Remodelling of Nucleus-Vacuole Junctions During Metabolic and Proteostatic Stress

Abstract

Cellular adaptation to stress and metabolic cues requires a coordinated response of different intracellular compartments, separated by semipermeable membranes. One way to facilitate interorganellar communication is via membrane contact sites, physical bridges between opposing organellar membranes formed by an array of tethering machineries. These contact sites are highly dynamic and establish an interconnected organellar network able to quickly respond to external and internal stress by changing size, abundance and molecular architecture. Here, we discuss recent work on nucleus-vacuole junctions, connecting yeast vacuoles with the nucleus. Appearing as small, single foci in mitotic cells, these contacts expand into one enlarged patch upon nutrient exhaustion and entry into quiescence or can be shaped into multiple large foci essential to sustain viability upon proteostatic stress at the nuclear envelope. We highlight the remarkable plasticity and rapid remodelling of these contact sites upon metabolic or proteostatic stress and their emerging importance for cellular fitness.

Keywords

glucose metabolism NVJ Snd3 stress response quiescence

Introduction

Adaptation to changing environments is key to maintaining cellular and organismal survival. For microbial cells, evolutionary success depends on their ability to sense and rapidly adapt to fluctuating availability of nutrients or exposure to stress. Cellular metabolism needs to be adjusted to allow growth and division in times of plenty and to sustain homeostasis and stress response when nutrients are limiting (Zhang and Cao, 2017). Optimal resource allocation requires sensing and signalling of extracellular conditions and a subsequent metabolic rewiring and cellular remodelling to adjust organellar functions. Direct physical contact between distinct organelles at membrane contact sites is thought to play a key role in the intracellular relay of biochemical information (Gatta and Levine, 2017). These sites serve as metabolic hubs and rapidly change size and abundance in response to various types of external and internal cues, thereby optimizing and fine-tuning organellar function to respective cellular needs. Contact sites allow the transfer of information in form of ions, lipids or small metabolites between distinct cellular subcompartments, thus providing a connection between spatially separated biochemical reactions within each organellar microenvironment (Xu and Huang, 2020). In cooperation with classical signalling pathways and vesicular transport, this form of interorganellar communication links the metabolic activities in different organelles to guarantee overall cellular homeostasis. Bridging of different organellar membranes at contact sites is established by specialized tethering machineries that shape the different contacts via protein-protein or protein-lipid interaction and serve to recruit and position additional proteins to tailor contact function or enforce contact formation (Eisenberg-Bord et al., 2016; Scorrano et al., 2019). Sites of contact have been reported across the eukaryotic kingdom and between virtually all organelles, with functions ranging from lipid flux and organelle fission to the involvement in degradative pathways like autophagy (Eisenberg-Bord et al., 2016; Levine and Patel, 2016; Gatta and Levine, 2017; Kohler et al., 2020). While being able to rigidly tether two opposing membranes, contact sites have also been shown to dynamically change in size, abundance and molecular composition in response to a variety of external and internal cues. Despite extensive research on the dynamic aspects of contact sites (Eisenberg-Bord et al., 2016; Nettebrock and Bohnert, 2019; Scorrano et al., 2019; Bohnert, 2020; Prinz et al., 2020), the signalling events triggering this remodelling are far from being understood. Reshaping of contact sites often occurs simultaneously at several organellar contact zones and includes the relocalization of distinct proteins from one site to another, supporting the notion that these contacts form a coordinated network able to collectively respond to specific stimuli (Hönscher et al., 2014; Elbaz-Alon et al., 2015; Bean et al., 2018; Hariri et al., 2018; Bohnert, 2019; Prinz et al., 2020).

The Making and Shaping of Nucleus-Vacuole Junctions

The budding yeast Saccharomyces cerevisiae represents a prime model organism for studies on the molecular architecture of contact sites and their regulation and multifaceted functions. Several processes and proteins associated with different contacts have been first described in yeast, followed by the identification of the mammalian counterparts (Elbaz-Alon et al., 2014; Hönscher et al., 2014; Hönscher and Ungermann, 2014; Eden, 2016; Malia and Ungermann, 2016; Wong et al., 2018). The first contact sites discovered in yeast are the nucleus-vacuole junctions (NVJs), connecting the vacuole with the perinuclear endoplasmic reticulum (ER) and thus the nuclear envelope (Pan et al., 2000). A few years ago, a potential equivalent in mammalian cells was described, tethering the ER to endosomes (Hönscher and Ungermann, 2014; Eden, 2016). Some NVJ-associated proteins find their counterparts in this mammalian membrane contact site and distinct functions are indeed conserved, in particular lipid transfer. Still, contacts between the ER and the endolysosomal system in higher eukaryotes are more complex than yeast NVJs, both in respect to structure and function. The extent of organellar contact as well as the tethering proteins that compose the contact site seem highly dependent on the state of endosomal maturation, and functions of these contact sites range from positioning, movement and fission of endosomes to the modulation of receptor signalling (Di Mattia et al., 2020).

The size and appearance of NVJs can range from small foci to large patches, establishing highly dynamic zones of organellar proximity between the ER as the key compartment for lipid synthesis and the vacuole as cellular waste bin, recycling facility and storage depot. Accumulating evidence places NVJs at the centre stage of lipid metabolism: these junctions recruit an array of proteins involved in different aspects of lipid metabolism and transport, and serve as a platform for lipid droplet (LD) biogenesis under stress (Pan et al., 2000; Jeong et al., 2017; Hariri et al., 2018).

