VRK2A is an A-type lamin–dependent nuclear envelope kinase that phosphorylates BAF

The nuclear envelope (NE) is critical for numerous fundamental cellular functions, and mutations in several NE constituents can lead to a heterogeneous spectrum of diseases. We used proximity biotinylation to uncover new constituents of the inner nuclear membrane (INM) by comparative BioID analysis of lamin A, Sun2 and a minimal INM-targeting motif. These studies identify vaccinia-related kinase-2 (VRK2) as a candidate constituent of the INM. The transmembrane VRK2A isoform is retained at the NE by association with A-type lamins. Furthermore, VRK2A physically interacts with A-type, but not B-type, lamins. Finally, we show that VRK2 phosphorylates barrier to autointegration factor (BAF), a small and highly dynamic chromatin-binding protein, which has roles including NE reassembly, cell cycle, and chromatin organization in cells, and subtly alters its nuclear mobility. Together these findings support the value of using BioID to identify unrecognized constituents of distinct subcellular compartments refractory to biochemical isolation and reveal VRK2A as a transmembrane kinase in the NE that regulates BAF.

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The cell cycle dependent mislocalisation of emerin may contribute to the Emery-Dreifuss muscular dystrophy phenotype

Journal of Cell Science ◽

10.1242/jcs.115.2.341 ◽

2002 ◽

Vol 115 (2) ◽

pp. 341-354 ◽

Cited By ~ 1

Author(s):

Elizabeth A. L. Fairley ◽

Andrew Riddell ◽

Juliet A. Ellis ◽

John Kendrick-Jones

Keyword(s):

Cell Cycle ◽

Muscular Dystrophy ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Transmembrane Domain ◽

Nuclear Lamina ◽

Lamin A ◽

Wild Type ◽

Cycle Dependent ◽

Mutant Forms

Emerin is the nuclear membrane protein defective in X-linked Emery-Dreifuss muscular dystrophy (X-EDMD). The majority of X-EDMD patients have no detectable emerin. However, there are cases that produce mutant forms of emerin, which can be used to study its function. Our previous studies have shown that the emerin mutants S54F, P183T, P183H, Del95-99, Del236-241 (identified in X-EDMD patients) are targeted to the nuclear membrane but to a lesser extent than wild-type emerin. In this paper, we have studied how the mislocalisation of these mutant emerins may affect nuclear functions associated with the cell cycle using flow cytometry and immunofluorescence microscopy. We have established that cells expressing the emerin mutant Del236-241 (a deletion in the transmembrane domain), which was mainly localised in the cytoplasm, exhibited an aberrant cell cycle length. Thereafter, by examining the intracellular localisation of endogenously expressed lamin A/C and exogenously expressed wild-type and mutant forms of emerin after a number of cell divisions, we determined that the mutant forms of emerin redistributed endogenous lamin A/C. The extent of lamin A/C redistribution correlated with the amount of EGFP-emerin that was mislocalised. The amount of EGFP-emerin mislocalized, in turn, was associated with alterations in the nuclear envelope morphology. The nuclear morphology and redistribution of lamin A/C was most severely affected in the cells expressing the emerin mutant Del236-241.It is believed that emerin is part of a novel nuclear protein complex consisting of the barrier-to-autointegration factor (BAF), the nuclear lamina, nuclear actin and other associated proteins. The data presented here show that lamin A/C localisation is dominantly directed by its interaction with certain emerin mutants and perhaps wild-type emerin as well. These results suggest that emerin links A-type lamins to the nuclear envelope and that the correct localisation of these nuclear proteins is important for maintaining cell cycle timing.

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Characterization of A 54-kD protein of the inner nuclear membrane: evidence for cell cycle-dependent interaction with the nuclear lamina.

