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. Author manuscript; available in PMC: 2018 Feb 23.
Published in final edited form as: Curr Opin Cell Biol. 2017 Feb 23;44:44–50. doi: 10.1016/j.ceb.2017.02.001

The nucleus: keeping it together by keeping it apart

C Patrick Lusk 1, Megan C King 1
PMCID: PMC5403602  NIHMSID: NIHMS851999  PMID: 28236735

Abstract

It has been postulated that the segregation of nucleus and cytoplasm supported the development of increased organismal complexity. For example, separating transcription and translation allows for mRNA splicing, while the sequestration of genomic DNA supports the innate immune system’s ability to equate cytoplasmic DNA with pathogens. Consistent with the importance of nucleocytoplasmic compartmentalization in a broad array of cellular processes, defects in maintaining discrete nuclear and cytoplasmic compartments, either due to loss of nuclear pore complex integrity, disrupted nuclear transport or ruptures of the nuclear envelope, lead to cellular dysfunction, cell death and disease. Here, we discuss recent insights into how loss of compartmentalization can arise as well as the consequences for cellular and organismal homeostasis.

Keywords: nuclear transport, nuclear rupture, mechanics, laminopathy, c9orf72, dipeptide repeat, hexanucleotide repeat expansion

Introduction

Fundamental mechanisms that maintain the segregation of the nuclear and cytosolic contents have classically been examined under the auspices of “basic” research. Recently, several studies have now identified compromised nuclear compartmentalization as a hallmark of disease, from normal aging to genetically-linked neurodegenerative disease, and potentially even to cellular transformation. Here, we consider how loss of nuclear compartmentalization could contribute to these diseases through the lens of our foundational knowledge of the nuclear transport system, which promises to provide deep insight into disease mechanisms and future potential for targeted molecular intervention.

Establishing stable nuclear and cytoplasmic compartments

The two lipid bilayers that compose the nuclear envelope (NE) form a barrier that effectively compartmentalizes eukaryotic cells into nucleus and cytoplasm; as these membranes are continuous with the endoplasmic reticulum (ER), the NE is essentially an ER subcompartment. The physical integration of the NE and ER suggests that establishment of a distinct nuclear compartment likely arose in concert with (or subsequent to) the acquisition of an endomembrane system, likely through an intermediate state (or proto-nuclear envelope) in which free diffusion could occur between a membrane-encircled genome and the surrounding cell [1,2] (Fig. 1). The protocoatomer hypothesis suggests that a common membrane bending (or stabilizing) machinery arose early in evolution and later became specialized as a critical scaffold for the docking of nuclear pore complexes (NPCs) into the NE [2]. Indeed, the scaffold of the NPC is made up of about a dozen constituent proteins (called nucleoporins or nups) that bear a striking structural similarity to the clathrin and COP coat complexes [3]. The initial NPC membrane coat, which resides at the “pore membrane” where the inner and outer nuclear membranes converge, likely provided the structural basis for ensuring that all macromolecules were routed through pores in the NE (Fig. 1). The later formation of a diffusion barrier by nups rich in phenylalanine-glycine (FG) repeats anchored to this membrane coat likely laid the groundwork for the future regulation of nuclear-cytoplasmic exchange of macromolecules by NPCs and soluble nuclear transport receptors (NTRs; Fig. 1) [4,5].

Figure 1.

Figure 1

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Schematic of likely steps leading to the formation of the nucleocytoplasmic barrier. At left, a primitive endomembrane system (blue) is developed with connections to the genome mediated by membrane proteins and an ancient proto-coatomer (bracket shapes) capable of stabilizing membrane curvature. Ribosomes are grey with red nascent polypeptide. In middle, the protocoatomer provides the building blocks for the NPC architecture, which drives exchange through pores in the “proto-nuclear envelope”. The contents of the nucleus and cytoplasm are not fully segregated until the last eukaryotic common ancestor (LECA; right), which would incorporate the FG-nups into the NPC scaffold, allowing the generation of a size-selective diffusion barrier and active nuclear transport mediated by NTRs (green in inset). Inset of NPC showing the major architectural units including the inner rings (purple), outer rings (orange), FG-nups (blue squiggles) and nuclear basket (green). Ran-GTP is found predominantly in the nucleus, where it releases import cargoes from NTRs and stabilizes export complexes.

