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« Previous Abstract"Effects of nucleotide binding fold mutations on STE6, a yeast ABC protein"    Next AbstractGenetic screens and selections for cell and nuclear fusion mutants »

Mol Biol Cell


Title:"Metabolic instability and constitutive endocytosis of STE6, the a-factor transporter of Saccharomyces cerevisiae"
Author(s):Berkower C; Loayza D; Michaelis S;
Address:"Department of Cell Biology and Anatomy, Johns Hopkins University School of Medicine, Baltimore, MD 21205"
Journal Title:Mol Biol Cell
Year:1994
Volume:5
Issue:11
Page Number:1185 - 1198
DOI: 10.1091/mbc.5.11.1185
ISSN/ISBN:1059-1524 (Print) 1059-1524 (Linking)
Abstract:"STE6, a member of the ATP binding cassette (ABC) transporter superfamily, is a membrane protein required for the export of the a-factor mating pheromone in Saccharomyces cerevisiae. To initiate a study of the intracellular trafficking of STE6, we have examined its half-life and localization. We report here that STE6 is metabolically unstable in a wild-type strain, and that this instability is blocked in a pep4 mutant, suggesting that degradation of STE6 occurs in the vacuole and is dependent upon vacuolar proteases. In agreement with a model whereby STE6 is routed to the vacuole via endocytosis from the plasma membrane, we show that degradation of STE6 is substantially reduced at nonpermissive temperature in mutants defective in delivery of proteins to the plasma membrane (sec6) or in endocytosis (end3 and end4). Whereas STE6 appears to undergo constitutive internalization from the plasma membrane, as do the pheromone receptors STE2 and STE3, we show that two other proteins, the plasma membrane ATPase (PMA1) and the general amino acid permease (GAP1), are significantly more stable than STE6, indicating that rapid turnover in the vacuole is not a fate common to all plasma membrane proteins in yeast. Investigation of STE6 partial molecules (half- and quarter-molecules) indicates that both halves of STE6 contain sufficient information to mediate internalization. Examination of STE6 localization by indirect immunofluorescence indicates that STE6 is found in a punctate, possibly vesicular, intracellular pattern, distinct from the rim-staining pattern characteristic of PMA1. The punctate pattern is consistent with the view that most of the STE6 molecules present in a cell at any given moment could be en route either to or from the plasma membrane. In a pep4 mutant, STE6 is concentrated in the vacuole, providing further evidence that the vacuole is the site of STE6 degradation, while in an end4 mutant STE6 exhibits rim-staining, indicating that it can accumulate in the plasma membrane when internalization is blocked. Taken together, the results presented here suggest that STE6 first travels to the plasma membrane and subsequently undergoes endocytosis and degradation in the vacuole, with perhaps only a transient residence at the plasma membrane; an alternative model, in which STE6 circumvents the plasma membrane, is also discussed"
Keywords:ATP-Binding Cassette Transporters/genetics/*metabolism Amino Acid Transport Systems Base Sequence Cell Membrane/metabolism Endocytosis/genetics/*physiology Endopeptidases/metabolism Fungal Proteins/genetics/*metabolism *Glycoproteins Mating Factor Membran;
Notes:"MedlineBerkower, C Loayza, D Michaelis, S eng GM41223/GM/NIGMS NIH HHS/ Research Support, Non-U.S. Gov't Research Support, U.S. Gov't, P.H.S. 1994/11/01 Mol Biol Cell. 1994 Nov; 5(11):1185-98. doi: 10.1091/mbc.5.11.1185"

 
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