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

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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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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Internuclear exchange of an inner nuclear membrane protein (p55) in heterokaryons: in vivo evidence for the interaction of p55 with the nuclear lamina.

The Journal of Cell Biology ◽

10.1083/jcb.111.6.2225 ◽

1990 ◽

Vol 111 (6) ◽

pp. 2225-2234 ◽

Cited By ~ 78

Author(s):

L Powell ◽

B Burke

Keyword(s):

Nuclear Membrane ◽

Lateral Diffusion ◽

Nuclear Lamina ◽

Membrane System ◽

Mouse Cell ◽

Nuclear Pore ◽

Nuclear Pore Complexes ◽

Inner Nuclear Membrane ◽

Pore Complexes

The movement between nuclei of an integral protein of the inner nuclear membrane has been studied in rat/mouse and rat/hamster heterokaryons. This protein, p55, was found to equilibrate between nuclei over a period of approximately 6 h in the absence of new protein synthesis. When rat/mouse heterokaryons were constructed using an undifferentiated murine embryonal carcinoma (P19), which lacks lamins A and C, no accumulation of p55 in the mouse cell nucleus was observed. However, P19 nuclei could be rendered competent to accumulate p55 by transfecting the parent cells with human lamin A before cell fusion, supporting the notion that p55 may interact with the nuclear lamina. Since p55 does not appear to be able to dissociate from the nuclear membrane, it is concluded that this exchange between nuclei does not occur in the aqueous phase and instead is probably membrane mediated. It is proposed that this protein may be free to move between the inner and outer nuclear membranes via the continuities at the nuclear pore complexes and that transfer between nuclei occurs via lateral diffusion through the peripheral ER, which appears to form a single continuous membrane system in these heterokaryons. One implication of these observations is that accumulation of at least some integral proteins in the inner nuclear membrane may be mediated by interactions with other nuclear components and may not require a single defined targeting sequence.

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SINC, a type III secreted protein of Chlamydia psittaci, targets the inner nuclear membrane of infected cells and uninfected neighbors

Molecular Biology of the Cell ◽

10.1091/mbc.e14-11-1530 ◽

2015 ◽

Vol 26 (10) ◽

pp. 1918-1934 ◽

Cited By ~ 35

Author(s):

Sergio A. Mojica ◽

Kelley M. Hovis ◽

Matthew B. Frieman ◽

Bao Tran ◽

Ru-ching Hsia ◽

...

Keyword(s):

Nuclear Envelope ◽

Nuclear Membrane ◽

Nuclear Lamina ◽

Chlamydia Psittaci ◽

Hek293 Cells ◽

Secreted Protein ◽

Inner Nuclear Membrane ◽

Type Iii ◽

Infected Cells ◽

Digitonin Permeabilization

SINC, a new type III secreted protein of the avian and human pathogen Chlamydia psittaci, uniquely targets the nuclear envelope of C. psittaci–infected cells and uninfected neighboring cells. Digitonin-permeabilization studies of SINC-GFP–transfected HeLa cells indicate that SINC targets the inner nuclear membrane. SINC localization at the nuclear envelope was blocked by importazole, confirming SINC import into the nucleus. Candidate partners were identified by proximity to biotin ligase-fused SINC in HEK293 cells and mass spectrometry (BioID). This strategy identified 22 candidates with high confidence, including the nucleoporin ELYS, lamin B1, and four proteins (emerin, MAN1, LAP1, and LBR) of the inner nuclear membrane, suggesting that SINC interacts with host proteins that control nuclear structure, signaling, chromatin organization, and gene silencing. GFP-SINC association with the native LEM-domain protein emerin, a conserved component of nuclear “lamina” structure, or with a complex containing emerin was confirmed by GFP pull down. Our findings identify SINC as a novel bacterial protein that targets the nuclear envelope with the capability of globally altering nuclear envelope functions in the infected host cell and neighboring uninfected cells. These properties may contribute to the aggressive virulence of C. psittaci.