The interaction between the principle NVJ tethering pair, the perinuclear ER-resident protein Nvj1 and the palmitoylated protein Vac8 on the vacuolar membrane, represents a prerequisite for NVJ formation (Figure 1) (Pan et al., 2000). Nvj1 anchors its N-terminal domain to the inner nuclear membrane to span the ER lumen (Millen et al., 2008), and interaction with the Armadillo-domain protein Vac8 is facilitated via its C-terminus (Jeong et al., 2017). These tethers allow the recruitment of additional contact components, mostly proteins involved in lipid metabolism. This includes the oxysterol-binding protein Osh1, associating with cytoplasmic parts of Nvj1 via its ankyrin domain, and the enoyl-CoA reductase Tsc13, an essential component of the fatty acid elongation machinery localized in the ER membrane, which contacts Nvj1 via its transmembrane domain (Kohlwein et al., 2001; Levine and Munro, 2001; Kvam and Goldfarb, 2004; Kvam et al., 2005; Jeong et al., 2017; Manik et al., 2017). Nvj2, one of seven SMP-proteins in yeast, all of which localize to membrane contact sites, is a lipid-binding protein with a role in ceramide metabolism (Liu et al., 2017; Tamura et al., 2019). Nvj2 was found to prominently enrich at NVJs in late-logarithmic growth but seems to partly dissociate when cells enter stationary phase (Toulmay and Prinz, 2012). The integral ER-protein Mdm1 contacts the vacuole at the junctions via its lipid-binding PX-domain, thereby acting as an additional tether, and promotes LD biogenesis via localized fatty acid activation (Hariri et al., 2016, 2018). Interestingly, Mdm1 as well as its paralogue Nvj3 are targeted to the junctions independently of the main tether protein Nvj1 to establish organellar proximity (Henne et al., 2015), while for instance Osh1 and Tsc13 are recruited to the NVJs via Nvj1. The sterol-transfer protein Lam6 requires Vac8 to localize to the junctions, where it mediates the formation of sterol-enriched lipid microdomains on the vacuolar membrane upon glucose limitation and facilitates contact expansion (Elbaz-Alon et al., 2015; Murley et al., 2015). Vps13, a peripheral membrane protein that is enriched at the contacts between ER and vacuole under respiratory conditions, is involved in phospholipid transport (Lang et al., 2015; Park et al., 2016; Bean et al., 2018). Both yeast and mammalian Vps13 localize to and coordinate the size of several other contact sites, most likely due to altered lipid distribution, and only transiently associate with NVJs and ER-endosomal contacts, respectively (Lang et al., 2015; Park et al., 2016; Rzepnikowska et al., 2017a, 2017b; Bean et al., 2018; Gao and Yang, 2018). Though orthologues of several NVJ-associated proteins involved in lipid metabolism, such as Vps13, Mdm1, Nvj2, and Osh1, are present in higher eukaryotes, counterparts of the main tethering pair Nvj1-Vac8 have been only identified in other fungi (Millen et al., 2008; Beh et al., 2012; Toulmay and Prinz, 2012; Helle et al., 2013; Manik et al., 2017; Rzepnikowska et al., 2017b; Garapati and Mishra, 2018; Singh et al., 2020). Thus, especially membrane contact site-situated effector proteins involved in lipid metabolism seem to be conserved over species boundaries, as elaborated in several excellent reviews (Eden, 2016; Henne, 2017; Scorrano et al., 2019; Bohnert, 2020; Di Mattia et al., 2020), while principle structural tethers seem to vary substantially.

Figure 1.

Overview of nucleus-vacuole junctions. A: The main tethering pair of NVJs (dark blue), alternative tethers (mid blue), accessory proteins involved in lipid metabolism (light blue) and regulatory proteins (red) are depicted and their main function is given. Please note that orientations and domain borders are represented according to predictions, but relative protein size and structure are not true to scale. B: Schematic representation of main NVJ components. Protein sizes are true to scale with breaks of 100 amino acids, where necessary. Transmembrane domains (red) and specific domains (dark blue) are highlighted. Protein regions facing the cytosol are shaded in light blue, those towards the ER lumen are highlighted in yellow. Sig.P. = signal peptide; φ = hydrophobic region; PXA = Phox-associated; LD = lipid droplet; RGS = regulator of G protein signalling; PX = Phox; CN = C-terminal nexin; PH = pleckstrin homology; SMP = synaptogamin-like-mitochondrial-lipid binding protein; StARkin = domain closely resembling StART (steroidogenic acute regulatory protein-related lipid-transfer) domain; ANK = ankyrin; OBD = oxysterol-binding domain; NC = N–terminal chorein domain; SHR BD = SHORT_ROOT transcription factor binding domain; APT1 = aberrant pollen transmission 1 protein; ATG_C = Autophagy-related protein C-terminal domain. Information regarding domain borders were taken from respective literature, Uniprot and SGD (Kohlwein et al., 2001; Toulmay and Prinz 2012; Henne et al., 2015; Murley et al., 2015; Jeong et al., 2017; Manik et al., 2017; Rzepnikowska et al., 2017a, 2017b; Dziurdzik et al., 2018; Tosal-Castano et al., 2021).

While these additional NVJ residents regulate NVJ dynamics, plasticity and function, and are enriched at these contact zones under specific conditions, they are not required for contact formation per se. In our recent work, we identified the integral ER protein Snd3 as a novel component of NVJs (Figure 1) and show that this protein is crucial to establish NVJs (Tosal-Castano et al., 2021). We demonstrate that Snd3 interacts with and stabilizes Nvj1 once it is inserted into the ER membrane. In absence of Snd3, Nvj1 is rapidly removed from the ER via ER-associated degradation (ERAD). As the topology of Nvj1 is rather unique, spanning both membranes of the nuclear envelope (Millen et al., 2008), stabilization of this protein by Snd3 is required to preclude premature retro-translocation and proteasomal degradation via ERAD (Tosal-Castano et al., 2021). After successful insertion of Nvj1 into the nuclear envelope, primordial NVJs are formed via interaction between the main tethering pair Vac8 and Nvj1, followed by recruitment of other NVJ-associated proteins (Kohlwein et al., 2001; Levine and Munro, 2001; Kvam and Goldfarb, 2004; Kvam et al., 2005). Upon glucose exhaustion or during respiratory growth on glycerol, Snd3 itself is targeted to the NVJs, facilitating contact site expansion (Tosal-Castano et al., 2021). While more and more proteins are being identified to decorate the NVJs, a comprehensive analysis of the NVJ proteome under different metabolic regimes is still lacking.

