Dynamic redistribution of calmodulin in HeLa cells during cell division as revealed by a GFP-calmodulin fusion protein technique

C.J. Li; R. Heim; P. Lu; Y. Pu; R.Y. Tsien; D.C. Chang

doi:10.1242/jcs.112.10.1567

Dynamic redistribution of calmodulin in HeLa cells during cell division as revealed by a GFP-calmodulin fusion protein technique

Journal of Cell Science ◽

10.1242/jcs.112.10.1567 ◽

1999 ◽

Vol 112 (10) ◽

pp. 1567-1577 ◽

Cited By ~ 4

Author(s):

C.J. Li ◽

R. Heim ◽

P. Lu ◽

Y. Pu ◽

R.Y. Tsien ◽

...

Keyword(s):

Cell Division ◽

Hela Cells ◽

Mammalian Cells ◽

Membrane Fraction ◽

Fluorescent Protein ◽

Active Role ◽

Biochemical Properties ◽

Equatorial Region ◽

Cleavage Furrow ◽

Inhibitory Peptide

It has been suggested by many studies that Ca2+ signaling plays an important role in regulating key steps in cell division. In order to study the down stream components of calcium signaling, we have fused the gene of calmodulin (CaM) with that of green fluorescent protein (GFP) and expressed it in HeLa cells. The GFP-CaM protein was found to have similar biochemical properties as the wild-type CaM, and its distribution was also similar to that of the endogenous CaM. Using this GFP-tagged CaM as a probe, we have conducted a detailed examination of the spatial- and temporal-dependent redistribution of calmodulin in living mammalian cells during cell division. Our major findings are: (1) high density of CaM was found to distribute in two sub-cellular locations during mitosis; one fraction was concentrated in the spindle poles, while the other was concentrated in the sub-membrane region around the cell. (2) The sub-membrane fraction of CaM became aggregated at the equatorial region where the cleavage furrow was about to form. The timing of this localized aggregation of CaM was closely associated with the onset of cytokinesis. (3) Using a TA-CaM probe, we found that the sub-membrane fraction of CaM near the cleavage furrow was selectively activated during cell division. (4) When we injected a CaM-specific inhibitory peptide into early anaphase cells, cytokinesis was either blocked or severely delayed. These findings suggest that, in addition to Ca2+ ion, CaM may represent a second signal that can also play an active role in determining the positioning and timing of the cleavage furrow formation.

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Nocodazole and cytochalasin D induce tetraploidy in mammalian cells

AJP Cell Physiology ◽

10.1152/ajpcell.1984.246.1.c154 ◽

1984 ◽

Vol 246 (1) ◽

pp. C154-C156 ◽

Cited By ~ 21

Author(s):

G. W. Zieve

Keyword(s):

Cell Division ◽

Mammalian Cells ◽

Cytochalasin D ◽

Microtubule Assembly ◽

Reversible Inhibitor ◽

Cleavage Furrow ◽

Synchronized Cells ◽

Cells In Culture ◽

Wide Range

Nocodazole, a rapidly reversible inhibitor of microtubule assembly is useful for preparing mammalian cells synchronized at all stages of mitosis. When synchronized cells are allowed to progress through mitosis in the presence of cytochalasin D, the cleavage furrow is inhibited and dikaryon cells are formed. These cells become homogeneous populations of stable mononuclear tetraploid cells after the following cell division. This procedure is applicable to a wide range of mammalian cells in culture.

