Cytoplasmic control of nuclear assembly

The reconstitution of a replication-competent, transcriptionally active nucleus following mitosis, fertilization or nuclear transplantation involves a stepwise series of reactions, most (if not all) of which are controlled by the cytoplasmic environment. This review discusses the nature of cytoplasmic contributions to the development of the male pronucleus at fertilization, and the effect of altering the cytoplasmic environment on nuclear assembly. The system used to investigate these regulations consists of permeabilized sea urchin sperm nuclei incubated under controlled conditions in a cell-free extract of fertilized sea urchin eggs. (1) In egg cytoplasmic extract, male pronuclear formation is initiated by the disassembly of the sperm nuclear lamina as a result of lamin phosphorylation by a cytosolic protein kinase C. (2) Sperm histones are phosphorylated by an as yet unidentified soluble kinase. (3) The conical sperm nucleus decondenses into a spherical pronucleus in an ATP-and cytosolic pH-dependent manner. (4) Chromatin decondensation is associated with the replacement of sperm histones by maternal histones. (5) Nuclear membranes form by ATP-dependent binding of vesicles to chromatin and GTP-dependent fusion of these vesicles to one another. (6) Three cytoplasmic vesicle populations with distinct biochemical, chromatin-binding and fusion properties are required for nuclear envelope assembly. (7) Targeting of the bulk of nuclear membrane vesicles to chromatin is mediated by an integral membrane protein similar to human lamin B receptor. (8) The last step of male pronuclear formation, nuclear swelling, is promoted by the assembly of nuclear pores, nuclear import of soluble lamins and growth of the nuclear membranes. (9) Once inside the nucleus, lamin B associates with lamin B receptors, presumably to tether the inner nuclear membrane with the lamina. Overall, these processes are similar to those characterizing nuclear reconstitution after mitosis in somatic cells or nuclear remodeling following transplantation into oocytes or eggs. The influence of the egg cytoplasmic environment on some aspects of nuclear remodeling after nuclear transplantation is also discussed.

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Nuclear envelope disassembly in mitotic extract requires functional nuclear pores and a nuclear lamina

Journal of Cell Science ◽

10.1242/jcs.111.9.1293 ◽

1998 ◽

Vol 111 (9) ◽

pp. 1293-1303 ◽

Cited By ~ 6

Author(s):

P. Collas

Keyword(s):

Nuclear Envelope ◽

Sea Urchin ◽

Nuclear Membrane ◽

Critical Role ◽

Nuclear Lamina ◽

Nuclear Pore ◽

Nuclear Pores ◽

Lamin B ◽

Nuclear Membranes

Using sea urchin embryonic and in-vitro-assembled nuclei incubated in sea urchin mitotic extract, I provide evidence for a requirement for functional nuclear pores and a nuclear lamina for nuclear envelope disassembly in vitro. In interphase gastrula nuclei, lamin B interacts with p56, an integral protein of inner nuclear membrane cross-reacting with antibodies to human lamin B receptor. Incubation of gastrula nuclei in mitotic cytosol containing an ATP-generating system rapidly induces hyperphosphorylation of p56 and lamin B. Subsequently, p56-lamin B interactions are weakened and the two proteins segregate into distinct nuclear envelope-derived vesicles upon disassembly of nuclear membranes and of the lamina. Nuclear disassembly is accompanied by chromatin condensation. Blocking nuclear pore function with wheat germ agglutinin or antibodies to nucleoporins prevents p56 and lamin B hyperphosphorylation, nuclear membrane breakdown and lamina solubilization. These events are not rescued by permeabilization of nuclear membranes to molecules of 150, 000 Mr with lysolecithin. In-vitro-assembled nuclei containing nuclear membranes with functional pores but no lamina do not disassemble in mitotic cytosol in spite of p56 hyperphosphorylation. Nuclear import of soluble lamin B and reformation of a lamina in interphase extract restores nuclear disassembly in mitotic cytosol. The data indicate a role for functional nuclear pores in nuclear disassembly in vitro. They show that p56 hyperphosphorylation is not sufficient for nuclear membrane disassembly in mitotic cytosol and argue that the nuclear lamina plays a critical role in nuclear disassembly at mitosis.