NVJ Expansion Upon Glucose Exhaustion and Entry Into Quiescence

Upon entry into stationary phase or in response to stress, NVJ size increases, and the small NVJ foci visible at the interface between the nucleus and the vacuole grow into large, expanded patches (Pan et al., 2000; Kohlwein et al., 2001; Levine and Munro, 2001; Hariri et al., 2018). Along this line, we could show that glucose exhaustion triggers NVJ expansion and recruitment of Snd3 as additional contact site resident (Figure 2A). When cells rapidly divide in high glucose, Snd3 is evenly distributed throughout the ER but already essentially contributes to the formation of primordial NVJs via stabilisation of the main tether Nvj1 once it is translocated. As soon as glucose becomes limiting, Snd3 is targeted to the junctions, which coincides with the enrichment of Nvj1 and massive NVJ expansion. Vice versa, glucose re-addition to glucose-starved cells triggers the rapid dissociation of Snd3 from the junctions, followed by the slow disassembly of these contacts (Tosal-Castano et al., 2021). We further show that recruitment of Snd3 to the junctions and concomitant NVJ expansion is controlled by central glucose signalling pathways, establishing a link between metabolic rewiring and contact site dynamics (Figure 2A). The protein kinase A (PKA) as well as the AMP-dependent kinase Snf1 represent two evolutionary conserved branches of the metabolic signalling network, activated in response to high glucose or glucose depletion, respectively (Hedbacker and Carlson, 2008; Zhang and Cao, 2017; Stasyk and Stasyk, 2019). Mimicking the presence of glucose via (i) genetic inactivation of the inhibitory subunit of PKA, resulting in hyperactive PKA signalling, or (ii) disruption of AMP-dependent Snf1 signalling, prevented Snd3 targeting to and Nvj1 enrichment at the contact sites despite glucose depletion (Tosal-Castano et al., 2021).

Figure 2.

NVJ expansion upon glucose depletion and entry into quiescence. A: The ER-protein Snd3 both enriches at and governs the expansion of the nucleus-vacuole junctions (NVJs) when yeast cells grow into glucose exhaustion, a process regulated by central glucose signalling pathways. Upon glucose replenishment, Snd3 quickly redistributes along the perinuclear ER, followed by a slower disassembly of NVJs. B: Expansion of NVJs is a robust predictor of cell fate, when yeast cells acutely starved for glucose face quiescence versus senescence decisions. In a clonal population, cells that efficiently expand the NVJs upon acute starvation and cell cycle arrest are more likely to enter quiescence, defined as the ability to re-enter the cell cycle when glucose is replenished again. Vice versa, cells becoming senescent are less likely to show this contact site expansion during acute glucose removal. For details, please see main text. PKA = protein kinase A; N = nucleus; V = vacuole.

In response to glucose exhaustion, cells exit the cell cycle and enter quiescence, a non-proliferative state with rather heterogenous properties associated with high stress resistance and longevity. Entry into quiescence has been shown to be accompanied by a drastic remodelling of distinct organelles and cellular structures (Sagot and Laporte, 2019). Recent work from Wood et al. demonstrates that this organellar remodelling entails a prominent expansion of NVJs that serves as predictor of cell fate (Wood et al., 2020). Using abrupt restriction of glucose to force exit from cell cycle, the authors assessed biomarkers for nutrient signalling, interorganellar crosstalk, stress response and organelle homeostasis to predict quiescence versus senescence decisions of individual cells within an isogenic yeast population (Figure 2B) (Wood et al., 2020). In an elegant approach using multi-colour time-lapse imaging and automated single-cell analysis, they monitored protein-fluorophore chimeras, including Nvj1, throughout growth in high glucose, acute starvation for several hours and subsequent glucose replenishment. To maintain cellular viability upon abrupt starvation, cells need to quickly adapt by rewiring cellular homeostasis and exit cell cycle, which requires central metabolic signalling networks, including an inhibition of PKA signalling and the activation of the AMPK/Snf1 pathway (Zhang and Cao, 2017). Interestingly, Wood et al. discovered that a high abundance of the nutrient-signalling protein kinase Rim15 (Swinnen et al., 2006) prior to acute starvation is a strong indicator for successful entry into quiescence and thus the ability to regrow when glucose is replenished. In addition, Nvj1 as a marker for interorganellar connectivity turned out to be a strong predictor of cell fate. Cells within a clonal population that rapidly expanded NVJs during acute starvation were more likely to become quiescent, while senescent cells mostly lacked NVJ expansion. Still, the presence of Nvj1 was not required for entry into quiescence (Wood et al., 2020). Thus, even though NVJs seem to respond to signalling pathways coordinating the cellular path towards quiescence or senescence upon acute starvation, a distinct physiological role for Nvj1 in this process has not been identified yet. While indeed NVJ expansion might merely represent a phenotypic marker of quiescence, it is also feasible that for instance Mdm1, which was recently established as an alternative NVJ tether (Henne et al., 2015; Hariri et al., 2018), compensates for the absence of Nvj1, allowing the formation of organellar contact despite lack of the main tether.

NVJ Remodelling to Resolve Proteostatic Stress at the Nuclear Envelope

Expansion of the contact region between the nucleus and the vacuole is not limited to nutritional stress but also occurs upon exposure to other stresses, in particular ER stress (Hariri et al., 2018). Establishing physical contact between the ER and the vacuole as main catabolic compartment, the NVJs are in a prime position to contribute to quality control of the nuclear envelope. The degradation of damaged material of the perinuclear ER and nucleolar proteins at the NVJs via piecemeal microautophagy of the nucleus (PMN), a selective form of autophagic recycling, represents one of the best-characterized functions of these contact sites (Millen et al., 2009; Golam Mostofa et al., 2018; Otto and Thumm, 2021). Here, parts of the nuclear envelope invaginate into the vacuolar lumen and small vesicles are pinched off to be digested. In addition to a core set of autophagy-related (Atg) proteins required for final stages of PMN (Krick et al., 2008), also the lipid microenvironment at NVJs is suggested to contribute to PMN. Pinching off these bleb-like structures necessitates high membrane curvature, which is facilitated by incorporation of very-long chain fatty acids into phospholipids. Accordingly, insufficient fatty acid elongation compromises biogenesis of PMN vesicles (Kvam et al., 2005). Beyond this established role of NVJs during PMN and thus bulk removal of parts of the nuclear envelope, NVJs seems to be involved in another, more specific branch of protein quality control of the nucleus. Lord and Wente recently reported that the presence of NVJs was crucial to remove misassembled nuclear pore complexes (NPCs). Using mutants deficient in the assembly of NPCs, multi-subunit complexes composed of several nucleoporins that facilitate nucleocytoplasmic transport, the authors could show that NVJs are critical to sustain cellular fitness upon perturbation of NPC assembly (Figure 3) (Lord and Wente, 2020). In contrast to metazoans, yeast undergoes a closed mitosis, thus NPCs have to be inserted into the intact nuclear envelope during interphase in a complex process (Boettcher and Barral, 2013). As NPC assembly defects are observed in replicatively aged cells (Rempel et al., 2019), it might be interesting to test for a possible contribution of NVJs to the quality control of the nuclear envelope in old mother cells.