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The ultrastructure of cell division in Euglena gracilis

Journal of Cell Science ◽

10.1242/jcs.31.1.25 ◽

1978 ◽

Vol 31 (1) ◽

pp. 25-35

Author(s):

M.A. Gillott ◽

R.E. Triemer

Keyword(s):

Cell Division ◽

Nuclear Envelope ◽

Basal Body ◽

Euglena Gracilis ◽

Equatorial Region ◽

Basal Bodies ◽

Cleavage Furrow ◽

Free Zone ◽

Prophase Nucleus

The ultrastructure of mitosis in Euglena gracilis was investigated. At preprophase the nucleus migrates anteriorly and associates with the basal bodies. Flagella and basal bodies replicate at preprophase. Cells retain motility throughout division. The reservoir and the prophase nucleus elongate perpendicular to the incipient cleavage furrow. One basal body pair surrounded by a ribosome-free zone is found at each of the nuclear poles. The spindle forms within the intact nuclear envelope- Polar fenestrae are absent. At metaphase, the endosome is elongated from pole to pole, and chromosomes are loosely arranged in the equatorial region. Distinct, trilayered kinetochores are present. Spindle elongates as chromosomes migrate to the poles forming a dumb-bell shaped nucleus by telophase. Daughter nuclei are formed by constriction of the nuclear envelope. Cytokinesis is accomplished by furrowing. Cell division in Euglena is compared with that of certain other algae.

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Nuclear-Associated Plasmid, But Not Cell-Associated Plasmid, is Correlated With Transgene Expression in Cultured Mammalian Cells

10.1115/imece2000-2232 ◽

2000 ◽

Author(s):

Molly B. James ◽

Todd D. Giorgio

Keyword(s):

Hela Cell ◽

Hela Cells ◽

Plasmid Dna ◽

Mammalian Cells ◽

Transgene Expression ◽

Quantitative Method ◽

Fluorescent Protein ◽

Cmv Promoter ◽

Green Fluorescent ◽

Plasmid Delivery

Abstract Intracellular plasmid is rapidly incorporated into the nucleus of HeLa cells following cationic lipoplex transfection. CV1 cells are less effective in translocating plasmid to the nucleus and also express less transgene than HeLa cells. Cultured HeLa and CV1 cells and corresponding isolated nuclei were analyzed after transfection of a Cy3 labeled pGreenLantern plasmid (Cy3-pGL). Flow cytometry was used to measure both plasmid delivery and transgene expression from the plasmid encoding a CMV promoter driven green fluorescent protein. During transfection, HeLa cells rapidly incorporated the plasmid, reaching a maximum of 80% Cy3-pGL positive cells 8 hours post-transfection. The average Cy3-pGL positive HeLa cell contained approximately 2470 plasmid copies. 48% of the nuclei isolated from the transfected HeLa cells were positive for the plasmid marker after 8 hours. In contrast to HeLa cells, fewer CV1 cells and CV1 nuclei incorporated plasmid DNA with peak transfection occurring after 12 hours for 36% of the cells and after 8 hours for 12% of the nuclei. However, the average Cy3-pGL positive CV1 cell did not have a significantly different number of total cellular plasmid copies than the average positive HeLa cell. CV1 nuclei, however, had half as much plasmid as HeLa nuclei. HeLa cells are more efficient than CV1 cells at transporting plasmid from the cytoplasm to the nucleus. This study demonstrates the use of a novel quantitative method to study plasmid transport from the cytoplasm to nucleus and the effect on transgene expression.

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Modulation of phosphatidylinositol 4-phosphate levels by CaBP7 controls cytokinesis in mammalian cells

Molecular Biology of the Cell ◽

10.1091/mbc.e14-07-1243 ◽

2015 ◽

Vol 26 (8) ◽

pp. 1428-1439 ◽

Cited By ~ 9

Author(s):

Dayani Rajamanoharan ◽

Hannah V. McCue ◽

Robert D. Burgoyne ◽

Lee P. Haynes

Keyword(s):