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Targeting of membranes to sea urchin sperm chromatin is mediated by a lamin B receptor-like integral membrane protein.

The Journal of Cell Biology ◽

10.1083/jcb.135.6.1715 ◽

1996 ◽

Vol 135 (6) ◽

pp. 1715-1725 ◽

Cited By ~ 72

Author(s):

P Collas ◽

J C Courvalin ◽

D Poccia

Keyword(s):

Membrane Protein ◽

Nuclear Envelope ◽

Sea Urchin ◽

Binding Capacity ◽

Integral Membrane Protein ◽

Sperm Chromatin ◽

Lamin B ◽

Lamin B Receptor ◽

Pronuclear Formation

We have identified an integral membrane protein of sea urchin gametes with an apparent molecular mass of 56 kD that cross-reacts with an antibody against the nucleoplasmic NH2-terminal domain of human lamin B receptor (LBR). In mature sperm, p56 is located at the tip and base of the nucleus from where it is removed by egg cytosol in vitro. In the egg, p56 is present in a subset of cytoplasmic membranes (MV2 beta) which contributes the bulk of the nuclear envelope during male pronuclear formation. p56-containing vesicles are required for nuclear envelope assembly and have a chromatin-binding capacity that is mediated by p56. Lamin B is not present in these vesicles and is imported into the nucleus from a soluble pool at a later stage of pronuclear formation. Lamin B incorporation and addition of new membranes are necessary for pronuclear swelling and nuclear envelope growth. We suggest that p56 is a sea urchin LBR homologue that targets membranes to chromatin and later anchors the membrane to the lamina.

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Assembly of the nuclear pore: biochemically distinct steps revealed with NEM, GTP gamma S, and BAPTA.

The Journal of Cell Biology ◽

10.1083/jcb.132.1.5 ◽

1996 ◽

Vol 132 (1) ◽

pp. 5-20 ◽

Cited By ~ 120

Author(s):

C Macaulay ◽

D J Forbes

Keyword(s):

Nuclear Membrane ◽

Vesicle Fusion ◽

Nuclear Pore ◽

Nuclear Pores ◽

Nuclear Assembly ◽

Nuclear Membranes ◽

Nuclear Pore Assembly ◽

Gamma S ◽

Nuclear Reconstitution

A key event in nuclear formation is the assembly of functional nuclear pores. We have used a nuclear reconstitution system derived from Xenopus eggs to examine the process of nuclear pore assembly in vitro. With this system, we have identified three reagents which interfere with nuclear pore assembly, NEM, GTP gamma S, and the Ca++ chelator, BAPTA. These reagents have allowed us to determine that the assembly of a nuclear pore requires the prior assembly of a double nuclear membrane. Inhibition of nuclear vesicle fusion by pretreatment of the membrane vesicle fraction with NEM blocks pore complex assembly. In contrast, NEM treatment of already fused double nuclear membranes does not block pore assembly. This indicates that NEM inhibits a single step in pore assembly--the initial fusion of vesicles required to form a double nuclear membrane. The presence of GTP gamma S blocks pore assembly at two distinct steps, first by preventing fusion between nuclear vesicles, and second by blocking a step in pore assembly that occurs on already fused double nuclear membranes. Interestingly, when the Ca2+ chelator BAPTA is added to a nuclear assembly reaction, it only transiently blocks nuclear vesicle fusion, but completely blocks nuclear pore assembly. This results in the formation of a nucleus surrounded by a double nuclear membrane, but devoid of nuclear pores. To order the positions at which GTP gamma S and BAPTA interfere with pore assembly, a novel anchored nuclear assembly assay was developed. This assay revealed that the BAPTA-sensitive step in pore assembly occurs after the second GTP gamma S-sensitive step. Thus, through use of an in vitro nuclear reconstitution system, it has been possible to biochemically define and order multiple steps in nuclear pore assembly.

