Journal Article10.1111/J.1600-0854.2004.00168.X
The internalization of yeast Ste6p follows an ordered series of events involving phosphorylation, ubiquitination, recognition and endocytosis.
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TL;DR: The results demonstrate that Ste6p follows the PURE pathway and that GFP‐tagged Ste 6p provides a powerful model protein for studies of endocytosis and post‐endocytic events in yeast.
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Abstract: A general pathway for the internalization of plasma membrane proteins that involves phosphorylation, ubiquitination, recognition and endocytosis has recently emerged from multiple studies in yeast. We refer to this series of events as the PURE pathway. Here we investigate whether the yeast a-factor transporter Ste6p, an ATP-binding cassette protein, utilizes the PURE pathway. Deletion of a 52-amino acid sequence (the ‘A box’) within the linker region of Ste6p has previously been shown to block ubiquitination and endocytosis (Kolling R, Losko S. EMBO J 1997; 16:2251-2261). Using wild-type and mutant forms of GFP-tagged Ste6p, we identified two residues (T613 and S623) within the A box as likely sites of Ste6p phosphorylation important for internalization. Mutation of these residues to alanine blocked ubiquitination and endocytosis of Ste6p, similar to the effect of deleting the entire A box, while substitution with glutamic acid (to mimic phosphorylation) suppressed the ubiquitination and endocytic defects. Importantly, a translational fusion of monoubiquitin to the C-terminus of Ste6p-T613A, S623A or Ste6p-ΔA restored endocytosis, providing strong evidence that the role of phosphorylation is to direct ubiquitination, which in turn is a critical signal for Ste6p internalization. We also identified multiple (five) lysine residues in the linker that are important for Ste6p ubiquitination. Our results demonstrate that Ste6p follows the PURE pathway and that GFP-tagged Ste6p provides a powerful model protein for studies of endocytosis and post-endocytic events in yeast.
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Citations
ABC Transporters in Saccharomyces cerevisiae and Their Interactors: New Technology Advances the Biology of the ABCC (MRP) Subfamily
TL;DR: a revised unified nomenclature for the six yeast ABC subfamilies is proposed to reflect the current mammalian designations ABCA to ABCG, and iMYTH technology has successfully identified novel interactors of Ycf1p and promises to be an invaluable tool in future efforts to comprehensively define the yeast ABC interactome.
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Negative regulation of the yeast ABC transporter Ycf1p by phosphorylation within its N-terminal extension.
TL;DR: Evidence is provided that negative, as well as positive, regulation of Ycf1p is mediated by phosphorylation, and two kinase genes are identified, CKA1 and HAL5, deletion of which increases YCF1p function.
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Local Pheromone Release from Dynamic Polarity Sites Underlies Cell-Cell Pairing during Yeast Mating.
Laura Merlini,Bita Khalili,Felipe O. Bendezú,Daniel Hurwitz,Daniel Hurwitz,Vincent Vincenzetti,Dimitrios Vavylonis,Sophie G. Martin +7 more
TL;DR: It is proposed that efficient cell pairing relies on fluctuating local signal emission and perception, which become locked into place through stimulation, which leads to efficient pair formation.
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Phosphorylation and ubiquitination are necessary for Na,K-ATPase endocytosis during hypoxia.
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TL;DR: Evidence that ubiquitination plays an important role in cellular adaptation to hypoxia by regulating Na,K-ATPase alpha(1)-subunit endocytosis is provided.
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A survey of all 11 ABC transporters in fission yeast: two novel ABC transporters are required for red pigment accumulation in a Schizosaccharomyces pombe adenine biosynthetic mutant.
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