Herpesvirus Nuclear Egress

Roller, Richard J.; Baines, Joel D.

doi:10.1007/978-3-319-53168-7_7

Cited by 46 publications

(56 citation statements)

References 177 publications

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“…The intrinsic ability of the NEC to deform and bud membranes and to oligomerize into a hexagonal coat is well established [reviewed in (Bigalke and Heldwein 2016, Mettenleiter 2016, Bigalke and Heldwein 2017, Roller and Baines 2017)]. However, it is unclear how the capsid triggers the formation of the NEC coat around it or how the NEC coat is anchored to the capsid.…”

Section: Discussionmentioning

confidence: 99%

“…All herpesviruses can establish lifelong, latent infections within the host, from which they can periodically reactivate, spreading to uninfected tissues and hosts and causing a number of ailments. When the virus actively replicates during a primary infection or reactivation of a latent infection, the progeny virions are assembled and released from the cell in a process termed egress whereby herpesvirus capsids traverse cellular membranes twice [reviewed in (Johnson and Baines 2011, Bigalke and Heldwein 2016, Roller and Baines 2017)]. First, nuclear capsids bud at the inner nuclear membrane (INM) forming enveloped vesicles that pinch off into the perinuclear space.…”

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Structural basis for capsid recruitment and coat formation during HSV-1 nuclear egress

Draganova

Zhang

et al. 2020

Preprint

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18During herpesvirus infection, egress of nascent viral capsids from the nucleus is mediated by the 19 viral nuclear egress complex (NEC). NEC deforms the inner nuclear membrane (INM) around 20 the capsid by forming a hexagonal array. However, how the NEC coat interacts with the capsid 21 and how curved coats are generated to enable budding is yet unclear. Here, by structure-guided 22 truncations, confocal microscopy, and cryoelectron tomography, we show that binding of the 23 capsid protein UL25 promotes the formation of NEC pentagons rather than hexagons. We 24 hypothesize that during nuclear budding, binding of UL25 situated at the pentagonal capsid 25 vertices to the NEC at the INM promotes formation of NEC pentagons that would anchor the 26 NEC coat to the capsid. Incorporation of NEC pentagons at the points of contact with the 27 vertices would also promote assembly of the curved hexagonal NEC coat around the capsid, 28 leading to productive egress of UL25-decorated capsids. 30To replicate, all viruses must assemble their progeny virions and release them from the cell while 31 overcoming many obstacles, including cellular compartmentalization. Viruses are thus experts at 32 hijacking, manipulating, and, sometimes, even remodeling cellular architecture during viral 33 morphogenesis and egress. Identifying and understanding the unique aspects of virus-induced 34 cellular remodeling could unveil targets for therapeutic intervention; yet, we are only beginning 35 to understand the mechanisms behind many of these processes. 36 One prominent example of virus-induced remodeling of cellular architecture can be 37 observed during egress of herpesviruses -enveloped, double-stranded DNA viruses that infect a 38 wide range of hosts, from mollusks to humans. All herpesviruses can establish lifelong, latent 39 infections within the host, from which they can periodically reactivate, spreading to uninfected 40 tissues and hosts and causing a number of ailments. When the virus actively replicates during a 41 primary infection or reactivation of a latent infection, the progeny virions are assembled and 42 released from the cell in a process termed egress whereby herpesvirus capsids traverse cellular 43 membranes twice [reviewed in (Johnson and Baines 2011, Bigalke and Heldwein 2016, Roller 44 and Baines 2017)]. First, nuclear capsids bud at the inner nuclear membrane (INM) forming 45 enveloped vesicles that pinch off into the perinuclear space. These perinuclear viral particles fuse 46 with the outer nuclear membrane, which releases the capsids into the cytosol. Cytoplasmic 47 capsids then bud again at vesicles derived from the trans-Golgi network and early endosomes 48 [reviewed in (Johnson and Baines 2011)] to form mature, infectious virions that are released 49 from the cell by exocytosis. Whereas many enveloped viruses acquire their lipid envelopes by 50 budding at the cytoplasmic membranes or the plasma membrane, herpesviruses are unusual 51 among vertebrate viruses in their ability to bud at the nuclear env...