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Live fluorescence imaging reveals early recruitment of emerin, LBR, RanBP2, and Nup153 to reforming functional nuclear envelopes

Journal of Cell Science ◽

10.1242/jcs.113.5.779 ◽

2000 ◽

Vol 113 (5) ◽

pp. 779-794 ◽

Cited By ~ 14

Author(s):

T. Haraguchi ◽

T. Koujin ◽

T. Hayakawa ◽

T. Kaneda ◽

C. Tsutsumi ◽

...

Keyword(s):

Nuclear Pore Complex ◽

Nuclear Membrane ◽

Nuclear Import ◽

Nuclear Pore ◽

Simultaneous Observation ◽

Lamin B ◽

Nuclear Membranes ◽

Lamin B Receptor ◽

The Times ◽

Early Recruitment

We determined the times when the nuclear membrane, nuclear pore complex (NPC) components, and nuclear import function were recovered during telophase in living HeLa cells. Simultaneous observation of fluorescently-labeled NLS-bearing proteins, lamin B receptor (LBR)-GFP, and Hoechst33342-stained chromosomes revealed that nuclear membranes reassembled around chromosomes by 5 minutes after the onset of anaphase (early telophase) whereas nuclear import function was recovered later, at 8 minutes. GFP-tagged emerin also accumulated on chromosomes 5 minutes after the onset of anaphase. Interestingly, emerin and LBR initially accumulated at distinct, separate locations, but then became uniform 8 minutes after the onset of anaphase, concurrent with the recovery of nuclear import function. We further determined the timing of NPC assembly by immunofluorescence staining of cells fixed at precise times after the onset of anaphase. Taken together, these results showed that emerin, LBR, and several NPC components (RanBP2, Nup153, p62), but not Tpr, reconstitute around chromosomes very early in telophase prior to the recovery of nuclear import activity.

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Lamin B receptor: role on chromatin structure, cellular senescence and possibly aging

Biochemical Journal ◽

10.1042/bcj20200165 ◽

2020 ◽

Vol 477 (14) ◽

pp. 2715-2720

Author(s):

Susana Castro-Obregón

Keyword(s):

Cellular Senescence ◽

Nuclear Membrane ◽

Chromatin Structure ◽

Cholesterol Synthesis ◽

Reductase Activity ◽

Chimeric Protein ◽

Nuclear Lamina ◽

Lamin B ◽

Inner Nuclear Membrane ◽

Lamin B Receptor

The nuclear envelope is composed by an outer nuclear membrane and an inner nuclear membrane, which is underlain by the nuclear lamina that provides the nucleus with mechanical strength for maintaining structure and regulates chromatin organization for modulating gene expression and silencing. A layer of heterochromatin is beneath the nuclear lamina, attached by inner nuclear membrane integral proteins such as Lamin B receptor (LBR). LBR is a chimeric protein, having also a sterol reductase activity with which it contributes to cholesterol synthesis. Lukasova et al. showed that when DNA is damaged by ɣ-radiation in cancer cells, LBR is lost causing chromatin structure changes and promoting cellular senescence. Cellular senescence is characterized by terminal cell cycle arrest and the expression and secretion of various growth factors, cytokines, metalloproteinases, etc., collectively known as senescence-associated secretory phenotype (SASP) that cause chronic inflammation and tumor progression when they persist in the tissue. Therefore, it is fundamental to understand the molecular basis for senescence establishment, maintenance and the regulation of SASP. The work of Lukasova et al. contributed to our understanding of cellular senescence establishment and provided the basis that lead to the further discovery that chromatin changes caused by LBR reduction induce an up-regulated expression of SASP factors. LBR dysfunction has relevance in several diseases and possibly in physiological aging. The potential bifunctional role of LBR on cellular senescence establishment, namely its role in chromatin structure together with its enzymatic activity contributing to cholesterol synthesis, provide a new target to develop potential anti-aging therapies.