The Journal of Cell Biology ◽

10.1083/jcb.114.3.389 ◽

1991 ◽

Vol 114 (3) ◽

pp. 389-400 ◽

Cited By ~ 36

Author(s):

S M Bailer ◽

H M Eppenberger ◽

G Griffiths ◽

E A Nigg

Keyword(s):

Cell Cycle ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Cultured Cells ◽

Nuclear Lamina ◽

Biochemical Properties ◽

Inner Nuclear Membrane ◽

Cycle Dependent ◽

Mitotic Phosphorylation

Using a mAb (R-7), we have characterized a 54-kD protein of the chicken nuclear envelope. Based on its biochemical properties and subnuclear distribution p54 is likely to be an integral membrane component specific to the inner nuclear membrane. Fractionation experiments indicate that p54 interacts, directly or indirectly, with the nuclear lamina, and analysis of p54 in cultured cells suggests that this interaction is controlled by cell cycle-dependent posttranslational modification, most likely phosphorylation. Modification of p54 results in a slightly reduced electrophoretic mobility, and it converts the protein from a detergent-resistant to a detergent-extractable form. Detergent solubilization of p54 can be induced in vivo by treating isolated nuclei or nuclear envelopes with highly purified cdc2 kinase, one of the most prominent kinases active in mitotic cells. These results suggest that mitotic phosphorylation of p54 might contribute to control nuclear envelope dynamics during mitosis in vivo.

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Myne-1, a spectrin repeat transmembrane protein of the myocyte inner nuclear membrane, interacts with lamin A/C

Journal of Cell Science ◽

10.1242/jcs.115.1.61 ◽

2002 ◽

Vol 115 (1) ◽

pp. 61-70 ◽

Cited By ~ 3

Author(s):

John M. K. Mislow ◽

Marian S. Kim ◽

Dawn Belt Davis ◽

Elizabeth M. McNally

Keyword(s):

Muscular Dystrophy ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Transmembrane Domain ◽

Transmembrane Protein ◽

Lamin A ◽

Spectrin Repeat ◽

Inner Nuclear Membrane ◽

C Terminus

Mutations in the genes encoding the inner nuclear membrane proteins lamin A/C and emerin produce cardiomyopathy and muscular dystrophy in humans and mice. The mechanism by which these broadly expressed gene products result in tissue-specific dysfunction is not known. We have identified a protein of the inner nuclear membrane that is highly expressed in striated and smooth muscle. This protein, myne-1 (myocyte nuclear envelope), is predicted to have seven spectrin repeats, an interrupted LEM domain and a single transmembrane domain at its C-terminus. We found that myne-1 is expressed upon early muscle differentiation in multiple intranuclear foci concomitant with lamin A/C expression. In mature muscle, myne-1 and lamin A/C are perfectly colocalized, although colocalization with emerin is only partial. Moreover, we show that myne-1 and lamin A/C coimmunoprecipitate from differentiated muscle in vitro. The muscle-specific inner nuclear envelope expression of myne-1, along with its interaction with lamin A/C, indicates that this gene is a potential mediator of cardiomyopathy and muscular dystrophy.

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Nonlamin components of the lamina: a paucity of proteins

Biochemistry and Cell Biology ◽

10.1139/o99-049 ◽

1999 ◽

Vol 77 (4) ◽

pp. 311-319

Author(s):

Nathalie Chaly ◽

Ursula Stochaj

Keyword(s):

Cell Cycle ◽

Nuclear Envelope ◽

Experimental Evidence ◽

Nuclear Membrane ◽

Nuclear Organization ◽

Diverse Group ◽

Structural Elements ◽

Inner Nuclear Membrane ◽

Chromatin Loops ◽

Universal Feature

Current models of nuclear organization propose that nuclear functions are modulated in part by reversible tethering of chromatin loops to structural elements of the nucleoplasm and the nuclear envelope. Lamins are the best-characterized proteins of the lamina portion of the nuclear envelope and are involved in binding chromatin to the inner nuclear membrane. However, they are not a universal feature of eukaryotic nuclei and do not account fully for the putative functions of the lamina in all organisms. It is possible that nonlamin components of the lamina may substitute for lamins in organisms from which they are absent and modify the properties of lamins during development and the cell cycle. We review the properties of the relatively small number of such components that have been reported, including the young arrest (fs(1)Ya) protein of Drosophila, statin, circumferin, and the MAN antigens. The experimental evidence indicates they are a diverse group of proteins, and that at least some have the potential to modulate the interactions of chromatin, lamins, and the nuclear membranes.Key words: nuclear envelope, lamina, YA protein, statin, circumferin.