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Assembly/disassembly of the nuclear envelope membrane: Cell cycle-dependent binding of nuclear membrane vesicles to chromatin in vitro

Cell ◽

10.1016/0092-8674(91)90155-r ◽

1991 ◽

Vol 65 (2) ◽

pp. 209-217 ◽

Cited By ~ 68

Author(s):

Rupert Pfaller ◽

Carl Smythe ◽

John W. Newport

Keyword(s):

Cell Cycle ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Membrane Vesicles ◽

Envelope Membrane ◽

Cycle Dependent ◽

Membrane Cell

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Sequential PKC- and Cdc2-mediated phosphorylation events elicit zebrafish nuclear envelope disassembly

Journal of Cell Science ◽

10.1242/jcs.112.6.977 ◽

1999 ◽

Vol 112 (6) ◽

pp. 977-987 ◽

Cited By ~ 2

Author(s):

P. Collas

Keyword(s):

Nuclear Envelope ◽

Nuclear Membrane ◽

Nuclear Lamina ◽

Cdc2 Kinase ◽

Lamin B ◽

Inner Nuclear Membrane ◽

Nuclear Envelope Breakdown ◽

Simultaneous Inhibition ◽

Integral Proteins

Molecular markers of the zebrafish inner nuclear membrane (NEP55) and nuclear lamina (L68) were identified, partially characterized and used to demonstrate that disassembly of the zebrafish nuclear envelope requires sequential phosphorylation events by first PKC, then Cdc2 kinase. NEP55 and L68 are immunologically and functionally related to human LAP2beta and lamin B, respectively. Exposure of zebrafish nuclei to meiotic cytosol elicits rapid phosphorylation of NEP55 and L68, and disassembly of both proteins. L68 phosphorylation is completely inhibited by simultaneous inhibition of Cdc2 and PKC and only partially blocked by inhibition of either kinase. NEP55 phosphorylation is completely prevented by inhibition or immunodepletion of cytosolic Cdc2. Inhibition of cAMP-dependent kinase, MEK or CaM kinase II does not affect NEP55 or L68 phosphorylation. In vitro, nuclear envelope disassembly requires phosphorylation of NEP55 and L68 by both mammalian PKC and Cdc2. Inhibition of either kinase is sufficient to abolish NE disassembly. Furthermore, novel two-step phosphorylation assays in cytosol and in vitro indicate that PKC-mediated phosphorylation of L68 prior to Cdc2-mediated phosphorylation of L68 and NEP55 is essential to elicit nuclear envelope breakdown. Phosphorylation elicited by Cdc2 prior to PKC prevents nuclear envelope disassembly even though NEP55 is phosphorylated. The results indicate that sequential phosphorylation events elicited by PKC, followed by Cdc2, are required for zebrafish nuclear disassembly. They also argue that phosphorylation of inner nuclear membrane integral proteins is not sufficient to promote nuclear envelope breakdown, and suggest a multiple-level regulation of disassembly of nuclear envelope components during meiosis and at mitosis.

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Fibroblasts lacking nuclear lamins do not have nuclear blebs or protrusions but nevertheless have frequent nuclear membrane ruptures

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1812622115 ◽

2018 ◽

Vol 115 (40) ◽

pp. 10100-10105 ◽

Cited By ~ 20

Author(s):

Natalie Y. Chen ◽

Paul Kim ◽

Thomas A. Weston ◽

Lovelyn Edillo ◽

Yiping Tu ◽

...

Keyword(s):

Dna Damage ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Membrane Integrity ◽