Cell Division ◽

Hela Cells ◽

Calcium Binding ◽

Mammalian Cells ◽

Calcium Binding Protein ◽

Model Systems ◽

Intercellular Bridge ◽

Phosphoinositide Signaling ◽

Novel Association ◽

Phosphatidylinositol 4

Calcium and phosphoinositide signaling regulate cell division in model systems, but their significance in mammalian cells is unclear. Calcium-binding protein-7 (CaBP7) is a phosphatidylinositol 4-kinaseIIIβ (PI4KIIIβ) inhibitor required during cytokinesis in mammalian cells, hinting at a link between these pathways. Here we characterize a novel association of CaBP7 with lysosomes that cluster at the intercellular bridge during cytokinesis in HeLa cells. We show that CaBP7 regulates lysosome clustering and that PI4KIIIβ is essential for normal cytokinesis. CaBP7 depletion induces lysosome mislocalization, extension of intercellular bridge lifetime, and cytokinesis failure. These data connect phosphoinositide and calcium pathways to lysosome localization and normal cytokinesis in mammalian cells.

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PERSISTENCE OF MESSENGER RNA THROUGH MITOSIS IN HELA CELLS

The Journal of Cell Biology ◽

10.1083/jcb.40.2.497 ◽

1969 ◽

Vol 40 (2) ◽

pp. 497-507 ◽

Cited By ~ 57

Author(s):

L. D. Hodge ◽

E. Robbins ◽

M. D. Scharff

Keyword(s):

Electron Microscopy ◽

Protein Synthesis ◽

Cell Division ◽

Hela Cells ◽

Messenger Rna ◽

Mammalian Cells ◽

Actinomycin D ◽

Progressive Increase ◽

The Reformation

The decrease in protein synthesis which occurs in mammalian cells during cell division is associated with significant disaggregation of polyribosomes. For determining whether messenger RNA survives this disaggregation, the reformation of polyribosomes was investigated in synchronized HeLa cells as they progressed from metaphase into interphase in the presence of 2 µg/ml Actinomycin D. The persistence of messenger during cell division was evidenced by: (1) a progressive increase in the rate of protein synthesis in both treated and untreated cells for 45 min after metaphase; (2) reformation of polyribosomes, as determined by both sucrose gradients and electron microscopy, within 30 min after the addition of Actinomycin D to metaphase cells; (3) the persistence of approximately 50% of the rapidly labeled nonribosomal RNA which had associated with polyribosomes just before metaphase; (4) the resumption of synthesis, following cell division, of 6 selected peptides in Actinomycin-treated cells.

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Light-induced blockage of cell division with a chromatin-targeted phototoxic fluorescent protein

Biochemical Journal ◽

10.1042/bj20101217 ◽

2011 ◽

Vol 435 (1) ◽

pp. 65-71 ◽

Cited By ~ 32

Author(s):

Ekaterina O. Serebrovskaya ◽

Tatiana V. Gorodnicheva ◽

Galina V. Ermakova ◽

Elena A. Solovieva ◽

George V. Sharonov ◽

...

Keyword(s):

Cell Division ◽

Mammalian Cells ◽

Fluorescent Protein ◽

Green Light ◽

Specific Cell ◽

Light Illumination ◽

Division Rate ◽

Green Fluorescent ◽

Mitosis And Meiosis

Proteins of the GFP (green fluorescent protein) family are widely used as passive reporters for live cell imaging. In the present study we used H2B (histone H2B)–tKR (tandem KillerRed) as an active tool to affect cell division with light. We demonstrated that H2B–tKR-expressing cells behave normally in the dark, but transiently cease proliferation following green-light illumination. Complete light-induced blockage of cell division for approx. 24 h was observed in cultured mammalian cells that were either transiently or stably transfected with H2B–tKR. Illuminated cells then returned to normal division rate. XRCC1 (X-ray cross complementing factor 1) showed immediate redistribution in the illuminated nuclei of H2B–tKR-expressing cells, indicating massive light-induced damage of genomic DNA. Notably, nondisjunction of chromosomes was observed for cells that were illuminated during metaphase. In transgenic Xenopus embryos expressing H2B–tKR under the control of tissue-specific promoters, we observed clear retardation of the development of these tissues in green-light-illuminated tadpoles. We believe that H2B–tKR represents a novel optogenetic tool, which can be used to study mitosis and meiosis progression per se, as well as to investigate the roles of specific cell populations in development, regeneration and carcinogenesis in vivo.