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Section: Discussionmentioning

confidence: 99%

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confidence: 99%

Structural basis for capsid recruitment and coat formation during HSV-1 nuclear egress

Draganova

Zhang

et al. 2020

Preprint

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“…Surprisingly, Wash's role in this process is bipotent and, independent of Recently, Nuclear Envelope (NE-) budding was identified as an alternative pathway for nuclear exit, particularly for large developmentally-required ribonucleoprotein (megaRNP) complexes that would otherwise need to unfold/remodel to fit through the NPCs (Fradkin and Budnik, 2016;Hatch and Hetzer, 2014;Hatch and Hetzer, 2012;Jokhi et al, 2013;Li et al, 2016;Parchure et al, 2017;Speese et al, 2012). In this pathway, large macromolecule complexes, such as megaRNPs, are encircled by the nuclear lamina (type-A and type-B lamins) and inner nuclear membrane, are pinched off from the inner nuclear membrane, cross the perinuclear space, fuse with the outer nuclear membrane, and release the megaRNPs into the cytoplasm (Figure 1A-C).Strikingly, NE-budding shares many features with the nuclear egress mechanism used by herpesviruses, common pathogens that cause and/or contribute to a diverse array of human diseases (Bigalke and Heldwein, 2016;Hagen et al, 2015;Lye et al, 2017;Mettenleiter et al, 2013;Parchure et al, 2017;Roller and Baines, 2017). As viruses often take advantage of preexisting host pathways for their livelihoods, the parallel between nuclear exit of herpesvirus nucleocapsids and that of megaRNPs suggests that NE-budding may be a general cellular mechanism that elegantly allows for the nuclear export of endogenous megaRNPs and/or other large cargos (cf.…”

mentioning

confidence: 99%

“…As viruses often take advantage of preexisting host pathways for their livelihoods, the parallel between nuclear exit of herpesvirus nucleocapsids and that of megaRNPs suggests that NE-budding may be a general cellular mechanism that elegantly allows for the nuclear export of endogenous megaRNPs and/or other large cargos (cf. (Fradkin and Budnik, 2016;Mettenleiter et al, 2013;Parchure et al, 2017;Roller and Baines, 2017). Indeed, this pathway has also been implicated in the removal of obsolete macromolecular complexes or other material (i.e., large protein aggregates, polyubiquitylated proteins) from the nucleus (Jokhi et al, 2013;Ramaswami et al, 2013;Rose and Schlieker, 2012).The NE-budding pathway was first demonstrated in Drosophila synapse development, proving to be essential for neuromuscular junction integrity.…”

mentioning

confidence: 99%

“…Strikingly, NE-budding shares many features with the nuclear egress mechanism used by herpesviruses, common pathogens that cause and/or contribute to a diverse array of human diseases (Bigalke and Heldwein, 2016;Hagen et al, 2015;Lye et al, 2017;Mettenleiter et al, 2013;Parchure et al, 2017;Roller and Baines, 2017). As viruses often take advantage of preexisting host pathways for their livelihoods, the parallel between nuclear exit of herpesvirus nucleocapsids and that of megaRNPs suggests that NE-budding may be a general cellular mechanism that elegantly allows for the nuclear export of endogenous megaRNPs and/or other large cargos (cf.…”

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confidence: 99%

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Wash and the WASH Regulatory Complex function in Nuclear Envelope budding