Figure 3.

NVJ expansion upon defective NPC assembly is required to sustain cellular fitness. Proteotoxic stress upon impaired nuclear pore complex (NPC) assembly in a nup116 mutant triggers NVJ reshaping, leading to increased contact formation and multiple, large NVJ foci. This alleviates NPC assembly perturbations and promotes viability. Survival upon genetic disruption of NPC assembly (nup116 mutant) requires NVJs, while under physiological conditions (wildtype) other cellular surveillance systems are in place to resolve the rare NPC assembly defects, rendering NVJs unnecessary for cellular viability. For details, please see main text. N = nucleus; V = vacuole.

Lord and Wente demonstrated that a mutant form of Nup116, a nucleoporin suggested to promote NPC biogenesis by stabilizing assembly intermediates (Onischenko et al., 2017), is defective in NPC assembly at elevated temperatures, resulting in clustered nucleoporin patches that are degraded in an autophagy-dependent manner to remodel the nuclear envelope (Lord and Wente, 2020). Proteostatic stress upon disturbed NPC assembly triggered a prominent reshaping of NVJs: while the regions of contact between the nuclear envelope and the vacuole increased, Nvj1 did not appear in a single, enlarged patch but rather in multiple foci, decorating contact sites with numerous small vacuoles. Interestingly, Snd3 (alias Pho88), which the authors used as a marker for the perinuclear ER, did not concentrate at these Nvj1-decorated foci upon perturbed NPC assembly. Thus, while remodelling and expansion of the contacts occurs upon nutritional and proteostatic stress, the molecular composition of these enlarged NVJs seems to differ.

Mdm1, which coordinates LD biogenesis at NVJs upon nutrient limitation (Hariri et al., 2018), decorated the multiple NVJs just as Nvj1 upon NPC misassembly. Increased Mdm1 recruitment coincided with a clustering of LDs around the contact zones. Interestingly, these remodelled NVJs cooperate with LDs to relieve proteostatic stress upon NPC misassembly and to maintain viability, and loss of either one compromised cellular fitness. As inactivation of LD biogenesis or NVJ formation did not affect the viability of unperturbed wildtype cells (Lord and Wente, 2020), other surveillance systems might be in place to deal with occasional disturbances of NPC assembly in physiological conditions (Thaller et al., 2019). In this line, NPCs and nucleoporins were shown to be degraded via selective autophagy in unperturbed wildtype cells without the need for NVJ assembly or functional PMN (Tomioka et al., 2020). However, upon mutation or additional stress that hamper NPC assembly, possibly overloading available proteostatic capacity under resting conditions, NVJs emerge as important factors to relieve nuclear envelope stress. As fully assembled NPCs are usually excluded from the nuclear envelope region establishing the NVJs (Severs et al., 1976; Pan et al., 2000; Roberts et al., 2003), direct PMN-mediated degradation seems rather unlikely. Still, impaired NPCs and in particular assembly intermediates could be direct cargo of PMN at NVJs. Alternatively, NVJs might serve an indirect role in the removal of misassembled NPCs, for instance via spatial organization of LDs, which contribute to the generation of specific lipid microenvironments and have been shown to assist in the removal of misfolded proteins to relief proteostatic stress.

Spatial Organisation of LDs at NVJs: A Contingency Route Upon Excessive Proteotoxic Stress?

Upon metabolic stress, NVJs serve as platforms for the organisation and biosynthesis of a specific LD subpopulation (Hariri et al., 2018). LDs bud off from the ER network and consist of a core of neutral lipids surrounded by a monolayer of phospholipids. These highly dynamic and versatile organelles function as lipid reservoirs to meet the cell’s requirements in times of nutrient limitation and to support the detoxification of excess fatty acids or harmful lipid species. Moreover, accumulating evidence points towards a crucial role of LDs in the removal of misfolded proteins from the cytosol and especially the ER (Jason et al., 2015; Moldavski et al., 2015; Henne et al., 2018). Under conditions of severe proteotoxic stress, LDs are assumed to serve as ‘protein sink’ to support the proteasomal system in aggregate clearance. Accordingly, cells devoid of LDs remove misfolded proteins less efficiently (Moldavski et al., 2015). ER stress induced by acute lipid imbalance causes a massive increase in LD number, in particular at sites of ER aggregates (Jason et al., 2015). Those LDs were found to be loaded with polyubiquitinated proteins and the ER chaperone Kar2, suggesting that LDs indeed sequester damaged proteins at these sites. Subsequent vacuolar degradation of these LDs and their proteotoxic cargo was facilitated by a selective form of autophagy termed microlipophagy, in which the vacuole directly engulfs its cargo (Jason et al., 2015).

Thus, the LD population decorating the periphery of the ER-vacuole contact zone might be in a prime position to sequester misfolded proteins from the ER and facilitate efficient microphagic removal due to the close proximity to the vacuole. Accordingly, not only LD biogenesis and NVJ formation but also Atg1 as key autophagy regulator were required for degradation of NPC assembly intermediates (Lord and Wente, 2020). One might speculate that NVJ-mediated spatial organisation of LDs aids in localized protein removal and subsequent vacuolar engulfment, supporting the proteasome in the turnover of misfolded proteins from the ER upon persisting stress. Mdm1, which facilitates the biosynthesis and clustering of LDs at the periphery of ER-vacuole contacts upon limitation, was also found enriched at the junctions upon compromised NPC assembly. Hence, Mdm1 might link NVJs to LD organisation when cells are subjected to metabolic and proteostatic stress (Henne et al., 2015; Hariri et al., 2018). The notion that LDs serve as ‘escape hatches’ for the retrieval of misfolded proteins is well-supported experimentally (Ploegh, 2007; Jason et al., 2015; Moldavski et al., 2015). However, whether specifically the LDs decorating the NVJs upon proteotoxic stress serve a dedicated function in protein quality control of the ER remains to be shown.

