Abstract
Selective endocytosis followed by degradation is a major mechanism for downregulating plasma membrane transporters in response to specific environmental cues. In Saccharomyces cerevisiae, this endocytosis is promoted by ubiquitylation catalyzed by the Rsp5 ubiquitin-ligase, targeted to transporters via adaptors of the alpha-arrestin family. However, the molecular mechanisms of this targeting and their control according to conditions remain incompletely understood. In this work, we dissect the molecular mechanisms eliciting the endocytosis of Can1, the arginine permease, in response to cycloheximide-induced TORC1 hyperactivation. We show that cycloheximide promotes Rsp5-dependent Can1 ubiquitylation and endocytosis in a manner dependent on the Bul1/2 alpha-arrestins. Also crucial for this downregulation is a short acidic patch sequence in the N-terminus of Can1 likely acting as a binding site for Bul1/2. The previously reported inhibition by cycloheximide of transporter recycling, from the trans-Golgi network to the plasma membrane, seems to additionally contribute to efficient Can1 downregulation. Our results also indicate that, contrary to the previously described substrate-transport elicited Can1 endocytosis mediated by the Art1 alpha-arrestin, Bul1/2-mediated Can1 ubiquitylation occurs independently of the conformation of the transporter. This study provides further insights into how distinct alpha-arrestins control the ubiquitin-dependent downregulation of a specific amino acid transporter under different conditions.
Highlights
Microbial Molecular Genetics Laboratory, Institute of Biosciences and Applications, National Centre for Scientific Research “Demokritos”, Patr
In the absence of Can1 substrates in the medium, CHXinduced ubiquitylation, endocytosis, and vacuolar sorting of Can1 are mediated solely by the TORC1-activated Bul1/2 adaptors acting through the Bul1/2 their binding site since (Bul-BS) at the N-terminus of the transporter
In order to study the effect of cycloheximide (CHX) on Can1 molecules solely present at the plasma membrane and not at internal compartments, we expressed wt and mutant
Summary
Grigoriou E & 27 Neapoleos St., 15341 Agia Paraskevi, Greece; Molecular Physiology of the Cell Laboratory, Université Libre de Bruxelles (ULB), IBMM, 6041 Gosselies, Abstract: Selective endocytosis followed by degradation is a major mechanism for downregulating plasma membrane transporters in response to specific environmental cues. In Saccharomyces cerevisiae, this endocytosis is promoted by ubiquitylation catalyzed by the Rsp ubiquitin-ligase, targeted to transporters via adaptors of the alpha-arrestin family. We dissect the molecular mechanisms eliciting the endocytosis of Can, the arginine permease, in response to cycloheximide-induced TORC1 hyperactivation. Rsp5-dependent Can ubiquitylation and endocytosis in a manner dependent on the Bul1/2 alphaarrestins. Crucial for this downregulation is a short acidic patch sequence in the N-terminus of. Transporters are very often subject to tight control, as initially illustrated by regulation of LacY cell-surface expression via transcriptional control of the lac operon [2]
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