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Nicotine Induces Polyspermy in Sea Urchin Eggs through a Non-Cholinergic Pathway Modulating Actin Dynamics

Cells ◽

10.3390/cells9010063 ◽

2019 ◽

Vol 9 (1) ◽

pp. 63 ◽

Cited By ~ 1

Author(s):

Nunzia Limatola ◽

Filip Vasilev ◽

Luigia Santella ◽

Jong Tai Chun

Keyword(s):

Sea Urchin ◽

Nicotinic Acetylcholine Receptors ◽

Acetylcholine Receptors ◽

Molecular Mechanisms ◽

Actin Dynamics ◽

Dependent Manner ◽

Animal Cells ◽

Sea Urchin Eggs ◽

Cholinergic Pathway ◽

Dose Dependent

While alkaloids often exert unique pharmacological effects on animal cells, exposure of sea urchin eggs to nicotine causes polyspermy at fertilization in a dose-dependent manner. Here, we studied molecular mechanisms underlying the phenomenon. Although nicotine is an agonist of ionotropic acetylcholine receptors, we found that nicotine-induced polyspermy was neither mimicked by acetylcholine and carbachol nor inhibited by specific antagonists of nicotinic acetylcholine receptors. Unlike acetylcholine and carbachol, nicotine uniquely induced drastic rearrangement of egg cortical microfilaments in a dose-dependent way. Such cytoskeletal changes appeared to render the eggs more receptive to sperm, as judged by the significant alleviation of polyspermy by latrunculin-A and mycalolide-B. In addition, our fluorimetric assay provided the first evidence that nicotine directly accelerates polymerization kinetics of G-actin and attenuates depolymerization of preassembled F-actin. Furthermore, nicotine inhibited cofilin-induced disassembly of F-actin. Unexpectedly, our results suggest that effects of nicotine can also be mediated in some non-cholinergic pathways.

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ELECTRON MICROSCOPY OF THE NUCLEAR MEMBRANE OF AMOEBA PROTEUS

The Journal of Cell Biology ◽

10.1083/jcb.2.4.445 ◽

1956 ◽

Vol 2 (4) ◽

pp. 445-448 ◽

Cited By ~ 60

Author(s):

Marie H. Greider ◽

Wencel J. Kostir ◽

Walter J. Frajola

Keyword(s):

Electron Microscopy ◽

Electron Microscope ◽

Nuclear Membrane ◽

Outer Layer ◽

Microscope Study ◽

Electron Microscope Study ◽

Cell Types ◽

Amoeba Proteus ◽

Nuclear Membranes ◽

Thin Sectioning

An electron microscope study of the nuclear membrane of Amoeba proteus by thin sectioning techniques has revealed an ultrastructure in the outer layer of the membrane that is homologous to the pores and annuli observed in the nuclear membranes of many other cell types studied by these techniques. An inner honeycombed layer apparently unique to Amoeba proteus is also described.

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Enucleation of Sea-Urchin Blastomeres with or without Removal of Asters

Journal of Cell Science ◽

10.1242/jcs.s3-93.24.475 ◽

1952 ◽

Vol s3-93 (24) ◽

pp. 475-486

Author(s):

I. JOAN LORCH

Keyword(s):

Sea Urchin ◽

Nuclear Membrane ◽

Cell Stage ◽

Sea Urchin Egg ◽

In Cells

The following experiments were carried out on one blastomere at the two-cell stage of the sea-urchin egg: 1. Removal of the nucleus. 2. Removal of the nucleus and surrounding cytoplasm (centrosphere). 3. Attempted removal of the centrosphere only. In cells from which the nucleus had been removed the asters multiplied for up to 7 hours and then disappeared. During the period of aster multiplication, cleavage furrows often appeared between the asters but did not succeed in dividing the cell. After about 8 hours, cleavage into a large number of spheroidal cells occurred. When the nucleus and centrosphere were removed no asters were formed and no cleavage furrows were observed until after about 8 hours, when division into a large number of spheroidal cells occurred. When attempts were made to remove the centrosphere, leaving the nucleus intact, asters were always eventually re-formed Before the re-formation of asters neither the nucleus nor the cytoplasm divided although dissolution of the nuclear membrane, followed by its reappearance, occurred. After re-formation of the asters cleavage appeared to be normal.

