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Mechanism of farnesylated CAAX protein processing by the intramembrane protease Rce1. | LitMetric

AI Article Synopsis

  • CAAX proteins are crucial for various cellular processes, including growth and cancer development, and involve around 120 mammalian proteins that interact with cell membranes.
  • The localization of these proteins is managed through post-translational modifications of their CAAX motifs, which entails several steps like prenylation and cleavage, primarily facilitated by the enzyme Rce1.
  • Research reveals the crystal structure of a Rce1 homologue, shedding light on its unique membrane structure and how it interacts with farnesylated peptides, leading to the hypothesis that Rce1 may be the pioneer of a new family of intramembrane proteases.

Article Abstract

CAAX proteins have essential roles in multiple signalling pathways, controlling processes such as proliferation, differentiation and carcinogenesis. The ∼120 mammalian CAAX proteins function at cellular membranes and include the Ras superfamily of small GTPases, nuclear lamins, the γ-subunit of heterotrimeric GTPases, and several protein kinases and phosphatases. The proper localization of CAAX proteins to cell membranes is orchestrated by a series of post-translational modifications of the carboxy-terminal CAAX motifs (where C is cysteine, A is an aliphatic amino acid and X is any amino acid). These reactions involve prenylation of the cysteine residue, cleavage at the AAX tripeptide and methylation of the carboxyl-prenylated cysteine residue. The major CAAX protease activity is mediated by Rce1 (Ras and a-factor converting enzyme 1), an intramembrane protease (IMP) of the endoplasmic reticulum. Information on the architecture and proteolytic mechanism of Rce1 has been lacking. Here we report the crystal structure of a Methanococcus maripaludis homologue of Rce1, whose endopeptidase specificity for farnesylated peptides mimics that of eukaryotic Rce1. Its structure, comprising eight transmembrane α-helices, and catalytic site are distinct from those of other IMPs. The catalytic residues are located ∼10 Å into the membrane and are exposed to the cytoplasm and membrane through a conical cavity that accommodates the prenylated CAAX substrate. We propose that the farnesyl lipid binds to a site at the opening of two transmembrane α-helices, which results in the scissile bond being positioned adjacent to a glutamate-activated nucleophilic water molecule. This study suggests that Rce1 is the founding member of a novel IMP family, the glutamate IMPs.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3864837PMC
http://dx.doi.org/10.1038/nature12754DOI Listing

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