Verboon

Nakamura

Decker

et al. 2019

Preprint

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Nuclear envelope budding is a recently described phenomenon wherein large macromolecular complexes can be packaged inside the nucleus and be extruded through the nuclear membranes, completely bypassing nuclear pores. While factors have been identified both as cargos or actively involved in this process, much remains unknown about the molecules that generate the forces and membrane deformations which appear inherent. Using fluorescence and electron microscopy, biochemical and cell biological assays, and genetic perturbations in the Drosophila model, we identify Wash, its regulatory complex, and Arp2/3 as novel players in NE-budding. Surprisingly, Wash's role in this process is bipotent and, independent of Recently, Nuclear Envelope (NE-) budding was identified as an alternative pathway for nuclear exit, particularly for large developmentally-required ribonucleoprotein (megaRNP) complexes that would otherwise need to unfold/remodel to fit through the NPCs (Fradkin and Budnik, 2016;Hatch and Hetzer, 2014;Hatch and Hetzer, 2012;Jokhi et al., 2013;Li et al., 2016;Parchure et al., 2017;Speese et al., 2012). In this pathway, large macromolecule complexes, such as megaRNPs, are encircled by the nuclear lamina (type-A and type-B lamins) and inner nuclear membrane, are pinched off from the inner nuclear membrane, cross the perinuclear space, fuse with the outer nuclear membrane, and release the megaRNPs into the cytoplasm (Figure 1A-C).Strikingly, NE-budding shares many features with the nuclear egress mechanism used by herpesviruses, common pathogens that cause and/or contribute to a diverse array of human diseases (Bigalke and Heldwein, 2016;Hagen et al., 2015;Lye et al., 2017;Mettenleiter et al., 2013;Parchure et al., 2017;Roller and Baines, 2017). As viruses often take advantage of preexisting host pathways for their livelihoods, the parallel between nuclear exit of herpesvirus nucleocapsids and that of megaRNPs suggests that NE-budding may be a general cellular mechanism that elegantly allows for the nuclear export of endogenous megaRNPs and/or other large cargos (cf. (Fradkin and Budnik, 2016;Mettenleiter et al., 2013;Parchure et al., 2017;Roller and Baines, 2017). Indeed, this pathway has also been implicated in the removal of obsolete macromolecular complexes or other material (i.e., large protein aggregates, polyubiquitylated proteins) from the nucleus (Jokhi et al., 2013;Ramaswami et al., 2013;Rose and Schlieker, 2012).The NE-budding pathway was first demonstrated in Drosophila synapse development, proving to be essential for neuromuscular junction integrity. Here, a C-terminal fragment (dFz2C) of the fly Wingless receptor, dFz2C, was shown to associate with megaRNPs that formed foci at the nuclear periphery and exited the nucleus by budding through the nuclear envelope ( Figure 1B-C) (Speese et al., 2012). Failure of this process resulted in aberrant

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Nuclear envelope budding: Getting large macromolecular complexes out of the nucleus

Sule,

Nakamura,

Parkhurst

2023

BioEssays

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Transport of macromolecules from the nucleus to the cytoplasm is essential for nearly all cellular and developmental events, and when mis‐regulated, is associated with diseases, tumor formation/growth, and cancer progression. Nuclear Envelope (NE)‐budding is a newly appreciated nuclear export pathway for large macromolecular machineries, including those assembled to allow co‐regulation of functionally related components, that bypasses canonical nuclear export through nuclear pores. In this pathway, large macromolecular complexes are enveloped by the inner nuclear membrane, transverse the perinuclear space, and then exit through the outer nuclear membrane to release its contents into the cytoplasm. NE‐budding is a conserved process and shares many features with nuclear egress mechanisms used by herpesviruses. Despite its biological importance and clinical relevance, little is yet known about the regulatory and structural machineries that allow NE‐budding to occur in any system. Here we summarize what is currently known or proposed for this intriguing nuclear export process.

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Herpesvirus Nuclear Egress

Cited by 46 publications

References 177 publications

Structural basis for capsid recruitment and coat formation during HSV-1 nuclear egress

Structural basis for capsid recruitment and coat formation during HSV-1 nuclear egress

Wash and the WASH Regulatory Complex function in Nuclear Envelope budding

Nuclear envelope budding: Getting large macromolecular complexes out of the nucleus

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