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Endoplasmic reticulum-to-Golgi transitions upon herpes virus infection

F1000Research ◽

10.12688/f1000research.12252.2 ◽

2018 ◽

Vol 6 ◽

pp. 1804 ◽

Cited By ~ 5

Author(s):

Peter Wild ◽

Andres Kaech ◽

Elisabeth M. Schraner ◽

Ladina Walser ◽

Mathias Ackermann

Keyword(s):

Endoplasmic Reticulum ◽

Nuclear Envelope ◽

Golgi Complex ◽

Nuclear Membrane ◽

Progeny Virus ◽

Cytoplasmic Matrix ◽

Outer Nuclear Membrane ◽

Nuclear Membranes ◽

Perinuclear Space ◽

Hsv 1

Background: Herpesvirus capsids are assembled in the nucleus, translocated to the perinuclear space by budding, acquiring tegument and envelope, or released to the cytoplasm via impaired nuclear envelope. One model proposes that envelopment, “de-envelopment” and “re-envelopment” is essential for production of infectious virus. Glycoproteins gB/gH were reported to be essential for de-envelopment, by fusion of the “primary” envelope with the outer nuclear membrane. Yet, a high proportion of enveloped virions generated from genomes with deleted gB/gH were found in the cytoplasm and extracellular space, suggesting the existence of alternative exit routes.Methods: We investigated the relatedness between the nuclear envelope and membranes of the endoplasmic reticulum and Golgi complex, in cells infected with either herpes simplex virus 1 (HSV-1) or a Us3 deletion mutant thereof, or with bovine herpesvirus 1 (BoHV-1) by transmission and scanning electron microscopy, employing freezing technique protocols.Results: The Golgi complex is a compact entity in a juxtanuclear position covered by a membrane on thecisface. Golgi membranes merge with membranes of the endoplasmic reticulum forming an entity with the perinuclear space. All compartments contained enveloped virions. After treatment with brefeldin A, HSV-1 virions aggregated in the perinuclear space and endoplasmic reticulum, while infectious progeny virus was still produced.Conclusions: The data suggest that virions derived by budding at nuclear membranes are intraluminally transported from the perinuclear space via Golgi -endoplasmic reticulum transitions into Golgi cisternae for packaging. Virions derived by budding at nuclear membranes are infective like Us3 deletion mutants, which accumulate in the perinuclear space. Therefore, i) de-envelopment followed by re-envelopment is not essential for production of infective progeny virus, ii) the process taking place at the outer nuclear membrane is budding not fusion, and iii) naked capsids gain access to the cytoplasmic matrix via impaired nuclear envelope as reported earlier.

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Analysis of intracellular and intraviral localization of the human cytomegalovirus UL53 protein

Journal of General Virology ◽

10.1099/0022-1317-83-5-1005 ◽

2002 ◽

Vol 83 (5) ◽

pp. 1005-1012 ◽

Cited By ~ 37

Author(s):

P. Dal Monte ◽

S. Pignatelli ◽

N. Zini ◽

N. M. Maraldi ◽

E. Perret ◽

...

Keyword(s):

Human Cytomegalovirus ◽

Nuclear Membrane ◽

Human Fibroblasts ◽

Nuclear Periphery ◽

Structural Protein ◽

Lamin B ◽

Mature Virus Particle ◽

Ul53 Gene ◽

Simplex Virus

Human cytomegalovirus (HCMV) UL53 belongs to a family of conserved herpesvirus genes. In this work, the expression and localization of the UL53 gene product was analysed. Results obtained showed that pUL53 is a new structural protein. In infected human fibroblasts, pUL53 localizes in cytoplasmic perinuclear granular formations together with other structural viral proteins. In the nucleus, pUL53 forms patches at the nuclear periphery and co-localizes with lamin B at the internal nuclear membrane level. Immunoelectron microscopy studies have disclosed that nuclear pseudo-inclusions are labelled, whereas nucleocapsid formations within the intranuclear skein are negative. Furthermore, the mature virus particle maintains pUL53 at its tegumental level. These data suggest that pUL53 could be involved either in nucleocapsid maturation or in the egress of nucleocapsids from the nucleus to the cytoplasm through the nuclear membrane, a role compatible with the function hypothesized for UL31, its positional homologue in herpes simplex virus type 1.

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