The establishment of NPCs as a barrier to free diffusion for macromolecules with a Stokes radius of >~2.5 nm, corresponding to a protein of ~35–40 kDa in mass [6] would present a clear impediment to the exchange of macromolecules necessary for a number of essential cellular processes. One of the intuitive consequences of this compartmentalization is the physical segregation of the genome (and therefore transcription) away from ribosomes (and therefore translation). Indeed, it has been postulated that the origin of introns and the mRNA splicing machinery is intimately linked to the establishment of separate nuclear and cytoplasmic compartments [7]. Moreover, the ribosome is built upon its rRNA core, and acts on an mRNA template; both RNAs are synthesized from a nuclear DNA template, necessitating mechanisms to export these large cargos to the cytoplasm, where mature ribosomes reside and translation take place [8]. Accessory proteins (NTRs, some of which are also called karyopherins or importins/exportins) that bind such large molecules promote their passage through the FG-repeat rich NPC core, while the directionality of transport is contributed by asymmetric nuclear and/or cytosolic factors, most notably the Ran GTPase, which is in the GTP-bound form in the nucleus and the GDP-bound form in the cytoplasm [9](Fig. 1). Thus, the steady-state localization of a given factor is predominantly determined by 1) its size (either alone or in complex), which will define its ability to equilibrate in a passive fashion between nucleus and cytoplasm, 2) whether active transport pathways drive its import or export to/from the nucleus and 3) the retention of a factor by its interactions with architectural components restricted to either compartment [10]. As we will discuss below, both passive and active transport will both be affected by perturbations that disrupt the nucleocytoplasmic barrier either through the loss of NPC function, or, mechanical disruption of the NE membranes.

To limit mechanical disruption of the NE, the nucleus is stabilized by the nuclear lamina, an integrated scaffold composed of nuclear lamins, integral inner nuclear membrane (INM) proteins and (predominantly heterochromatic) chromatin [11]. A- and B-type lamins, members of the intermediate filament family, each form distinct but inter-dependent protein networks that line the INM as recently visualized with super-resolution approaches [12,13]. It is possible that imparting mechanical stability also limits NE dynamics, as exemplified by the lamin-based immobilization of NPCs [14]. Indeed, the mobility of NPCs might serve as a bellwether that reflects the plasticity of the NE system. For example, in embryonic Drosophila cells NPCs are highly mobile; this mobility is later restricted by upregulation of lamins and lamin binding proteins during differentiation [15]. Indeed, in terminally differentiated neurons, scaffold nucleoporins are some of the most stable proteins, turning over in timespans of months to years [16,17]. This lack of turnover is not without consequence, however, as it opens the door for NPCs to accumulate damage with age.

Leaky NPCs, NPC dysfunction and disease

Indeed, oxidative damage to NPCs has been observed in C. elegans and in old rat brains leading to a disruption of the NPC diffusion barrier and the nuclear aggregation of cytosolic proteins, a typical phenotype of neurodegenerative disease pathology [18] (Fig. 2). Analogously, toxic cytosolic protein aggregates accumulate in neurodegenerative disease [19] and these might also impact nuclear compartmentalization by sequestering specific NTRs [20] (Fig. 2A). More recently, the loss of nuclear compartmentalization was shown to impact the progression of neurodegenerative diseases like amyotrophic lateral sclerosis (ALS) and frontotemporal dementia (FTD), but through a distinct mechanism. Forms of these diseases are thought to be caused by the expression of a hexanucleotide (GGGGCC) repeat expansion (HRE) in an intron of the C9orf72 gene, but it remains debated whether the toxicity of the repeats stems from the resulting transcript, which may form parallel arrays of G-quadruplexes capable of binding other proteins and RNAs [21], and/or non-AUG translation, producing small dipeptide repeat (DPR) proteins (Fig 2B). Nonetheless, from yeast to mammals, the overexpression of these repeats leads to cellular toxicity, suggesting the evolutionary conservation of molecular components that, when disrupted, help drive the disease.