Nuclear Lamina ◽

Virtual Absence ◽

Inner Nuclear Membrane ◽

Nuclear Lamins ◽

Transmission Electron ◽

Nuclear Lamin

The nuclear lamina, an intermediate filament meshwork lining the inner nuclear membrane, is formed by the nuclear lamins (lamins A, C, B1, and B2). Defects or deficiencies in individual nuclear lamin proteins have been reported to elicit nuclear blebs (protrusions or outpouchings of the nuclear envelope) and increase susceptibility for nuclear membrane ruptures. It is unclear, however, how a complete absence of nuclear lamins would affect nuclear envelope morphology and nuclear membrane integrity (i.e., whether nuclear membrane blebs or protrusions would occur and, if not, whether cells would be susceptible to nuclear membrane ruptures). To address these issues, we generated mouse embryonic fibroblasts (MEFs) lacking all nuclear lamins. The nuclear lamin-deficient MEFs had irregular nuclear shapes but no nuclear blebs or protrusions. Despite a virtual absence of nuclear blebs, MEFs lacking nuclear lamins had frequent, prolonged, and occasionally nonhealing nuclear membrane ruptures. By transmission electron microscopy, the inner nuclear membrane in nuclear lamin-deficient MEFs have a “wavy” appearance, and there were discrete discontinuities in the inner and outer nuclear membranes. Nuclear membrane ruptures were accompanied by a large increase in DNA damage, as judged by γ-H2AX foci. Mechanical stress increased both nuclear membrane ruptures and DNA damage, whereas minimizing transmission of cytoskeletal forces to the nucleus had the opposite effects.

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Loss of a-Type Lamin Expression Compromises Nuclear Envelope Integrity Leading to Muscular Dystrophy

The Journal of Cell Biology ◽

10.1083/jcb.147.5.913 ◽

1999 ◽

Vol 147 (5) ◽

pp. 913-920 ◽

Cited By ~ 787

Author(s):

Teresa Sullivan ◽

Diana Escalante-Alcalde ◽

Harshida Bhatt ◽

Miriam Anver ◽

Narayan Bhat ◽

...

Keyword(s):

Muscular Dystrophy ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Mammalian Cells ◽

Nuclear Architecture ◽

Nuclear Lamina ◽

Postnatal Growth ◽

Developmentally Regulated ◽

Inner Nuclear Membrane ◽

Cardiac Muscles

The nuclear lamina is a protein meshwork lining the nucleoplasmic face of the inner nuclear membrane and represents an important determinant of interphase nuclear architecture. Its major components are the A- and B-type lamins. Whereas B-type lamins are found in all mammalian cells, A-type lamin expression is developmentally regulated. In the mouse, A-type lamins do not appear until midway through embryonic development, suggesting that these proteins may be involved in the regulation of terminal differentiation. Here we show that mice lacking A-type lamins develop to term with no overt abnormalities. However, their postnatal growth is severely retarded and is characterized by the appearance of muscular dystrophy. This phenotype is associated with ultrastructural perturbations to the nuclear envelope. These include the mislocalization of emerin, an inner nuclear membrane protein, defects in which are implicated in Emery-Dreifuss muscular dystrophy (EDMD), one of the three major X-linked dystrophies. Mice lacking the A-type lamins exhibit tissue-specific alterations to their nuclear envelope integrity and emerin distribution. In skeletal and cardiac muscles, this is manifest as a dystrophic condition related to EDMD.

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Cell cycle-dependent changes in the dynamics of MAP 2 and MAP 4 in cultured cells.

The Journal of Cell Biology ◽

10.1083/jcb.109.1.211 ◽

1989 ◽

Vol 109 (1) ◽

pp. 211-223 ◽

Cited By ~ 21

Author(s):

J B Olmsted ◽

D L Stemple ◽

W M Saxton ◽

B W Neighbors ◽

J R McIntosh

Keyword(s):