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Use of Uranium-Labeled Antibodies for Electron Microscopic Localization of Various Antigens in Mammalian Cells

Proceedings, annual meeting, Electron Microscopy Society of America ◽

10.1017/s0424820100060696 ◽

1967 ◽

Vol 25 ◽

pp. 136-137

Author(s):

J. P. Petrali ◽

E. J. Donati ◽

L. A. Sternberger

Keyword(s):

Endoplasmic Reticulum ◽

Hela Cells ◽

Mammalian Cells ◽

Specific Antiserum ◽

Electron Microscopic ◽

E Coli ◽

Cytoplasmic Membranes ◽

Viral Progeny ◽

Ultrathin Sections ◽

Electron Microscopic Localization

Specific contrast is conferred to subcellular antigen by applying purified antibodies, exhaustively labeled with uranium under immunospecific protection, to ultrathin sections. Use of Seligman’s principle of bridging osmium to metal via thiocarbohydrazide (TCH) intensifies specific contrast. Ultrathin sections of osmium-fixed materials were stained on the grid by application of 1) thiosemicarbazide (TSC), 2) unlabeled specific antiserum, 3) uranium-labeled anti-antibody and 4) TCH followed by reosmication. Antigens to be localized consisted of vaccinia antigen in infected HeLa cells, lysozyme in monocytes of patients with monocytic or monomyelocytic leukemia, and fibrinogen in the platelets of these leukemic patients. Control sections were stained with non-specific antiserum (E. coli).In the vaccinia-HeLa system, antigen was localized from 1 to 3 hours following infection, and was confined to degrading virus, the inner walls of numerous organelles, and other structures in cytoplasmic foci. Surrounding architecture and cellular mitochondria were unstained. 8 to 14 hours after infection, antigen was localized on the outer walls of the viral progeny, on cytoplasmic membranes, and free in the cytoplasm. Staining of endoplasmic reticulum was intense and focal early, and weak and diffuse late in infection.

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Cardiolipin-Containing Lipid Membranes Attract the Bacterial Cell Division Protein DivIVA

International Journal of Molecular Sciences ◽

10.3390/ijms22158350 ◽

2021 ◽

Vol 22 (15) ◽

pp. 8350

Author(s):

Naďa Labajová ◽

Natalia Baranova ◽

Miroslav Jurásek ◽

Robert Vácha ◽

Martin Loose ◽

...

Keyword(s):

Cell Division ◽

Lipid Bilayers ◽

Bacterial Cell ◽

Lipid Membranes ◽

Model Organism ◽

Active Role ◽

Membrane Curvature ◽

Bacterial Cell Division ◽

Division Site ◽

Clostridioides Difficile

DivIVA is a protein initially identified as a spatial regulator of cell division in the model organism Bacillus subtilis, but its homologues are present in many other Gram-positive bacteria, including Clostridia species. Besides its role as topological regulator of the Min system during bacterial cell division, DivIVA is involved in chromosome segregation during sporulation, genetic competence, and cell wall synthesis. DivIVA localizes to regions of high membrane curvature, such as the cell poles and cell division site, where it recruits distinct binding partners. Previously, it was suggested that negative curvature sensing is the main mechanism by which DivIVA binds to these specific regions. Here, we show that Clostridioides difficile DivIVA binds preferably to membranes containing negatively charged phospholipids, especially cardiolipin. Strikingly, we observed that upon binding, DivIVA modifies the lipid distribution and induces changes to lipid bilayers containing cardiolipin. Our observations indicate that DivIVA might play a more complex and so far unknown active role during the formation of the cell division septal membrane.