Figure 2.

Figure 2

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Consequences of disruptions of nucleocytoplasmic compartmentalization. A. Cytosolic aggregates of β-sheet proteins can sequester NTRs and mRNA export factors, leading to the accumulation of mRNA in the nucleus. B. The transcription of the HRE of the C9orf72 intron (red) leads to the production of parallel RNA G-quadruplexes that can accumulate in RNA foci or be exported (through an unknown mechanism) into the cytosol, where they can interact with other proteins (like RanGAP) or be translated into DPRs. DPRs can direct bind to the FG-nups within the NPC to block nuclear transport. C. In more extreme circumstances a nuclear rupture event can allow even large organelles into the nucleus and will expose genomic DNA to the cytoplasm. Both cytosolic DNA and immature RNA can be recognized by pattern recognition receptors (PRRs) and illicit an immune response. D. Damage to NPCs in old neurons can lead to a breakdown of the permeability barrier and the free exchange of nuclear and cytosolic contents, leading to the accumulation of cytosolic proteins in the nucleus and nuclear-restricted nucleic acids (like immature mRNAs) in the cytosol. Cytoplasmic DNases (like TREX1) could drive DNA damage when they access the nucleoplasm.

Several recent studies suggest that the nuclear transport apparatus could be the evolutionarily conserved machinery targeted by HRE expression [2124]. First, the overexpression of multiple NTRs leads to a decline in HRE toxicity in yeast, suggesting a capacity to overcome a block in nuclear transport [23]. These results were mirrored by several studies in Drosophila in which genetic perturbation of both the soluble phase (i.e. NTRs and Ran/Ran binding proteins) and the stationary phase (i.e. the NPC) of the nuclear transport machinery (Fig 1) leads to the exacerbation or suppression of HRE toxicity in ways that confound a straightforward mechanistic interpretation [21,22,25]. This is likely because the HRE transcripts and the DPR proteins influence cell physiology in distinct manners, perhaps by directly inhibiting unique factors involved in nuclear transport. For example, the HRE transcripts can directly bind to the Ran GTPase activating protein (RanGAP), which might lead to its mislocalization into cytosolic foci [21]. The appearance of these foci in both brain sections and iPS-derived neurons from ALS patients suggests that mislocalized RanGAP is a pathological feature of the disease [21]. It remains unclear, however, whether these interactions perturb the ability of RanGAP to promote conversion of RanGTP to RanGDP in the cytoplasm. Moreover, as additional components of the nuclear transport apparatus are also mislocalized under these conditions, including some nups, it may be that a more general effect on the nuclear transport system is responsible.

In order to gain a broader picture of the potential mechanisms by which HREs influence cellular function, unbiased proteomic approaches sought to identify DPR interacting proteins [25,26]; both nups and NTRs were identified [25]. Interestingly, there was a clear propensity for DPRs to interact with low complexity, often intrinsically disordered proteins (IDPs) that associate with membrane-less organelles [9]. Indeed, the infiltration of DPRs into phase-separated domains both in vivo and in vitro influences their biophysical properties and function [25,26]. Interestingly, there are many similarities between IDPs that form membrane-less organelles and the FG-nups [9]. In fact, it has long been understood that FG-nups can undergo a phase-transition into a hydrogel in vitro [27], which might be reinforced by intermolecular β-sheet interfaces that also contribute to amyloid formation [28]. While it remains debated whether such a hydrogel exists in the central channel of the NPC, recent work demonstrates that arginine-rich DPR repeat proteins can interact directly with a polymeric, amyloid-like form of the FG-nups, Nup54 and Nup98 [24].

