Your search keyword '"Latrunculin"' showing total 446 results

201. Inhibition of Rho-kinase induces αB-crystallin expression in lens epithelial cells

Author

J. Samuel Zigler, Rahul N Khurana, P. Vasantha Rao, Hiroaki Shimokawa, R. Maddala, and David L. Epstein

Subjects

rho GTP-Binding Proteins, Botulinum Toxins, Pyridines, Swine, Biophysics, Protein Serine-Threonine Kinases, Mitogen-activated protein kinase kinase, Biology, p38 Mitogen-Activated Protein Kinases, Biochemistry, Stress Fibers, Lens, Crystalline, Animals, ASK1, c-Raf, Enzyme Inhibitors, Protein kinase A, Cytoskeleton, Molecular Biology, Rho-associated protein kinase, ADP Ribose Transferases, rho-Associated Kinases, Intracellular Signaling Peptides and Proteins, Epithelial Cells, Cell Biology, Protein-Tyrosine Kinases, Amides, Crystallins, Molecular biology, eye diseases, Cell biology, Mutation, Latrunculin, sense organs, MDia1, Mitogen-Activated Protein Kinases

Abstract

The small heat shock protein, alphaB-crystallin, has been shown to interact with actin and intermediate filament proteins. However, little is known regarding the cellular mechanisms regulating such interactions. In this study, we explored the role of the Rho/Rho-kinase pathway in alphaB-crystallin distribution and expression in porcine lens epithelial cells. alphaB-crystallin was distributed uniformly throughout the cytoplasm and did not exhibit any unique redistribution in response to actin depolymerization induced by Rho/Rho-kinase inhibitors (C3-exoenzyme or Y-27632) or by overexpression of the dominant negative mutant of Rho-kinase (DNRK) in porcine lens epithelial cells. Interestingly, alphaB-crystallin levels markedly increased in lens epithelial cells treated with the inhibitors of Rho/Rho-kinase proteins (lovastatin, Y-27632 or DNRK) while a protein kinase C inhibitor (GF109203x) was found to have no effect. Further, Y-27632 showed a dose (2-50 microM) response effect on alphaB-crystallin induction. Nocodazole, a microtubule-depolymerizing agent, elicited an increase in alphaB-crystallin levels but latrunculin, an actin depolymerizing agent, did not show any significant effect. Pretreatment with cycloheximide or genistein blocked the Rho-kinase inhibitor-induced increase in alphaB-crystallin protein levels. Rho-kinase inhibitor-induced increases in alphaB-crystallin levels were found to be associated with activation of P38 mitogen-activated protein kinase (MAPK). These results suggest that Rho/Rho-kinase negatively regulates alphaB-crystallin expression, and this response appears to be dependent on tyrosine-protein kinase and P38 MAPK function. Finally, alphaB-crystallin induction appears to be better correlated with the direct inhibition of Rho/Rho-kinase than with actin depolymerization per se.

Published

2002

202. Control of Actin Dynamics by Proteins Made of β-Thymosin Repeats

Author

Maud Hertzog, Dominique Didry, Marie-France Carlier, Michael R. Bubb, and Elena G. Yarmola

Subjects

biology, Arp2/3 complex, Actin remodeling, macromolecular substances, Cell Biology, Microfilament, Biochemistry, Cell biology, Profilin, biology.protein, Latrunculin, Actin-binding protein, MDia1, Molecular Biology, Ternary complex, hormones, hormone substitutes, and hormone antagonists

Abstract

Actobindin is an actin-binding protein from amoeba, which consists of two beta-thymosin repeats and has been shown to inhibit actin polymerization by sequestering G-actin and by stabilizing actin dimers. Here we show that actobindin has the same biochemical properties as the Drosophila or Caenorhabditis elegans homologous protein that consists of three beta-thymosin repeats. These proteins define a new family of actin-binding proteins. They bind G-actin in a 1:1 complex with thermodynamic and kinetic parameters similar to beta-thymosins. Like beta-thymosins, they slow down nucleotide exchange on G-actin and make a ternary complex with G-actin and Latrunculin A. On the other hand, they behave as functional homologs of profilin because their complex with MgATP-G-actin, unlike beta-thymosin-actin, participates in filament barbed end growth, like profilin-actin complex. Therefore these proteins play an active role in actin-based motility processes. In addition, proteins of the actobindin family interact with the pointed end of actin filaments and inhibit pointed end growth, maybe via the interaction of the beta-thymosin repeats with two terminal subunits.