Outlook

Accumulating studies on the dynamic remodelling and physiological relevance of NVJs highlight these contact sites as hubs to integrate metabolic cues and stress responses to determine cellular fate (Hariri et al., 2018; Lord and Wente, 2020; Wood et al., 2020; Tosal-Castano et al., 2021). While compromised NVJ formation remains without major effect on cellular viability in unperturbed cells (Wood et al., 2020), disruption of specific aspects of proteostasis, as shown for deficiencies in NPC assembly (Lord and Wente, 2020), necessitate efficient NVJ formation for survival.

This might be the case for other scenarios of cumulative cellular damage, for instance during cellular ageing (Chen et al., 2020, 2021; Li et al., 2020; Moreno and Aldea, 2020; Mouton et al., 2020). Though NVJs are not essential to drive entry into quiescence upon glucose starvation, prominent NVJ expansion seems to accompany this transition (Wood et al., 2020). Cells can persist in a quiescent state for a long time, awaiting re-entry into cell cycle upon more favourable conditions. Thus, NVJs might serve to spatially concentrate specific enzymatic activities necessary to maintain cellular homeostasis when cells have to persist for an extended period of time in a dormant state characterized by slow metabolism. In support of this, NVJs act as platforms for the local synthesis of a distinct LD subpopulation when cells face nutritional stress (Hariri et al., 2018, 2019). On the other hand, NVJ expansion prior to entry into quiescence might support immediate restart of cell growth and proliferation once nutrients are available again. This could provide an evolutionary advantage when microbial cells have to rapidly increase protein and lipid biogenesis to populate their environment and propagate their heritage (Sun and Gresham, 2021). It is tempting to speculate that NVJs represent some kind of storage units for a distinct set of proteins, in particular for enzymes involved in lipid metabolism, keeping them available for rapid re-distribution as soon as cells encounter conditions suitable for growth. In this line, Snd3 is released from enlarged NVJ patches in starved cells within minutes after glucose is replenished (Tosal-Castano et al., 2021). Whether Snd3 might for instance be involved in the interplay between NVJs and LDs, which is suggested to mitigate proteostatic stress in the nuclear envelope to sustain viability (Lord and Wente, 2020), remains to be shown. As a specific relocalization of Snd3 to the NVJ foci in these conditions was not observed, this protein might respond selectively to nutritional cues. Still, lack of Snd3 as crucial factor for NVJ expansion reduces competitive fitness in large-scale studies (Giaever et al., 2002; Qian et al., 2012), suggesting important functions of this protein to sustain survival of a clonal population.

While global responses to general nutrient deprivation are in place to regulate entrance into quiescence, cells also possess genetic programs specifically tailored to starvation of distinct macronutrients (Boer et al., 2010; Conway et al., 2012; Sun et al., 2020). Not only the set of genes necessary to maintain viability during starvation but also the concomitant cellular remodelling differs depending on the depleted nutrient (Klosinska et al., 2011; Sagot and Laporte, 2019). Thus, NVJs might differentially contribute to entry into or exit from quiescence depending on the respective nutrient scarcity. The protein levels of Nvj1 as the main tether are upregulated in glucose-starved and stationary cells (Pan et al., 2000; Tosal-Castano et al., 2021), most probably controlled by the stress-response element in the promoter region of Nvj1 (Moskvina et al., 1998). Still, the proteome of expanded NVJs is not known yet and will most likely differ depending on the specific cellular status. For instance, proteostatic stress restricted to the nuclear envelope or ER stress drive reshaping and expansion of the NVJs, but a general induction of protein misfolding via heat shock does not affect NVJ appearance (Hariri et al., 2018; Lord and Wente, 2020).

In sum, NVJs emerge as hubs that integrate distinct cellular stress signals and metabolic cues to regulate cell fate. The molecular machineries driving NVJ remodelling and tailoring NVJ molecular composition to the respective cellular needs are far from being understood and represent an exciting challenge for further research.

Footnotes

Declaration of Conflicting Interests

The author(s) declared no potential conflicts of interest with respect to the research, authorship, and/or publication of this article.

Funding

The author(s) disclosed receipt of the following financial support for the research, authorship, and/or publication of this article: This work was supported by the Austrian Science Fund FWF (J4342-B21 to VK; P27183-B24 to SB), the Swedish Research Council (2015-05468 and 2019-05249 to SB), the Knut and Alice Wallenberg foundation (2017.0091 to SB) and the Stiftelsen Olle Engkvist Byggmästare (194-0681 to SB).

ORCID iDs

Verena Kohler

Sabrina Büttner

References

Bean

BDM

Dziurdzik

Kolehmainen

Fowler

CMS

Kwong

Grad

Davey

Schluter

Conibear

(2018). Competitive organelle-specific adaptors recruit Vps13 to membrane contact sites. J Cell Biol 217, 3593–3607. doi: 10.1083/JCB.201804111

Beh

McMaster

Kozminski

Menon

(2012). A detour for yeast oxysterol binding proteins. J Biol Chem 287, 11481–11488. doi: 10.1074/jbc.R111.338400

Boer

Crutchfield

Bradley

Botstein

Rabinowitz

(2010). Growth-limiting intracellular metabolites in yeast growing under diverse nutrient limitations. Mol Biol Cell 21, 198–211. doi: 10.1091/mbc.E09-07-0597

Boettcher

Barral

(2013). The cell biology of open and closed mitosis. Nucleus 4, 160–165. doi: 10.4161/nucl.24676

Bohnert

(2019). Organelle contact sites: lipid droplets hooked by metabolically controlled tethers. Curr Biol 29, R375–R377. doi: 10.1016/j.cub.2019.03.049

Bohnert

(2020). Tether me, tether me not—dynamic organelle contact sites in metabolic rewiring. Dev Cell 54, 212–225. doi: 10.1016/j.devcel.2020.06.026

Chen

Shen

Gao

Luo

(2021). Stress response capacity analysis during aging and possible new insights into aging studies. Curr Genet. Advance online publication. doi: 10.1007/s00294-021-01159-2

Chen

Shen

Zhang

Xiong

Ouyang

Luo

(2020). Age-dependent decline in stress response capacity revealed by proteins dynamics analysis. Sci Rep 10, 15211. doi: 10.1038/s41598-020-72167-4

Conway

Grunwald

Heideman

(2012). Glucose, nitrogen, and phosphate repletion in saccharomyces cerevisiae: common transcriptional responses to different nutrient signals. G3: Genes| Genomes| Genetics 2, 1003–1017. doi: 10.1534/g3.112.002808

10.