The binding of DPRs to polymers of FG-nups is reflected in vivo by the accumulation of DPRs at NPCs [24]. Interestingly, the nanoscale distribution of DPRs suggest an enrichment along the NPC channel walls in contrast to other FG-nup epitopes, such as those in Nup62 [29] or wheat germ agglutinin (which binds to GlcNacylation in the FG domains) that reside at the center of the channel [24]. This distribution could reflect the restriction of β-sheet interactions that polymerize FG-nups in vitro to the channel walls. Alternatively, the DPRs may drive non-physiological interactions among the FG-nups that contribute to the observed disruption of nuclear import and export [24] (Fig. 2B). A prediction of the latter model would be that the NPC diffusion barrier would also be affected by DPR binding, which has yet to be tested. Regardless, these data provide compelling molecular insight into a direct mechanism by which HREs could disrupt nuclear transport. Excitingly, the DPRs may also provide a tool to probe the properties of the NPC channel to help solve a long-standing question as to the native organization of the FG-nups.

Causes and consequences of nuclear rupture

While an imbalance in the nuclear transport machinery can contribute to disease progression, recent evidence supports that more acute and dramatic releases of nuclear components into the cytoplasm (and in-flow of cytoplasmic contents into the nucleus) is driven by nuclear rupture events (Fig 2C). In these cases, it is thought that both the inner and outer nuclear membranes undergo rupture, which is sometimes preceded by the formation of a NE bleb [30,31]. Recently, there have been two contexts in which nuclear rupture occurs at high frequency, which may be driven by distinct factors, and have distinct consequences.

Two types of nuclear rupture occur downstream of chromosome segregation errors. In the first, highly persistent chromatin bridges, such as those that arise in cells with dicentric chromosomes due to telomere-telomere fusion, eventually lead to NE rupture in the subsequent interphase, which allows for the chromosomes to be fully segregated at the cost of a high mutational load presumably in the DNA that resided in the chromatin bridge [32]. In the second, a lagging chromosome nucleates formation of its own “micronucleus”, which is physically separated from the remainder of the chromosomes in the “primary nucleus”. For reasons that remain enigmatic, the NEs that define micronuclei fail to accumulate a normal NE proteome, including alterations to the nuclear lamina [33]. Interestingly, although micronuclei often succeed in establishing the NE barrier at mitotic exit, in the subsequent interphase many micronuclei undergo a catastrophic rupture [33]. Such ruptures sometimes are “healed”, while others appear to be irreparable. The loss of the intact NE barrier is linked to massive genome rearrangement events in which the entire (usually single) chromosome within the micronucleus is shattered and pieced back together (termed chromothripsis) – an occurrence linked to transformed cells, and a potential driver of further losses of genome integrity [34,35]. While much remains to be understood about this process, and its prevalence, it provides strong evidence for links between maintenance of the nuclear compartment and genome integrity. Although loss of nuclear compartmentalization in micronuclei correlates with deficiencies in replication [34], an increase in DNA damage load [3335], and an altered DNA damage response [36], much remains to be determined about the mechanisms at play.