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Unrestrained ESCRT-III drives chromosome fragmentation and micronuclear catastrophe

10.1101/517011 ◽

2019 ◽

Cited By ~ 8

Author(s):

Marina Vietri ◽

Sebastian W. Schultz ◽

Aurélie Bellanger ◽

Carl M. Jones ◽

Camilla Raiborg ◽

...

Keyword(s):

Nuclear Envelope ◽

Nuclear Membrane ◽

Genome Stability ◽

Membrane Deformation ◽

Chromosome Fragmentation ◽

Inner Nuclear Membrane ◽

Membrane Rupture ◽

Membrane Fission ◽

Stable Association ◽

Inner Nuclear Membrane Protein

AbstractThe ESCRT-III membrane fission machinery1,2 restores nuclear envelope integrity during mitotic exit3,4 and interphase5,6. Whereas primary nuclei resealing takes minutes, micronuclear envelope ruptures appear irreversible and result in catastrophic collapse associated with chromosome fragmentation and rearrangements (chromothripsis), thought to be a major driving force in cancer development7-10. Despite its importance11-13, the mechanistic underpinnings of nuclear envelope sealing in primary nuclei and the defects observed in micronuclei remain largely unknown. Here we show that CHMP7, the nucleator of ESCRT-III filaments at the nuclear envelope3,14, and the inner nuclear membrane protein LEMD215 act as a compartmentalization sensor detecting the loss of nuclear integrity. In cells with intact nuclear envelope, CHMP7 is actively excluded from the nucleus to preclude its binding to LEMD2. Nuclear influx of CHMP7 results in stable association with LEMD2 at the inner nuclear membrane that licenses local polymerization of ESCRT-III. Tight control of nuclear CHMP7 levels is critical, as induction of nuclear CHMP7 mutants is sufficient to induce unrestrained growth of ESCRT-III foci at the nuclear envelope, causing dramatic membrane deformation, local DNA torsional stress, single-stranded DNA formation and fragmentation of the underlying chromosomes. At micronuclei, membrane rupture is not associated with repair despite timely recruitment of ESCRT-III. Instead, micronuclei inherently lack the capacity to restrict accumulation of CHMP7 and LEMD2. This drives unrestrained ESCRT-III recruitment, membrane deformation and DNA defects that strikingly resemble those at primary nuclei upon induction of nuclear CHMP7 mutants. Preventing ESCRT-III recruitment suppresses membrane deformation and DNA damage, without restoring nucleocytoplasmic compartmentalization. We propose that the ESCRT-III nuclear integrity surveillance machinery is a double-edged sword, as its exquisite sensitivity ensures rapid repair at primary nuclei while causing unrestrained polymerization at micronuclei, with catastrophic consequences for genome stability16-18.

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Function and assembly of nuclear pore complex proteins

Biochemistry and Cell Biology ◽

10.1139/o99-038 ◽

1999 ◽

Vol 77 (4) ◽

pp. 321-329 ◽

Cited By ~ 14

Author(s):

Khaldon Bodoor ◽

Sarah Shaikh ◽

Paul Enarson ◽

Sharmin Chowdhury ◽

Davide Salina ◽

...

Keyword(s):