Di Mattia

Tomasetto

Alpy

(2020). Faraway, so close! Functions of endoplasmic reticulum–endosome contacts. Biochim Biophys Acta Mol Cell Biol Lipids 1865, 158490. doi: 10.1016/j.bbalip.2019.06.016

11.

Dziurdzik

Bean

BDM

Conibear

(2018). An interorganellar bidding war: Vps13 localization by competitive organelle-specific adaptors. Contact 1, 251525641881462. doi: 10.1177/2515256418814621

12.

Eden

(2016). The formation and function of ER-endosome membrane contact sites. Biochim Biophys Acta 1861, 874–879. doi: 10.1016/j.bbalip.2016.01.020

13.

Eisenberg-Bord

Shai

Schuldiner

Bohnert

(2016). A tether is a tether is a tether: tethering at membrane contact sites. Dev Cell 39, 395–409. doi: 10.1016/j.devcel.2016.10.022

14.

Elbaz-Alon

Eisenberg-Bord

Shinder

Stiller

Shimoni

Wiedemann

Geiger

Schuldiner

(2015). Lam6 regulates the extent of contacts between organelles. Cell Rep 12, 7–14. doi: 10.1016/j.celrep.2015.06.022

15.

Elbaz-Alon

Rosenfeld-Gur

Shinder

Futerman

Geiger

Schuldiner

(2014). A dynamic interface between vacuoles and mitochondria in yeast. Dev Cell 30, 95–102. doi: 10.1016/j.devcel.2014.06.007

16.

Gao

Yang

(2018). VPS13: a lipid transfer protein making contacts at multiple cellular locations. J Cell Biol 217, 3322–3324. doi: 10.1083/jcb.201808151

17.

Garapati

Mishra

(2018). Comparative genomics of nuclear envelope proteins. BMC Genomics 19, 823. doi: 10.1186/s12864-018-5218-4

18.

Gatta

Levine

(2017). Piecing together the patchwork of contact sites. Trends Cell Biol 27, 214–229. doi: 10.1016/j.tcb.2016.08.010

19.

Giaever

Chu

Connelly

Riles

Véronneau

Dow

Lucau-Danila

Anderson

André

, et al (2002). Functional profiling of the Saccharomyces cerevisiae genome. Nature 418, 387–391. doi: 10.1038/nature00935

20.

Hariri

Rogers

Ugrankar

Liu

Feathers

Henne

(2018). Lipid droplet biogenesis is spatially coordinated at ER –vacuole contacts under nutritional stress. EMBO Rep 19, 57–72. doi: 10.15252/embr.201744815

21.

Hariri

Speer

Bowerman

Rogers

Reetz

Datta

Feathers

Ugrankar

Nicastro

, et al (2019). Mdm1 maintains endoplasmic reticulum homeostasis by spatially regulating lipid droplet biogenesis. J Cell Biol 218, 1319–1334. doi: 10.1083/jcb.201808119

22.

Hariri

Ugrankar

Liu

Henne

(2016). Inter-organelle ER-endolysosomal contact sites in metabolism and disease across evolution. Commun Integr Biol 9, e1156278.

23.

Hedbacker

Carlson

(2008). SNF1/AMPK pathways in yeast. Front Biosci 13, 2408–2420. doi: 10.1080/19420889.2016.1156278

24.

Helle

SCJ

Kanfer

Kolar

Lang

Michel

Kornmann

(2013). Organization and function of membrane contact sites. Biochim Biophys Acta—Mol Cell Res 1833, 2526–2541. doi: 10.1016/j.bbamcr.2013.01.028

25.

Henne

(2017). Discovery and roles of ER-endolysosomal contact sites in disease. Adv Exp Med Biol 997, 135–147. doi: 10.1007/978-981-10-4567-7_10

26.

Henne

Reese

Goodman

(2018). The assembly of lipid droplets and their roles in challenged cells. Embo J 37, e98947. doi: 10.15252/embj.201898947

27.

Henne

Zhu

Balogi

Stefan

Pleiss

Emr

(2015). Mdm1/Snx13 is a novel ER-endolysosomal interorganelle tethering protein. J Cell Biol 210, 541–551. doi: 10.1083/jcb.201503088

28.

Hönscher

Mari

Auffarth

Bohnert

Griffith

Geerts

van der Laan

Cabrera

Reggiori

Ungermann

, et al (2014). Cellular metabolism regulates contact sites between vacuoles and mitochondria. Dev Cell 30, 86–94. doi: 10.1016/j.devcel.2014.06.006

29.

Hönscher

Ungermann

(2014). A close-up view of membrane contact sites between the endoplasmic reticulum and the endolysosomal system: from yeast to man. Crit Rev Biochem Mol Biol 49, 262–268. doi: 10.3109/10409238.2013.875512

30.

Jason

Garcia

Chan

RB.

, et al (2015). Role for lipid droplet biogenesis and microlipophagy in adaptation to lipid imbalance in yeast. Dev Cell 35, 584–599. doi: 10.1016/j.devcel.2015.11.010

31.

Jeong

Park

Kim

H-I

Lee

Y-J

Lee

Jun

Lee

(2017). Mechanistic insight into the nucleus-vacuole junction based on the Vac8p-Nvj1p crystal structure. Proc Natl Acad Sci U S A 114, E4539–E4548. doi: 10.1073/pnas.1701030114

32.

Klosinska

Crutchfield

Bradley

Rabinowitz

Broach

(2011). Yeast cells can access distinct quiescent states. Genes Dev 25, 336–349. doi: 10.1101/gad.2011311

33.

Kohler

Aufschnaiter

Büttner

(2020). Closing the gap: membrane contact sites in the regulation of autophagy. Cells 9, 1184. doi: 10.3390/cells9051184

34.

Kohlwein

Eder

Martin

Gable

Bacikova

Dunn

(2001). Tsc13p is required for fatty acid elongation and localizes to a novel structure at the nuclear-vacuolar interface in Saccharomyces cerevisiae. Mol Cell Biol 21, 109–125. doi: 10.1128/mcb.21.1.109-125.2001

35.

