Literature DB >> 10825201

The CaaX proteases, Afc1p and Rce1p, have overlapping but distinct substrate specificities.

C E Trueblood1, V L Boyartchuk, E A Picologlou, D Rozema, C D Poulter, J Rine.   

Abstract

Many proteins that contain a carboxyl-terminal CaaX sequence motif, including Ras and yeast a-factor, undergo a series of sequential posttranslational processing steps. Following the initial prenylation of the cysteine, the three C-terminal amino acids are proteolytically removed, and the newly formed prenylcysteine is carboxymethylated. The specific amino acids that comprise the CaaX sequence influence whether the protein can be prenylated and proteolyzed. In this study, we evaluated processing of a-factor variants with all possible single amino acid substitutions at either the a(1), the a(2), or the X position of the a-factor Ca(1)a(2)X sequence, CVIA. The substrate specificity of the two known yeast CaaX proteases, Afc1p and Rce1p, was investigated in vivo. Both Afc1p and Rce1p were able to proteolyze a-factor with A, V, L, I, C, or M at the a(1) position, V, L, I, C, or M at the a(2) position, or any amino acid at the X position that was acceptable for prenylation of the cysteine. Eight additional a-factor variants with a(1) substitutions were proteolyzed by Rce1p but not by Afc1p. In contrast, Afc1p was able to proteolyze additional a-factor variants that Rce1p may not be able to proteolyze. In vitro assays indicated that farnesylation was compromised or undetectable for 11 a-factor variants that produced no detectable halo in the wild-type AFC1 RCE1 strain. The isolation of mutations in RCE1 that improved proteolysis of a-factor-CAMQ, indicated that amino acid substitutions E139K, F189L, and Q201R in Rce1p affected its substrate specificity.

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Year:  2000        PMID: 10825201      PMCID: PMC85805          DOI: 10.1128/MCB.20.12.4381-4392.2000

Source DB:  PubMed          Journal:  Mol Cell Biol        ISSN: 0270-7306            Impact factor:   4.272


  46 in total

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2.  Endoproteolytic processing of a farnesylated peptide in vitro.

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Journal:  Proc Natl Acad Sci U S A       Date:  1992-05-15       Impact factor: 11.205

3.  Proteolytic processing of farnesylated peptides: assay and partial purification from pig brain membranes of an endopeptidase which has the characteristics of E.C. 3.4.24.15.

Authors:  T N Akopyan; Y Couedel; M Orlowski; M C Fournie-Zaluski; B P Roques
Journal:  Biochem Biophys Res Commun       Date:  1994-01-28       Impact factor: 3.575

4.  Consequences of altered isoprenylation targets on a-factor export and bioactivity.

Authors:  G A Caldwell; S H Wang; F Naider; J M Becker
Journal:  Proc Natl Acad Sci U S A       Date:  1994-02-15       Impact factor: 11.205

5.  Genetic evidence for in vivo cross-specificity of the CaaX-box protein prenyltransferases farnesyltransferase and geranylgeranyltransferase-I in Saccharomyces cerevisiae.

Authors:  C E Trueblood; Y Ohya; J Rine
Journal:  Mol Cell Biol       Date:  1993-07       Impact factor: 4.272

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Journal:  Proc Natl Acad Sci U S A       Date:  1992-10-15       Impact factor: 11.205

9.  Inhibitors of the isoprenylated protein endoprotease.

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Authors:  J F Hancock; A Hall
Journal:  EMBO J       Date:  1993-05       Impact factor: 11.598

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2.  Saccharomyces cerevisiae a-factor mutants reveal residues critical for processing, activity, and export.

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Review 3.  Therapeutic intervention based on protein prenylation and associated modifications.

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6.  Ste24p Mediates Proteolysis of Both Isoprenylated and Non-prenylated Oligopeptides.

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Review 7.  Biogenesis of the Saccharomyces cerevisiae pheromone a-factor, from yeast mating to human disease.

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8.  Structure of the integral membrane protein CAAX protease Ste24p.

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10.  A combination of metabolic labeling and 2D-DIGE analysis in response to a farnesyltransferase inhibitor facilitates the discovery of new prenylated proteins.

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