Membrane Protein ◽

Nuclear Envelope ◽

Nuclear Pore Complex ◽

Nuclear Membrane ◽

Current View ◽

Nuclear Pore ◽

Dynamic Component ◽

Inner Nuclear Membrane ◽

Inner Nuclear Membrane Protein ◽

Nuclear Membrane Protein

Nuclear pore complexes (NPCs) are extremely elaborate structures that mediate the bidirectional movement of macromolecules between the nucleus and cytoplasm. The current view of NPC organization features a massive symmetrical framework that is embedded in the double membranes of the nuclear envelope. It embraces a central channel of as yet ill-defined structure but which may accommodate particles with diameters up to 26 nm provided that they bear specific import/export signals. Attached to both faces of the central framework are peripheral structures, short cytoplasmic filaments, and a nuclear basket assembly, which interact with molecules transiting the NPC. The mechanisms of assembly and the nature of NPC structural intermediates are still poorly understood. However, mutagenesis and expression studies have revealed discrete sequences within certain NPC proteins that are necessary and sufficient for their appropriate targeting. In addition, some details are emerging from observations on cells undergoing mitosis where the nuclear envelope is disassembled and its components, including NPC subunits, are dispersed throughout the mitotic cytoplasm. At the end of mitosis, all of these components are reutilized to form nuclear envelopes in the two daughter cells. To date, it has been possible to define a time course of postmitotic assembly for a group of NPC components (CAN/Nup214, Nup153, POM121, p62 and Tpr) relative to the integral inner nuclear membrane protein LAP2 and the NPC membrane glycoprotein gp210. Nup153, a dynamic component of the nuclear basket, associates with chromatin towards the end of anaphase coincident with, although independent of, the inner nuclear membrane protein, LAP2. Assembly of the remaining proteins follows that of the nuclear membranes and occurs in the sequence POM121, p62, CAN/Nup214 and gp210/Tpr. Since p62 remains as a complex with three other NPC proteins (p58, p54, p45) during mitosis, and CAN/Nup214 maintains a similar interaction with its partner, Nup84, the relative timing of assembly of these additional four proteins may also be inferred. These observations suggest that there is a sequential association of NPC proteins with chromosomes during nuclear envelope reformation and the recruitment of at least eight of these precedes that of gp210. These findings support a model in which it is POM121 rather than gp210 that defines initial membrane-associated NPC assembly intermediates and which may therefore represent an essential component of the central framework of the NPC. Key words: nuclear pore complex, nucleoporin, mitosis, nuclear transport

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The fates of chicken nuclear lamin proteins during mitosis: evidence for a reversible redistribution of lamin B2 between inner nuclear membrane and elements of the endoplasmic reticulum.

The Journal of Cell Biology ◽

10.1083/jcb.107.2.397 ◽

1988 ◽

Vol 107 (2) ◽

pp. 397-406 ◽

Cited By ~ 49

Author(s):

R Stick ◽

B Angres ◽

C F Lehner ◽

E A Nigg

Keyword(s):

Endoplasmic Reticulum ◽

Nuclear Membrane ◽

Membrane Vesicles ◽

Soluble Form ◽

Lamin A ◽

Cell Fractionation ◽

Lamin B ◽

Inner Nuclear Membrane ◽

Nuclear Lamin ◽

Mitotic Cells

In chicken, three structurally distinct nuclear lamin proteins have been described. According to their migration on two-dimensional gels, these proteins have been designated as lamins A, B1, and B2. To investigate the functional relationship between chicken lamins and their mammalian counterparts, we have examined here the state of individual chicken lamin proteins during mitosis. Current models proposing functional specializations of mammalian lamin subtypes are in fact largely based on the observation that during mitosis mammalian lamin B remains associated with membrane vesicles, whereas lamins A and C become freely soluble. Cell fractionation experiments combined with immunoblotting show that during mitosis both chicken lamins B1 and B2 remain associated with membranes, whereas lamin A exists in a soluble form. In situ immunoelectron microscopy carried out on mitotic cells also reveals membrane association of lamin B2, whereas the distribution of lamin A is random. From these results we conclude that both chicken lamins B1 and B2 may functionally resemble mammalian lamin B. Interestingly, immunolabeling of mitotic cells revealed an association of lamin B2 with extended membrane cisternae that resembled elements of the endoplasmic reticulum. Quantitatively, we found that all large endoplasmic reticulum-like membranes present in metaphase cells were decorated with lamin B2-specific antibodies. Given that labeling of these mitotic membranes was lower than labeling of interphase nuclear envelopes, it appears likely that during mitotic disassembly and reassembly of the nuclear envelope lamin B2 may reversibly distribute between the inner nuclear membrane and the endoplasmic reticulum.

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Visualization of the Nuclear Lamina in Mouse Anterior Pituitary Cells and Immunocytochemical Detection of Lamin A/C by Quick-freeze Freeze-substitution Electron Microscopy

Journal of Histochemistry & Cytochemistry ◽

10.1369/jhc.4a6478.2005 ◽

2005 ◽

Vol 53 (4) ◽

pp. 497-507 ◽

Cited By ~ 17

Author(s):

Takao Senda ◽

Akiko Iizuka-Kogo ◽

Atsushi Shimomura

Keyword(s):