Krick

Muehe

Prick

Bremer

Schlotterhose

Eskelinen

E-L

Millen

Goldfarb

Thumm

(2008). Piecemeal microautophagy of the nucleus requires the core macroautophagy genes. Mol Biol Cell 19, 4492–4505. doi: 10.1091/mbc.E08-04-0363

36.

Kvam

Gable

Dunn

Goldfarb

(2005). Targeting of Tsc13p to nucleus-vacuole junctions: a role for very-long-chain fatty acids in the biogenesis of microautophagic vesicles. Mol Biol Cell 16, 3987–3998. doi: 10.1091/mbc.E05-04-0290

37.

Kvam

Goldfarb

(2004). Nvj1p is the outer-nuclear-membrane receptor for oxysterol-binding protein homolog Osh1p in Saccharomyces cerevisiae. J Cell Sci 117, 4959–4968. doi: 10.1242/jcs.01372

38.

Lang

John Peter

Walter

Kornmann

(2015). ER-mitochondrial junctions can be bypassed by dominant mutations in the endosomal protein Vps13. J Cell Biol 210, 883–890. doi: 10.1083/jcb.201502105

39.

Levine

Munro

(2001). Dual targeting of Osh1p, a yeast homologue of oxysterol-binding protein, to both the golgi and the nucleus-vacuole junction. Mol Biol Cell 12, 1633–1644. doi: 10.1091/mbc.12.6.1633

40.

Levine

Patel

(2016). Signalling at membrane contact sites: Two membranes come together to handle second messengers. Curr Opin Cell Biol 39, 77–83. doi: 10.1016/j.ceb.2016.02.011

41.

Jiang

Paxman

O'Laughlin

Klepin

Zhu

Pillus

Tsimring

Hasty

Hao

(2020). A programmable fate decision landscape underlies single-cell aging in yeast. Science 369, 325–329. doi: 10.1126/science.aax9552

42.

Liu

Choudhary

Toulmay

Prinz

(2017). An inducible ER-Golgi tether facilitates ceramide transport to alleviate lipotoxicity. J Cell Biol 216, 131–147. doi: 10.1083/jcb.201606059

43.

Lord

Wente

(2020). Nuclear envelope-vacuole contacts mitigate nuclear pore complex assembly stress. J Cell Biol 219, e202001165. doi: 10.1083/jcb.202001165

44.

Malia

Ungermann

(2016). Vacuole membrane contact sites and domains: emerging hubs to coordinate organelle function with cellular metabolism. Biochem Soc Trans 44, 528–533. doi: 10.1083/jcb.202001165

45.

Manik

Yang

Tong

(2017). Structure of yeast OSBP-Related protein Osh1 reveals key determinants for lipid transport and protein targeting at the Nucleus-Vacuole junction. Structure 25, 617–629.e3. doi: 10.1016/j.str.2017.02.010

46.

Millen

Krick

Prick

Thumm

Goldfarb

(2009). Measuring piecemeal microautophagy of the nucleus in Saccharomyces cerevisiae. Autophagy 5, 75–81. doi: 10.4161/auto.5.1.7181

47.

Millen

Pierson

Kvam

Olsen

Goldfarb

(2008). The luminal N-terminus of yeast Nvj1 is an inner nuclear membrane anchor. Traffic 9, 1653–1664. doi: 10.1111/j.1600-0854.2008.00789.x

48.

Moldavski

Amen

Levin-Zaidman

Eisenstein

Rogachev

Brandis

Kaganovich

Schuldiner

(2015). Lipid droplets are essential for efficient clearance of cytosolic inclusion bodies. Dev Cell 33, 603–610. doi: 10.1016/j.devcel.2015.04.015

49.

Moreno

Aldea

(2020). Proteostatic stress as a nodal hallmark of replicative aging. Exp Cell Res 394, 112163. doi: 10.1016/j.yexcr.2020.112163

50.

Moskvina

Schüller

Maurer

CTC

Mager

Ruis

(1998). A search in the genome of Saccharomyces cerevisiae for genes regulated via stress response elements. Yeast 14, 1041–1050. doi: 10.1002/(SICI)1097-0061(199808)14:11< 1041::AID-YEA296>3.0.CO;2-4

51.

Mostofa

Rahman

Koike

Yeasmin

Islam

Waliullah

Hosoyamada

Shimobayashi

Kobayashi

Hall

MN.

, et al (2018). CLIP and cohibin separate rDNA from nucleolar proteins destined for degradation by nucleophagy. J Cell Biol 217, 2675–2690. doi: 10.1083/jcb.201706164

52.

Mouton

Thaller

Crane

Rempel

Terpstra

Steen

Kaeberlein

Lusk

Boersma

Veenhoff

(2020). A physicochemical perspective of aging from single-cell analysis of PH, macromolecular and organellar crowding in yeast. Elife 9, 1–42. doi: 10.7554/ELIFE.54707

53.

Murley

Sarsam

Toulmay

Yamada

Prinz

Nunnari

(2015). Ltc1 is an ER-localized sterol transporter and a component of ER-mitochondria and ER-vacuole contacts. J Cell Biol 209, 539–548. doi: 10.1083/jcb.201502033

54.

Nettebrock

Bohnert

(2019). Born this way—biogenesis of lipid droplets from specialized ER subdomains. Biochim Biophys Acta—Mol Cell Biol Lipids 1865, 158448. doi: 10.1016/j.bbalip.2019.04.008

55.

Onischenko

Tang

Andersen

Knockenhauer

Vallotton

Derrer

Kralt

Mugler

Chan

Schwartz

Weis

(2017). Natively unfolded FG repeats stabilize the structure of the nuclear pore complex. Cell 171, 904–917.e19. doi: 10.1016/j.cell.2017.09.033

56.

Otto

Thumm

(2021). Mechanistic dissection of macro- and micronucleophagy. Autophagy 17, 626–614. doi: 10.1080/15548627.202025402

57.

Pan

Roberts

Chen

Kvam

Shulga

Huang

Lemmon

Goldfarb

(2000). Nucleus-vacuole junctions in Saccharomyces cerevisiae are formed through the direct interaction of Vac8p with Nvj1p. Mol Biol Cell 11, 2445–2457. doi: 10.1091/mbc.11.7.2445

58.

