Faculty Opinions recommendation of Polo-like kinase-2 is required for centriole duplication in mammalian cells.

2004 ◽  
Author(s):  
Iain Hagan
Keyword(s):  
Mammalian Cells ◽  
Centriole Duplication

scholarly journals Autoamplification and competition drive symmetry breaking: Initiation of centriole duplication by the PLK4-STIL network

2018 ◽  
Author(s):  
Marcin Leda ◽  
Andrew J. Holland ◽  
Andrew B. Goryachev
Keyword(s):  
Symmetry Breaking ◽  
Mammalian Cells ◽  
Molecular Mechanisms ◽  
Break Symmetry ◽  
Biophysical Model ◽  
Model Organisms ◽  
Centriole Duplication ◽  
Mother Centriole ◽  
Autocatalytic Activation

SummarySymmetry breaking, a central principle of physics, has been hailed as the driver of self-organization in biological systems in general and biogenesis of cellular organelles in particular, but the molecular mechanisms of symmetry breaking only begin to become understood. Centrioles, the structural cores of centrosomes and cilia, must duplicate every cell cycle to ensure their faithful inheritance through cellular divisions. Work in model organisms identified conserved proteins required for centriole duplication and found that altering their abundance affects centriole number. However, the biophysical principles that ensure that, under physiological conditions, only a single procentriole is produced on each mother centriole remain enigmatic. Here we propose a mechanistic biophysical model for the initiation of procentriole formation in mammalian cells. We posit that interactions between the master regulatory kinase PLK4 and its activator-substrate STIL form the basis of the procentriole initiation network. The model faithfully recapitulates the experimentally observed transition from PLK4 uniformly distributed around the mother centriole, the “ring”, to a unique PLK4 focus, the “spot”, that triggers the assembly of a new procentriole. This symmetry breaking requires a dual positive feedback based on autocatalytic activation of PLK4 and enhanced centriolar anchoring of PLK4-STIL complexes by phosphorylated STIL. We find that, contrary to previous proposals,in situdegradation of active PLK4 is insufficient to break symmetry. Instead, the model predicts that competition between transient PLK4 activity maxima for PLK4-STIL complexes explains both the instability of the PLK4 ring and formation of the unique PLK4 spot. In the model, strong competition at physiologically normal parameters robustly produces a single procentriole, while increasing overexpression of PLK4 and STIL weakens the competition and causes progressive addition of procentrioles in agreement with experimental observations.

scholarly journals A specific basal body linker protein provides the connection function for basal body inheritance in trypanosomes

2021 ◽  
Vol 118 (8) ◽  
pp. e2014040118
Author(s):  
De-Hua Lai ◽  
Flavia Moreira-Leite ◽  
Zhi-Shen Xu ◽  
Jiong Yang ◽  
Keith Gull
Keyword(s):  
Basal Body ◽  
Mammalian Cells ◽  
De Novo ◽  
Coiled Coil ◽  
Centriole Duplication ◽  
Cytoskeletal Component ◽  
Dividing Cells ◽  
Orthogonal Orientation ◽  
And Function ◽  
Additional Role

Centrioles and basal bodies (CBBs) are found in physically linked pairs, and in mammalian cells intercentriole connections (G1–G2 tether and S–M linker) regulate centriole duplication and function. In trypanosomes BBs are not associated with the spindle and function in flagellum/cilia nucleation with an additional role in mitochondrial genome (kinetoplast DNA [kDNA]) segregation. Here, we describe BBLP, a BB/pro-BB (pBB) linker protein in Trypanosoma brucei predicted to be a large coiled-coil protein conserved in the kinetoplastida. Colocalization with the centriole marker SAS6 showed that BBLP localizes between the BB/pBB pair, throughout the cell cycle, with a stronger signal in the old flagellum BB/pBB pair. Importantly, RNA interference (RNAi) depletion of BBLP leads to a conspicuous splitting of the BB/pBB pair associated only with the new flagellum. BBLP RNAi is lethal in the bloodstream form of the parasite and perturbs mitochondrial kDNA inheritance. Immunogold labeling confirmed that BBLP is localized to a cytoskeletal component of the BB/pBB linker, and tagged protein induction showed that BBLP is incorporated de novo in both new and old flagella BB pairs of dividing cells. We show that the two aspects of CBB disengagement—loss of orthogonal orientation and ability to separate and move apart—are consistent but separable events in evolutionarily diverse cells and we provide a unifying model explaining centriole/BB linkage differences between such cells.