Electron Microscopy ◽

Nuclear Membrane ◽

Anterior Pituitary ◽

Freeze Substitution ◽

Nuclear Lamina ◽

Immunogold Electron Microscopy ◽

Lamin A ◽

Pituitary Cells ◽

Inner Nuclear Membrane ◽

Anterior Pituitary Cells

We examined the nuclear lamina in the quickly frozen anterior pituitary cells by electron microscopic techniques combined with freeze substitution, deep etching, and immunocytochemistry and compared it with that in the chemically fixed cells. By quick-freeze freeze-substitution electron microscopy, an electron-lucent layer, as thick as 20 nm, was revealed just inside the inner nuclear membrane, whereas in the conventionally glutaraldehyde-fixed cells the layer was not seen. By quick-freeze deep-etch electron microscopy, we could not distinguish definitively the layer corresponding to the nuclear lamina in either fresh unfixed or glutaraldehyde-fixed cells. Immunofluorescence microscopy showed that lamin A/C in the nucleus was detected in the acetone-fixed cells and briefly in paraformaldehyde-fixed cells but not in the cells with prolonged paraformaldehyde fixation. Nuclear localization of lamin A/C was revealed by immunogold electron microscopy also in the quickly frozen and freeze-substituted cells, but not in the paraformaldehyde-fixed cells. Lamin A/C was localized mainly in the peripheral nucleoplasm within 60 nm from the inner nuclear membrane, which corresponded to the nuclear lamina. These results suggest that the nuclear lamina can be preserved both ultrastructurally and immunocytochemically by quick-freezing fixation, rather than by conventional chemical fixation.

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Fluorescent Labeling of the Nuclear Envelope by Localizing Green Fluorescent Protein on the Inner Nuclear Membrane

ACS Chemical Biology ◽

10.1021/acschembio.8b00219 ◽

2018 ◽

Vol 13 (6) ◽

pp. 1463-1469 ◽

Cited By ~ 1

Author(s):

Toshiyuki Taniyama ◽

Natsumi Tsuda ◽

Shinji Sueda

Keyword(s):

Green Fluorescent Protein ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Fluorescent Protein ◽

Fluorescent Labeling ◽

Inner Nuclear Membrane ◽

Green Fluorescent

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SUN-1 and ZYG-12, Mediators of Centrosome–Nucleus Attachment, Are a Functional SUN/KASH Pair in Caenorhabditis elegans

Molecular Biology of the Cell ◽

10.1091/mbc.e08-10-1034 ◽

2009 ◽

Vol 20 (21) ◽

pp. 4586-4595 ◽

Cited By ~ 45

Author(s):

IL Minn ◽

Melissa M. Rolls ◽

Wendy Hanna-Rose ◽

Christian J. Malone

Keyword(s):

Caenorhabditis Elegans ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Coiled Coil ◽

Physical Interaction ◽

Type Ii ◽

Inner Nuclear Membrane ◽

Sequence Elements ◽

Inner Nuclear Membrane Protein ◽

Sun Domain

Klarsicht/ANC-1/Syne/homology (KASH)/Sad-1/UNC-84 (SUN) protein pairs can act as connectors between cytoplasmic organelles and the nucleoskeleton. Caenorhabditis elegans ZYG-12 and SUN-1 are essential for centrosome–nucleus attachment. Although SUN-1 has a canonical SUN domain, ZYG-12 has a divergent KASH domain. Here, we establish that the ZYG-12 mini KASH domain is functional and, in combination with a portion of coiled-coil domain, is sufficient for nuclear envelope localization. ZYG-12 and SUN-1 are hypothesized to be outer and inner nuclear membrane proteins, respectively, and to interact, but neither their topologies nor their physical interaction has been directly investigated. We show that ZYG-12 is a type II outer nuclear membrane (ONM) protein and that SUN-1 is a type II inner nuclear membrane protein. The proteins interact in the luminal space of the nuclear envelope via the ZYG-12 mini KASH domain and a region of SUN-1 that does not include the SUN domain. SUN-1 is hypothesized to restrict ZYG-12 to the ONM, preventing diffusion through the endoplasmic reticulum. We establish that ZYG-12 is indeed immobile at the ONM by using fluorescence recovery after photobleaching and show that SUN-1 is sufficient to localize ZYG-12 in cells. This work supports current models of KASH/SUN pairs and highlights the diversity in sequence elements defining KASH domains.

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