Park

J-S

Thorsness

Policastro

McGoldrick

Hollingsworth

Thorsness

Neiman

(2016). Yeast Vps13 promotes mitochondrial function and is localized at membrane contact sites. Mol Biol Cell 27, 2435–2449. doi: 10.1091/mbc.E16-02-0112

59.

Ploegh

(2007). A lipid-based model for the creation of an escape hatch from the endoplasmic reticulum. Nature 448, 435–438. doi: 10.1038/nature06004

60.

Prinz

Toulmay

Balla

(2020). The functional universe of membrane contact sites. Nat Rev Mol Cell Biol 21, 7–24. doi: 10.1038/s41580-019-0180-9

61.

Qian

Xiao

Wang

Zhang

(2012). The genomic landscape and evolutionary resolution of antagonistic pleiotropy in yeast. Cell Rep 2, 1399–1410. doi: 10.1016/j.celrep.2012.09.017

62.

Rempel

Crane

Thaller

Mishra

Jansen

Janssens

Popken

Akşit

Kaeberlein

van der Giessen

, et al (2019). Age-dependent deterioration of nuclear pore assembly in mitotic cells decreases transport dynamics. Elife, 8, e48186. doi: 10.7554/eLife.48186

63.

Roberts

Moshitch-Moshkovitz

Kvam

O’Toole

Winey

Goldfarb

(2003). Piecemeal microautophagy of nucleus in Saccharomyces cerevisiae. Mol Biol Cell 14, 129–141. doi: 10.1091/mbc.E02-08-0483

64.

Rzepnikowska

Flis

Kaminska

Grynberg

Urbanek

Ayscough

Zoladek

(2017a). Amino acid substitution equivalent to human choreaacanthocytosis I2771R in yeast Vps13 protein affects its binding to phosphatidylinositol 3-phosphate. Hum Mol Genet 26, 1497–1510. doi: 10.1093/hmg/ddx054

65.

Rzepnikowska

Flis

Muñoz-Braceras

Menezes

Escalante

Zoladek

(2017b). Yeast and other lower eukaryotic organisms for studies of Vps13 proteins in health and disease. Traffic 18, 711–719. doi: 10.1111/tra.12523

66.

Sagot

Laporte

(2019). The cell biology of quiescent yeast—a diversity of individual scenarios. J Cell Sci 132, jcs213025. doi: 10.1242/jcs.213025

67.

Scorrano

De Matteis

Emr

Giordano

Hajnóczky

Kornmann

Lackner

Levine

Pellegrini

Reinisch

, et al (2019). Coming together to define membrane contact sites. Nat Commun 10, 1287. doi: 10.1038/s41467-019-09253-3

68.

Severs

Jordan

Williamson

(1976). Nuclear pore absence from areas of close association between nucleus and vacuole in synchronous yeast cultures. J Ultrasructure Res 54, 374–387. doi: 10.1016/S0022-5320(76)80023-8

69.

Singh

Wróblewska

de Boer

van der Klei

(2020). Hansenula polymorpha Vac8: a vacuolar membrane protein required for vacuole inheritance and nucleus-vacuole junction formation. Contact 3, 1--8. doi: 10.1177/2515256420974928.

70.

Stasyk

(2019). Glucose sensing and regulation in yeasts. In: Non-Conventional Yeasts: From Basic Research to Application. Cham: Springer International Publishing, 477–519. doi: 10.1007/978-3-030-21110-3_14

71.

Sun

Baryshnikova

Brandt

Gresham

(2020). Genetic interaction profiles of regulatory kinases differ between environmental conditions and cellular states. Mol Syst Biol 16, e9167. doi: 10.15252/msb.20199167

72.

Sun

Gresham

(2021). Cellular quiescence in budding yeast. Yeast 38, 12–29. doi: 10.1002/yea.3545

73.

Swinnen

Wanke

Roosen

Smets

Dubouloz

Pedruzzi

Cameroni

De Virgilio

Winderickx

(2006). Rim15 and the crossroads of nutrient signalling pathways in Saccharomyces cerevisiae. Cell Div 1, 3. doi: 10.1186/1747-1028-1-3

74.

Tamura

Kawano

Endo

(2019). Organelle contact zones as sites for lipid transfer. J Biochem 165, 115–123. doi: 10.1093/jb/mvy088

75.

Thaller

Allegretti

Borah

Ronchi

Beck

Lusk

(2019). An escrt-lem protein surveillance system is poised to directly monitor the nuclear envelope and nuclear transport system. Elife, 8, 1--36. doi: 10.7554/eLife.45284

76.

Tomioka

Kotani

Kirisako

, et al (2020). TORC1 inactivation stimulates autophagy of nucleoporin and nuclear pore complexes. J Cell Biol 219. doi: 10.1083/JCB.201910063

77.

Tosal-Castano

Peselj

Kohler

Habernig

Berglund

Ebrahimi

Vögtle

F-N

Höög

Andréasson

Büttner

, et al (2021). Snd3 controls nucleus-vacuole junctions in response to glucose signaling. Cell Rep 34, 108637. doi: 10.1016/j.celrep.2020.108637

78.

Toulmay

Prinz

(2012). A conserved membrane-binding domain targets proteins to organelle contact sites. J Cell Sci 125, 49–58. doi: 10.1242/jcs.085118

79.

Wong

Ysselstein

Krainc

(2018). Mitochondria-lysosome contacts regulate mitochondrial fission via RAB7 GTP hydrolysis. Nature 554, 382–386. doi: 10.1038/nature25486

80.

Wood

Kositangool

Hariri

Marchand

Henne

(2020). Nutrient signaling, stress response, and inter-organelle communication are non-canonical determinants of cell fate. Cell Rep 33, 108446. doi: 10.1016/j.celrep.2020.108446

81.

Huang

(2020). Lipid metabolism at membrane contacts: Dynamics and functions beyond lipid homeostasis. Front Cell Dev Biol 8, 615856. doi: 10.3389/fcell.2020.615856

82.

Zhang

Cao

(2017). Starvation signals in yeast are integrated to coordinate metabolic reprogramming and stress response to ensure longevity. Curr Genet 63, 839–843. doi: 10.1007/s00294-017-0697-4