The nuclei of certain cell types must balance deformability necessary for effective migration through complex environments with cell survival. Short-lived immune cells such as neutrophils down-regulate A-type lamins during differentiation, coincident with lobulation of the nucleus (potentially to increase nuclear deformability) [37]. By contrast, longer lived dendritic cells (DCs) express A-type lamins. DCs surveil for foreign antigens and, after activation, mature and migrate to the lymph nodes, ultimately presenting antigens to T-cells to support adaptive immune system function [38]. Two recent studies, using both DC and transformed cell line models, highlight how migration through constricted environments can lead to dramatic losses of nucleocytoplasmic compartmentalization, driven by herniation and rupture of the NE [30,31]. Remarkably, these events are often transient due to a NE repair mechanism catalyzed by the ESCRT machinery; a NE rupture would likely present a topology similar to the NE discontinuities sealed by the ESCRT machinery at mitotic exit [30,31,39,40]. Interestingly, NE ruptures that occur during migration through constricted environments occur coincidentally with loading of DNA repair factors onto chromatin [30,31], suggesting that such events could also be drivers of genome instability. While numerous questions remain about the source of the potential DNA damage that occurs in this context, simultaneously compromising the DNA damage response machinery and the ESCRT machinery necessary for “healing” NE ruptures leads to enhanced cell death [30,31]. Physical confinement of the nucleus induced by cytoskeletal contractility in non-migrating cells also appears to be sufficient to drive similar NE ruptures [41], suggesting that mechanisms capable of maintaining nuclear integrity in response to physical force are likely to be critical in a variety of cellular and tissue contexts.

What might be the consequences of such catastrophic loss of the nuclear barrier? Transient NE ruptures could explain the observation that large protein aggregates (or even organelles [42]) accumulate within the nucleoplasm of aged cells [43](Fig 2C). This suggests that large, non-dynamic proteinaceous structures may become irreversibly trapped within the nucleoplasm, particularly in post-mitotic cells that never have the ability to “purge” themselves through sequential processes of NE breakdown, chromosome segregation, and NE reformation [44]. The sheer size of large protein aggregates or organelles in the nucleus would present a serious challenge for the autophagy machinery that is mostly cytosolic, thereby driving loss of cellular function and viability.

Outlook: emerging themes for crosstalk between the nuclear barrier and immunosurveillance?

Although toxic nuclear aggregates can be a driver of disease, we argue that improperly compartmentalized nucleic acids arising from NE ruptures or dysfunctional NPCs is perhaps most likely to compromise homeostasis at the level of the organism (Fig 2). For example, the addition of the nucleus as a dedicated compartment that houses the DNA (and immature mRNA) allowed for the adoption of innate immunity pathways that take advantage of the sequestration of “self” DNA within the nucleus, making the nucleoplasm essentially “immune-privileged”. Innate immune pattern recognition receptors are poised to respond to cytoplasmic nucleic acids during interphase, which is taken as evidence of an ongoing infection [45]. Activation of this machinery can drive cell death, inflammation, and an immune response; inappropriate triggering of these pathways due to exposure of the chromatin to the cytoplasm with NE ruptures or “leaky” NPCs could therefore be a major driver of pathologies, from aging to autoimmune disease (Fig 2D). Indeed, a domain of the innate immunity factor cGAS has been used as an effective reporter for nuclear rupture [30,31], although future studies will be necessary to assess whether such losses of nuclear compartmentalization are sufficient to trigger the cGAS-STING pathway [46]. Moreover, nuclear rupture could lead to degradation of nuclear DNA by (normally cytosolic) DNases, for example TREX1 (DNase III), the 3′ nuclease that acts to resolve the DNA in chromatin bridges when the NE ruptures during failed chromosome segregation [32]. A defect in the NPC barrier could also allow immature RNA to circumvent the normal mRNA surveillance machinery that acts at the nuclear basket of the NPC [47]; such immature cytoplasmic RNA, sensed by defects in the 5′ RNA cap, for example, could also be perceived as viral RNA, again driving an immune response [48](Fig 2D). Although the potential for loss of nucleocytoplasmic compartmentalization to drive an immune response remains largely untested, it nonetheless presents a tantalizing possibility for future work to investigate the connection between the maintenance of the nuclear compartment and aging.

Acknowledgments

CPL is supported by the NIH (RO1GM105672 and R21GM109466). MCK is funded by the NSF (CMMI-1634988).

Footnotes

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