scholarly journals Centrin-2 Is Required for Centriole Duplication in Mammalian Cells

2002 ◽  
Vol 12 (15) ◽  
pp. 1287-1292 ◽  
Author(s):  
Jeffrey L Salisbury ◽  
Kelly M Suino ◽  
Robert Busby ◽  
Margaret Springett
Keyword(s):  
Mammalian Cells ◽  
Centriole Duplication

scholarly journals Centrobin

2005 ◽  
Vol 171 (3) ◽  
pp. 437-445 ◽  
Author(s):  
Chaozhong Zou ◽  
Jun Li ◽  
Yujie Bai ◽  
William T. Gunning ◽  
David E. Wazer ◽  
...  
Keyword(s):  
Cell Cycle ◽  
Mammalian Cells ◽  
Cell Cycle Progression ◽  
S Phase ◽  
Cycle Progression ◽  
Centriole Duplication ◽  
Pericentriolar Material ◽  
Core Components ◽  
Interfering Rna ◽  
Daughter Centriole

In mammalian cells, the centrosome consists of a pair of centrioles and amorphous pericentriolar material. The pair of centrioles, which are the core components of the centrosome, duplicate once per cell cycle. Centrosomes play a pivotal role in orchestrating the formation of the bipolar spindle during mitosis. Recent studies have linked centrosomal activity on centrioles or centriole-associated structures to cytokinesis and cell cycle progression through G1 into the S phase. In this study, we have identified centrobin as a centriole-associated protein that asymmetrically localizes to the daughter centriole. The silencing of centrobin expression by small interfering RNA inhibited centriole duplication and resulted in centrosomes with one or no centriole, demonstrating that centrobin is required for centriole duplication. Furthermore, inhibition of centriole duplication by centrobin depletion led to impaired cytokinesis.

scholarly journals Polo-like Kinase-2 Is Required for Centriole Duplication in Mammalian Cells

2004 ◽  
Vol 14 (13) ◽  
pp. 1200-1207 ◽  
Author(s):  
Silke Warnke ◽  
Stefan Kemmler ◽  
Rebecca S Hames ◽  
Hsiao-Lun Tsai ◽  
Urs Hoffmann-Rohrer ◽  
...  
Keyword(s):  
Mammalian Cells ◽  
Centriole Duplication

scholarly journals SFI1 promotes centriole duplication by recruiting USP9X to stabilize the microcephaly protein STIL

2019 ◽  
Vol 218 (7) ◽  
pp. 2185-2197 ◽  
Author(s):  
Andrew Kodani ◽  
Tyler Moyer ◽  
Allen Chen ◽  
Andrew Holland ◽  
Christopher A. Walsh ◽  
...  
Keyword(s):  
Mental Retardation ◽  
Mammalian Cells ◽  
Spindle Pole Body ◽  
Spindle Pole ◽  
S Phase ◽  
Loss Of Function ◽  
Centrosomal Protein ◽  
Centriole Duplication ◽  
Pole Body ◽  
Mammalian Homologue