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Enhanced brightness of bacterial luciferase by bioluminescence resonance energy transfer

Scientific Reports ◽

10.1038/s41598-021-94551-4 ◽

2021 ◽

Vol 11 (1) ◽

Author(s):

Tomomi Kaku ◽

Kazunori Sugiura ◽

Tetsuyuki Entani ◽

Kenji Osabe ◽

Takeharu Nagai

Keyword(s):

Energy Transfer ◽

Mammalian Cells ◽

Fluorescent Protein ◽

Color Change ◽

Yellow Fluorescent Protein ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Bioluminescence Resonance Energy Transfer ◽

Bacterial Luciferase ◽

Bacterial Bioluminescence

AbstractUsing the lux operon (luxCDABE) of bacterial bioluminescence system as an autonomous luminous reporter has been demonstrated in bacteria, plant and mammalian cells. However, applications of bacterial bioluminescence-based imaging have been limited because of its low brightness. Here, we engineered the bacterial luciferase (heterodimer of luxA and luxB) by fusion with Venus, a bright variant of yellow fluorescent protein, to induce bioluminescence resonance energy transfer (BRET). By using decanal as an externally added substrate, color change and ten-times enhancement of brightness was achieved in Escherichia coli when circularly permuted Venus was fused to the C-terminus of luxB. Expression of the Venus-fused luciferase in human embryonic kidney cell lines (HEK293T) or in Nicotiana benthamiana leaves together with the substrate biosynthesis-related genes (luxC, luxD and luxE) enhanced the autonomous bioluminescence. We believe the improved luciferase will forge the way towards the potential development of autobioluminescent reporter system allowing spatiotemporal imaging in live cells.

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ADP-Ribosylation Factor (ARF) Interaction Is Not Sufficient for Yeast GGA Protein Function or Localization

Molecular Biology of the Cell ◽

10.1091/mbc.e02-02-0078 ◽

2002 ◽

Vol 13 (9) ◽

pp. 3078-3095 ◽

Cited By ~ 30

Author(s):

Annette L. Boman ◽

Paul D. Salo ◽

Melissa J. Hauglund ◽

Nicole L. Strand ◽

Shelly J. Rensink ◽

...

Keyword(s):

Membrane Trafficking ◽

Mammalian Cells ◽

Fluorescent Protein ◽

Protein Localization ◽

Carboxypeptidase Y ◽

Minor Role ◽

Temperature Sensitive ◽

Adp Ribosylation ◽

And Function ◽

Adp Ribosylation Factor

Golgi-localized γ-ear homology domain, ADP-ribosylation factor (ARF)-binding proteins (GGAs) facilitate distinct steps of post-Golgi traffic. Human and yeast GGA proteins are only ∼25% identical, but all GGA proteins have four similar domains based on function and sequence homology. GGA proteins are most conserved in the region that interacts with ARF proteins. To analyze the role of ARF in GGA protein localization and function, we performed mutational analyses of both human and yeast GGAs. To our surprise, yeast and human GGAs differ in their requirement for ARF interaction. We describe a point mutation in both yeast and mammalian GGA proteins that eliminates binding to ARFs. In mammalian cells, this mutation disrupts the localization of human GGA proteins. Yeast Gga function was studied using an assay for carboxypeptidase Y missorting and synthetic temperature-sensitive lethality between GGAs andVPS27. Based on these assays, we conclude that non-Arf-binding yeast Gga mutants can function normally in membrane trafficking. Using green fluorescent protein-tagged Gga1p, we show that Arf interaction is not required for Gga localization to the Golgi. Truncation analysis of Gga1p and Gga2p suggests that the N-terminal VHS domain and C-terminal hinge and ear domains play significant roles in yeast Gga protein localization and function. Together, our data suggest that yeast Gga proteins function to assemble a protein complex at the late Golgi to initiate proper sorting and transport of specific cargo. Whereas mammalian GGAs must interact with ARF to localize to and function at the Golgi, interaction between yeast Ggas and Arf plays a minor role in Gga localization and function.

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