylcholine receptor incorporated into phospholipid bicelles. To demonstrate the practicality of this method, a cysteine‐mutated nitroxide spin label (SL) is positioned 1, 2, 3, and 4 residues away from a fully deuterated Val side chain (denoted i + 1 to i + 4). The characteristic periodicity of the α‐helical structure gives rise to a unique pattern in the ESEEM spectra. In the i + 1 and i + 2 samples, the ^2^H nuclei are too far away to be detected. However, with the 3.6 residue per turn pattern of an α‐helix, the i + 3 and i + 4 samples reveal a strong signal from the ^2^H nuclei of the Val side chain. Modeling studies verify these data suggesting that the closest ^2^H‐labeled Val to SL distance would in fact be expected in the i + 3 and i + 4 samples. This technique is very advantageous, because it provides pertinent qualitative structural information on an inherently difficult system like membrane proteins in a short period of time (minutes) with small amounts of protein (ΞΌg).


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