In mammals, centrioles participate in brain development, and human mutations affecting centriole duplication cause microcephaly. Here, we identify a role for the mammalian homologue of yeast SFI1, involved in the duplication of the yeast spindle pole body, as a critical regulator of centriole duplication in mammalian cells. Mammalian SFI1 interacts with USP9X, a deubiquitylase associated with human syndromic mental retardation. SFI1 localizes USP9X to the centrosome during S phase to deubiquitylate STIL, a critical regulator of centriole duplication. USP9X-mediated deubiquitylation protects STIL from degradation. Consistent with a role for USP9X in stabilizing STIL, cells from patients with USP9X loss-of-function mutations have reduced STIL levels. Together, these results demonstrate that SFI1 is a centrosomal protein that localizes USP9X to the centrosome to stabilize STIL and promote centriole duplication. We propose that the USP9X protection of STIL to facilitate centriole duplication underlies roles of both proteins in human neurodevelopment.

scholarly journals Molecular characterization of centriole assembly in ciliated epithelial cells

2007 ◽  
Vol 178 (1) ◽  
pp. 31-42 ◽  
Author(s):  
Eszter K. Vladar ◽  
Tim Stearns
Keyword(s):  
Epithelial Cells ◽  
Mammalian Cells ◽  
Intraflagellar Transport ◽  
Proximal Region ◽  
Basal Bodies ◽  
Tracheal Epithelial Cells ◽  
Centriole Duplication ◽  
Centriole Assembly ◽  
Ciliated Epithelial Cells ◽  
Centrosomal Proteins

Ciliated epithelial cells have the unique ability to generate hundreds of centrioles during differentiation. We used centrosomal proteins as molecular markers in cultured mouse tracheal epithelial cells to understand this process. Most centrosomal proteins were up-regulated early in ciliogenesis, initially appearing in cytoplasmic foci and then incorporated into centrioles. Three candidate proteins were further characterized. The centrosomal component SAS-6 localized to basal bodies and the proximal region of the ciliary axoneme, and depletion of SAS-6 prevented centriole assembly. The intraflagellar transport component polaris localized to nascent centrioles before incorporation into cilia, and depletion of polaris blocked axoneme formation. The centriolar satellite component PCM-1 colocalized with centrosomal components in cytoplasmic granules surrounding nascent centrioles. Interfering with PCM-1 reduced the amount of centrosomal proteins at basal bodies but did not prevent centriole assembly. This system will help determine the mechanism of centriole formation in mammalian cells and how the limitation on centriole duplication is overcome in ciliated epithelial cells.

Ultrastructural Alterations in Hela Cells Induced by Spider Venom

1967 ◽  
Vol 25 ◽  
pp. 20-21
Author(s):  
Dale E. McClendon ◽  
Paul N. Morgan ◽  
Bernard L. Soloff
Keyword(s):  
Growth Medium ◽  
Mammalian Cells ◽  
Carcinoma Cells ◽  
Venom Protein ◽  
Sterile Saline ◽  
Carbon Coated ◽  
Available Information ◽  
Loxosceles Reclusa ◽  
Essential Growth ◽  
Solution Cultures

It has been observed that minute amounts of venom from the brown recluse spider, Loxosceles reclusa, are capable of producing cytotoxic changes in cultures of certain mammalian cells (Morgan and Felton, 1965). Since there is little available information concerning the effect of venoms on susceptible cells, we have attempted to characterize, at the electron microscope level, the cytotoxic changes produced by the venom of this spider.Cultures of human epithelial carcinoma cells, strain HeLa, were initiated on sterile, carbon coated coverslips contained in Leighton tubes. Each culture was seeded with approximately 1x105 cells contained in 1.5 ml of a modified Eagle's minimum essential growth medium prepared in Hank's balanced salt solution. Cultures were incubated at 36° C. for three days prior to the addition of venom. The venom was collected from female brown recluse spiders and diluted in sterile saline. Protein determinations on the venom-were made according to the spectrophotometric method of Waddell (1956). Approximately 10 μg venom protein per ml of fresh medium was added to each culture after discarding the old growth medium. Control cultures were treated similarly, except that no venom was added. All cultures were reincubated at 36° C.

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

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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