Solid-State NMR Studies of a Diverged Microsomal Amino-Proximate {Delta}12 Desaturase Peptide Reveal Causes of Stability in Membrane: Tyrosine Anchoring and Arginine Snorkeling

doi:10.1529/biophysj.105.067884

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Biophys. J. BioFAST: First Published December 2, 2005. doi:10.1529/biophysj.105.067884
© 2005 by the Biophysical Society.

A more recent version of this article appeared on February 15, 2006.

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MEMBRANES

Solid-State NMR Studies of a Diverged Microsomal Amino-Proximate ${Delta}$ ¹² Desaturase Peptide Reveal Causes of Stability in Membrane: Tyrosine Anchoring and Arginine Snorkeling

William J. Gibbons ¹, Ethan S. Karp ¹, Nick A. Cellar ¹, Robert E. Minto ¹ and Gary A. Lorigan ¹^*

¹ Miami University

^* To whom correspondence should be addressed. E-mail: lorigag{at}muohio.edu.

Submitted on June 2, 2005
Revised on July 20, 2005
Accepted on 28 October 2005

Abstract
This study reports the solid-state NMR spectroscopic characterizationof the amino-proximate transmembrane domain (TM-A) of a divergedmicrosomal ${Delta}$ ¹²-desaturase (CREP-1) in a phospholipid bilayer. A series of TM-A peptides were synthesized with ²H-labeledside chains (Ala-53, -56, and -63, Leu-62, Val-50) and theirdynamic properties were studied in 1,2-dimyristoyl-sn-glycero-3-phosphatidylcholine(DMPC) bilayers at various temperatures. At 6 mol% peptide tolipid, ³¹P NMR spectra indicated that the peptides did not significantlydisrupt the phospholipid bilayer in the Lphase. The ²H NMRspectra from Ala-53 and Ala-56 samples revealed broad Pake patternswith quadrupolar splittings of 16.9 kHz and 13.3 kHz, respectively,indicating restricted motion confined within the hydrocarboncore of the phospholipid bilayer. Conversely, the deuteratedAla-63 sample revealed a peak centered at 0 kHz with a linewidthof 1.9 kHz indicating increased side chain motion and solvent-exposurerelative to the spectra of the other Ala residues. Val-50 andLeu-62 showed Pake patterns, with quadrupolar splittings of3.5 kHz and 3.7 kHz, respectively, intermediate to Ala-53/Ala-56and Ala-63. This indicates partial motional averaging and supportsa model with the Val and Leu residues embedded inside the lipidbilayer. Solid-state NMR spectroscopy performed on the ²H-labelledAla-56 TM-A peptide incorporated into magnetically aligned phospholipidbilayers indicated that the peptide is tilted 8° with respectto the membrane normal of the lipid bilayer. Snorkeling andanchoring interactions of Arg-44 and Tyr-60, respectively, withthe polar region or polar hydrophobic interface of the lipidbilayer are suggested as control elements for insertional depthand orientation of the helix in the lipid matrix. Thus, thisstudy defines the location of key residues in TM-A with respectto the lipid bilayer, the conformation in a biomembrane mimic,and presents a peptide-bilayer model useful in the considerationof local protein folding in the microsomal desaturases and amodel of arginine and tyrosine control of transmembrane proteinstability and insertion.