Fur4 mediated uracil-scavenging to screen for surface protein regulators

Paine, Katherine M.; Ecclestone, Gabrielle B; MacDonald, Chris

doi:10.1101/2021.05.27.445995

Cited by 6 publications

(3 citation statements)

References 54 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…To assess if these bud neck crowding events correlate with organelle inheritance, we used time lapse microscopy to follow the inheritance of the vacuole, which is conveniently both a large organelle that is inherited early in the budding process ( Li et al, 2021a ). Using a mNeonGreen tagged version of the uracil permease Fur4, which localises to the plasma membrane and also the vacuolar lumen ( Paine et al, 2021 ), we could track inheritance over time ( Supplemental Video 3 ). We also labelled the vacuole by performing a pulse-chase with media containing the red-fluorescent dye FM4-64 ( Vida & Emr, 1995 ).…”

Section: Resultsmentioning

confidence: 99%

Investigating molecular crowding during cell division and hyperosmotic stress in budding yeast with FRET

Lecinski

Shepherd

Frame

et al. 2021

New Methods and Sensors for Membrane and Cell Volume Research

Self Cite

View full text Add to dashboard Cite

Cell division, aging, and stress recovery triggers spatial reorganization of cellular components in the cytoplasm, including membrane bound organelles, with molecular changes in their compositions and structures. However, it is not clear how these events are coordinated and how they integrate with regulation of molecular crowding. We use the budding yeast Saccharomyces cerevisiae as a model system to study these questions using recent progress in optical fluorescence microscopy and crowding sensing probe technology. We used a Förster Resonance Energy Transfer (FRET) based sensor, illuminated by confocal microscopy for high throughput analyses and Slimfield microscopy for single-molecule resolution, to quantify molecular crowding. We determine crowding in response to cellular growth of both mother and daughter cells, in addition to osmotic stress, and reveal hot spots of crowding across the bud neck in the burgeoning daughter cell. This crowding might be rationalized by the packing of inherited material, like the vacuole, from mother cells. We discuss recent advances in understanding the role of crowding in cellular regulation and key current challenges and conclude by presenting our recent advances in optimizing FRET-based measurements of crowding whilst simultaneously imaging a third color, which can be used as a marker that labels organelle membranes. Our approaches can be combined with synchronised cell populations to increase experimental throughput and correlate molecular crowding information with different stages in the cell cycle.

show abstract

Section: Resultsmentioning

confidence: 99%

Investigating molecular crowding during cell division and hyperosmotic stress in budding yeast with FRET

Lecinski

Shepherd

Frame

et al. 2021

New Methods and Sensors for Membrane and Cell Volume Research

Self Cite

View full text Add to dashboard Cite

show abstract

“…Tryptophan auxotroph ( trp1∆ ) yeast cells based on the SEY6210 background were grown to mid-log phase before being spotted out across a 10-fold serial dilution and grown on plates of replete (40 mg/liter) and two restricted (5 and 2.5 mg/liter) tryptophan concentrations. To quantify growth, densitometry was used to measure the growth intensity across different dilutions on the plate ( Paine et al, 2021 Preprint ). Yeast growth at each dilution was normalized to a WT control on the same plate, and the difference was plotted for indicated tryptophan concentrations.…”

Section: Methodsmentioning

confidence: 99%

Recycling of cell surface membrane proteins from yeast endosomes is regulated by ubiquitinated Ist1

Laidlaw

Calder

MacDonald

2022

Journal of Cell Biology

Self Cite

View full text Add to dashboard Cite

Upon internalization, many surface membrane proteins are recycled back to the plasma membrane. Although these endosomal trafficking pathways control surface protein activity, the precise regulatory features and division of labor between interconnected pathways are poorly defined. In yeast, we show recycling back to the surface occurs through distinct pathways. In addition to retrograde recycling pathways via the late Golgi, used by synaptobrevins and driven by cargo ubiquitination, we find nutrient transporter recycling bypasses the Golgi in a pathway driven by cargo deubiquitination. Nutrient transporters rapidly internalize to, and recycle from, endosomes marked by the ESCRT-III associated factor Ist1. This compartment serves as both “early” and “recycling” endosome. We show Ist1 is ubiquitinated and that this is required for proper endosomal recruitment and cargo recycling to the surface. Additionally, the essential ATPase Cdc48 and its adaptor Npl4 are required for recycling, potentially through regulation of ubiquitinated Ist1. This collectively suggests mechanistic features of recycling from endosomes to the plasma membrane are conserved.

show abstract

“…The physical interactome was acquired from YeastMine (Balakrishnan et al, 2012) Tat2 recycling assay Tryptophan auxotroph (trp1∆) yeast cells were grown to mid log-phase before being spotted out across a 10fold serial dilution and grown on plates of indicated Tryptophan concentrations. Yeast growth was normalised from a wild-type control on the same plate and used the calculate the growth difference, as previously described (Paine et al, 2021).…”

Section: Bioinformaticsmentioning

confidence: 99%

Recycling of cell surface membrane proteins from yeast endosomes is regulated by ubiquitinated Ist1

Laidlaw

Calder

MacDonald

2021

Preprint

Self Cite

View full text Add to dashboard Cite

Trafficking of cell surface membrane proteins through a dynamic network of endomembrane compartments ensures correct cellular function. Upon internalisation, many surface proteins are either degraded or recycled back to the plasma membrane. Although these pathways control many biological processes, the precise regulatory features and division of labour between interconnected pathways is unclear. Using the budding yeast Saccharomyces cerevisiae, our work suggests retrograde recycling via the trans-Golgi Network (TGN) of cargoes like yeast synaptobrevins (Snc1 / Snc2), that rely on cargo ubiquitination, is distinct from endosomal trafficking of nutrient transporters. We provide evidence that nutrient transporters internalise to, and upon deubiquitination recycle from, endosomes marked by Vps4 and Ist1. A genetic screen for this recycling pathway previously implicated the ESCRT-III associated factor Ist1, suggesting Ist1 functionally defines yeast recycling endosomes. We demonstrate Ist1 ubiquitination affects its endosomal recruitment and ability to promote recycling. Finally, we reveal the ubiquitin-binding adaptor Npl4 and the essential ATPase Cdc48 are also involved in recycling. Our work suggests features of endosomal recycling are evolutionarily conserved.

show abstract

Fur4 mediated uracil-scavenging to screen for surface protein regulators

Cited by 6 publications

References 54 publications

Investigating molecular crowding during cell division and hyperosmotic stress in budding yeast with FRET

Investigating molecular crowding during cell division and hyperosmotic stress in budding yeast with FRET

Recycling of cell surface membrane proteins from yeast endosomes is regulated by ubiquitinated Ist1

Recycling of cell surface membrane proteins from yeast endosomes is regulated by ubiquitinated Ist1

Contact Info

Product

Resources

About