Published

2002

203. Cortical actin nodes: Their dynamics and recruitment of podosomal proteins as revealed by super-resolution and single-molecule microscopy

Author

Yuki M. Shirai, Takahiro K. Fujiwara, Akihiro Kusumi, Fumiyoshi Ishidate, Taka A. Tsunoyama, Koichiro M. Hirosawa, Atsushi Tsurumune, Akihiro C. E. Shibata, Kenichi Kondo, and Nao Hiramoto-Yamaki

Subjects

0301 basic medicine, lcsh:Medicine, Actin Filaments, Filamin, Biochemistry, chemistry.chemical_compound, Contractile Proteins, Fluorescence Microscopy, Myosin, Macromolecular Structure Analysis, Fluorescence microscope, lcsh:Science, Cells, Cultured, Microscopy, Multidisciplinary, biology, Light Microscopy, Single Molecule Imaging, Cell Motility, Cell Processes, Podosomes, Dynamic Actin Filaments, Cortactin, Research Article, Protein Structure, Imaging Techniques, Phalloidin, Motor Proteins, Actin Motors, macromolecular substances, Myosins, Research and Analysis Methods, 03 medical and health sciences, Molecular Motors, Fluorescence Imaging, Animals, Molecular Biology, Actin, lcsh:R, Biology and Life Sciences, Proteins, Cell Biology, Actins, Cytoskeletal Proteins, 030104 developmental biology, chemistry, Cytoplasm, Biophysics, biology.protein, Latrunculin, lcsh:Q, Actin Polymerization

Abstract

Electron tomography of the plasma membrane (PM) identified several layers of cortical actin meshwork running parallel to the PM cytoplasmic surface throughout the PM. Here, cortical actin structures and dynamics were examined in living cells, using super-resolution microscopy, with (x,y)- and z-resolutions of ~140 and ~400 nm, respectively, and single-molecule imaging. The super-resolution microscopy identified sub-micron-sized actin clusters that appeared identical by both phalloidin post-fixation staining and Lifeact-mGFP expression followed by fixation, and therefore, these actin clusters were named "actin-pl-clusters". In live cells, the actin-pl-clusters visualized by Lifeact-mGFP linked two or more actin filaments in the fine actin meshwork, acting as a node of the meshwork, and dynamically moved on/along the meshwork in a myosin II-dependent manner. Their formation depended on the Arp2/3 activities, suggesting that the movements could involve both the myosin motor activity and actin polymerization-depolymerization. The actin-pl-clusters differ from the actin nodes/asters found previously after latrunculin treatments, since myosin II and filamin A were not colocalized with the actin-pl-clusters, and the actin-pl-clusters were much smaller than the previously reported nodes/asters. The Lifeact linked to a fluorescently-labeled transmembrane peptide from syntaxin4 (Lifeact-TM) expressed in the PM exhibited temporary immobilization in the PM regions on which actin-pl-clusters and stress fibers were projected, showing that ≥66% of actin-pl-clusters and 89% of stress fibers were located in close proximity (within 3.5 nm) to the PM cytoplasmic surface. Podosome-associated cytoplasmic proteins, Tks4, Tks5, cortactin, and N-WASP, were transiently recruited to actin-pl-clusters, and thus, we propose that actin-pl-clusters also represent "actin podosome-like clusters".

