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Topology of the trans-membrane peptide WALP23 in model membranes under negative mismatch conditions

By E. Matalon, I. Kaminker, H. Zimmermann, M. Eisenstein, Y. Shai and D. Goldfarb


The organization and orientation of membrane−inserted helices is important for better understanding the mode of action of membrane−active peptides and of protein−membrane interactions. Here we report on the application of ESEEM (electron spin−echo envelope modulation) and DEER (double electron−electron resonance) techniques to probe the orientation and oligomeric state of an α−helical trans−membrane model peptide, WALP23, under conditions of negative mismatch between the hydrophobic cores of the model membrane and the peptide. Using ESEEM, we measured weak dipolar interactions between spin−labeled WALP23 and (2)H nuclei of either the solvent (D(2)O) or of lipids specifically deuterated at the choline group. The ESEEM data obtained from the deuterated lipids were fitted using a model that provided the spin label average distance from a layer of (2)H nuclei in the hydrophilic region of the membrane and the density of the (2)H nuclei in the layer. DEER was used to probe oligomerization through the dipolar interaction between two spin−labels on different peptides. We observed that the center of WALP23 does not coincide with the bilayer midplane and its N−terminus is more buried than the C−terminus. In addition, the ESEEM data fitting yielded a (2)H layer density that was much lower than expected. The DEER experiments revealed the presence of oligomers, the presence of which was attributable to the negative mismatch and the electrostatic dipole of the peptide. A discussion of a possible arrangement of the individual helices in the oligomers that is consistent with the ESEEM and DEER data is presente

Publisher: 'American Chemical Society (ACS)'
Year: 2013
DOI identifier: 10.1021/jp310056h
OAI identifier:
Provided by: MPG.PuRe
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