AI Article Synopsis

  • G protein-coupled receptors (GPCRs) are crucial signaling molecules involved in many physiological processes, with rhodopsin being the only one for which crystal structures are known.
  • Researchers used atomic force microscopy to study the organization of rhodopsin in native mouse photoreceptor membranes, showing that rhodopsin and opsin form structural dimers in a paracrystalline arrangement.
  • The study provides a semi-empirical model of GPCR structure in native membranes, revealing how rhodopsin interacts with other proteins through specific helix contacts.

Article Abstract

G protein-coupled receptors (GPCRs), which constitute the largest and structurally best conserved family of signaling molecules, are involved in virtually all physiological processes. Crystal structures are available only for the detergent-solubilized light receptor rhodopsin. In addition, this receptor is the only GPCR for which the presumed higher order oligomeric state in native membranes has been demonstrated (Fotiadis, D., Liang, Y., Filipek, S., Saperstein, D. A., Engel, A., and Palczewski, K. (2003) Nature 421, 127-128). Here, we have determined by atomic force microscopy the organization of rhodopsin in native membranes obtained from wild-type mouse photoreceptors and opsin isolated from photoreceptors of Rpe65-/- mutant mice, which do not produce the chromophore 11-cis-retinal. The higher order organization of rhodopsin was present irrespective of the support on which the membranes were adsorbed for imaging. Rhodopsin and opsin form structural dimers that are organized in paracrystalline arrays. The intradimeric contact is likely to involve helices IV and V, whereas contacts mainly between helices I and II and the cytoplasmic loop connecting helices V and VI facilitate the formation of rhodopsin dimer rows. Contacts between rows are on the extracellular side and involve helix I. This is the first semi-empirical model of a higher order structure of a GPCR in native membranes, and it has profound implications for the understanding of how this receptor interacts with partner proteins.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC1360145PMC
http://dx.doi.org/10.1074/jbc.M302536200DOI Listing

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