Cell Cycle ◽

Cultured Cells ◽

Cold Treatment ◽

Light Level ◽

Microtubule Associated Proteins ◽

Interphase Cells ◽

Associated Proteins ◽

Cycle Dependent ◽

And Control

To examine the behavior of microtubule-associated proteins (MAPs) in living cells, MAP 4 and MAP 2 have been derivatized with 6-iodoacetamido-fluorescein, and the distribution of microinjected MAP has been analyzed using a low light level video system and fluorescence redistribution after photobleaching. Within 1 min following microinjection of fluoresceinated MAP 4 or MAP 2, fluorescent microtubule arrays were visible in interphase or mitotic PtK1 cells. After cold treatment of fluorescent MAP 2-containing cells (3 h, 4 degrees C), microtubule fluorescence disappeared, and the only fluorescence above background was located at the centrosomes; microtubule patterns returned upon warming. Loss of microtubule immunofluorescence after nocodozole treatment was similar in MAP-injected and control cells, suggesting that injected fluorescein-labeled MAP 2 did not stabilize microtubules. The dynamics of the MAPs were examined further by FRAP. FRAP analysis of interphase cells demonstrated that MAP 2 redistributed with half-times slightly longer (60 +/- 25 s) than those for MAP 4 (44 +/- 20 s), but both types of MAPs bound to microtubules in vivo exchanged with soluble MAPs at rates exceeding the rate of tubulin turnover. These data imply that microtubules in interphase cells are assembled with constantly exchanging populations of MAP. Metaphase cells at 37 degrees C or 26 degrees C showed similar mean redistribution half-times for both MAP 2 and MAP 4; these were 3-4 fold faster than the interphase rates (MAP 2, t1/2 = 14 +/- 6 s; MAP 4, t1/2 = 17 +/- 5 s). The extent of recovery of spindle fluorescence in MAP-injected cells was to 84-94% at either 26 or 37 degrees C. Although most metaphase tubulin, like the MAPs, turns over rapidly and completely under physiologic conditions, published work shows either reduced rates or extents of turnover at 26 degrees C, suggesting that the fast mitotic MAP exchange is not simply because of fast tubulin turnover. Exchange of MAP 4 bound to telophase midbodies occurred with dynamics comparable to those seen in metaphase spindles (t1/2 = approximately 27 s) whereas midbody tubulin exchange was slow (greater than 300 s). These data demonstrate that the rate of MAP exchange on microtubules is a function of time in the cell cycle.

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

Molecular Biology of the Cell ◽

10.1091/mbc.e17-03-0138 ◽

2017 ◽

Vol 28 (17) ◽

pp. 2241-2250 ◽

Cited By ~ 21

Author(s):

Birendra KC ◽

Danielle G. May ◽

Benjamin V. Benson ◽

Dae In Kim ◽

Winnie G. Shivega ◽

...

Keyword(s):

Cell Cycle ◽

Nuclear Envelope ◽

Nuclear Membrane ◽

Binding Protein ◽

Chromatin Organization ◽

Lamin A ◽

Chromatin Binding ◽

Cellular Functions ◽

Inner Nuclear Membrane ◽

Subcellular Compartments

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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Distinct In Vivo Dynamics of Vertebrate SUMO Paralogues

Molecular Biology of the Cell ◽

10.1091/mbc.e04-07-0589 ◽

2004 ◽

Vol 15 (12) ◽

pp. 5208-5218 ◽

Cited By ~ 138

Author(s):

Ferhan Ayaydin ◽

Mary Dasso

Keyword(s):

Cell Cycle ◽

Nuclear Envelope ◽

Cell Lines ◽

Nuclear Membrane ◽

Fluorescent Protein ◽

Yellow Fluorescent Protein ◽

Late Anaphase ◽

Patterns Of Utilization

There are three mammalian SUMO paralogues: SUMO-1 is ∼45% identical to SUMO-2 and SUMO-3, which are 96% identical to each other. It is currently unclear whether SUMO-1, -2, and -3 function in ways that are unique, redundant, or antagonistic. To address this question, we examined the dynamics of individual SUMO paralogues by using cell lines that stably express each of the mammalian SUMO proteins fused to the yellow fluorescent protein (YFP). Whereas SUMO-2 and -3 showed very similar distributions throughout the nucleoplasm, SUMO-1 was uniquely distributed to the nuclear envelope and to the nucleolus. Photobleaching experiments revealed that SUMO-1 dynamics was much slower than SUMO-2 and -3 dynamics. Additionally, the mobility of SUMO paralogues differed between subnuclear structures. Finally, the timing and distributions were dissimilar between paralogues as cells exited from mitosis. SUMO-1 was recruited to nuclear membrane as nuclear envelopes reformed in late anaphase, and accumulated rapidly into the nucleus. SUMO-2 and SUMO-3 localized to chromosome earlier and accumulated gradually during telophase. Together, these findings demonstrate that mammalian SUMO-1 shows patterns of utilization that are clearly discrete from the patterns of SUMO-2 and -3 throughout the cell cycle, arguing that it is functionally distinct and specifically regulated in vivo.

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