NMR structure of the second intracellular loop of ...[Biochemistry. 2002]

Ph: 11888275

All Databases PubMed Nucleotide Protein Genome Structure OMIM PMC Journals Books

SearchDatabase nameforSearch term

Advanced Search (beta)

Limits Preview/Index History Clipboard Details

Your browser version may not work well with NCBI's Web applications. More information here...

Display Show

All: 1

Review: 0

Click to change filter selection through MyNCBI.

1: Biochemistry. 2002 Mar 19;41(11):3596-604.

Related Articles, Links

NMR structure of the second intracellular loop of the alpha 2A adrenergic receptor: evidence for a novel cytoplasmic helix.

Chung DA, Zuiderweg ER, Fowler CB, Soyer OS, Mosberg HI, Neubig RR.

Biophysics Research Division and Department of Pharmacology, The University of Michigan, Ann Arbor, Michigan 48109, USA.

A major, unresolved question in signal transduction by G protein coupled receptors (GPCRs) is to understand how, at atomic resolution, a GPCR activates a G protein. A step toward answering this question was made with the determination of the high-resolution structure of rhodopsin; we now know the intramolecular interactions that characterize the resting conformation of a GPCR. To what degree does this structure represent a structural paradigm for other GPCRs, especially at the cytoplasmic surface where GPCR-G protein interaction occurs and where the sequence homology is low among GPCRs? To address this question, we performed NMR studies on approximately 35-residue-long peptides including the critical second intracellular loop (i2) of the alpha 2A adrenergic receptor (AR) and of rhodopsin. To stabilize the secondary structure of the peptide termini, 4-12 residues from the adjacent transmembrane helices were included and structures determined in dodecylphosphocholine micelles. We also characterized the effects on an alpha 2A AR peptide of a D130I mutation in the conserved DRY motif. Our results show that in contrast to the L-shaped loop in the i2 of rhodopsin, the i2 of the alpha 2A AR is predominantly helical, supporting the hypothesis that there is structural diversity within GPCR intracellular loops. The D130I mutation subtly modulates the helical structure. The spacing of nonpolar residues in i2 with helical periodicity is a predictor of helical versus loop structure. These data should lead to more accurate models of the intracellular surface of GPCRs and of receptor-mediated G protein activation.

Publication Types:

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

PMID: 11888275 [PubMed - indexed for MEDLINE]

Display Show

You are viewing a mobilized version of this site...
View original page here

Entrez PubMed

PubMed Services

Related Resources