Published

2017

204. Pressure‐induced actin polymerization in vascular smooth muscle as a mechanism underlying myogenic behavior

Author

George Osol, Natalia I. Gokina, and Marilyn J. Cipolla

Subjects

Vascular smooth muscle, Cytochalasin B, macromolecular substances, Biology, Models, Biological, Biochemistry, Muscle, Smooth, Vascular, Actin remodeling of neurons, chemistry.chemical_compound, Biopolymers, Culture Techniques, Myosin, Pressure, Genetics, Animals, Cytoskeleton, Molecular Biology, Cytochalasin D, Actin remodeling, Cerebral Arteries, Actins, Cell biology, chemistry, cardiovascular system, Latrunculin, Vascular Resistance, Stress, Mechanical, MDia1, Muscle Contraction, Signal Transduction, Biotechnology

Abstract

We hypothesize that actin polymerization within vascular smooth muscle (VSM) in response to increased intravascular pressure is a novel and previously unrecognized mechanism underlying arterial myogenic behavior. This hypothesis is based on the following observations. 1) Unlike skeletal or cardiac muscle, VSM contains a substantial pool of unpolymerized globular (G) actin whose function is not known. 2) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure, demonstrating the dynamic nature of actin within VSM and implying a shift in the F:G equilibrium in favor of F-actin. 3) Agents that inhibit actin polymerization and stabilize the cytoskeleton (cytochalasins and latrunculin) inhibit the development of myogenic tone and decrease the effectiveness of myogenic reactivity. 4) Depolymerization of F-actin with cytochalasin D causes VSM relaxation and increased G-actin content, whereas polymerization of F-actin with jasplakinolide causes VSM contraction and decreased G-actin content. These results are consistent with observations in other cell types in which actin dynamics have been implicated in contractility and/or motility. Actin filament formation in VSM may therefore underlie mechanotransduction and, by providing additional sites for interaction with myosin, enhance force production in response to pressure. Although the mechanism by which actin polymerization is stimulated by pressure is not known, it likely occurs via integrin-mediated activation of signal transduction pathways previously associated with VSM contraction (e.g., PKC activation, Rho A, and tyrosine phosphorylation).

Published

2002

205. Chloroplast and oxygen evolution changes in Symbiodinium sp. as a response to latrunculin and butanedione monoxime treatments under various light conditions

Author

Paola Furla, Fabrice Priouzeau, Stéphanie Barnay-Verdier, Marco A. Villanueva, Symbiose Marine (SM), Evolution Paris Seine, Université des Antilles et de la Guyane (UAG)-Université Pierre et Marie Curie - Paris 6 (UPMC)-Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Centre National de la Recherche Scientifique (CNRS)-Université des Antilles et de la Guyane (UAG)-Université Pierre et Marie Curie - Paris 6 (UPMC)-Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Centre National de la Recherche Scientifique (CNRS), DGAPA-UNAM, Mexico, Université des Antilles et de la Guyane (UAG)-Université Pierre et Marie Curie - Paris 6 (UPMC)-Université Nice Sophia Antipolis (1965 - 2019) (UNS), and COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Centre National de la Recherche Scientifique (CNRS)-Université des Antilles et de la Guyane (UAG)-Université Pierre et Marie Curie - Paris 6 (UPMC)-Université Nice Sophia Antipolis (1965 - 2019) (UNS)

Subjects

0106 biological sciences, Coral reefs, Chloroplasts, Light, Myosin, Plant Science, macromolecular substances, Diacetyl, 01 natural sciences, Biochemistry, Chloroplast membrane, 03 medical and health sciences, Symbiodinium, Botany, Photosynthesis, Actin, 030304 developmental biology, Symbiotic zooxanthellae, 0303 health sciences, biology, [SDV.BID.EVO]Life Sciences [q-bio]/Biodiversity/Populations and Evolution [q-bio.PE], Cell Biology, General Medicine, Intracellular Membranes, Actin cytoskeleton, biology.organism_classification, Bridged Bicyclo Compounds, Heterocyclic, Chloroplast organization, Chloroplast, Oxygen, Actin Cytoskeleton, Biophysics, Dinoflagellida, Latrunculin, Thiazolidines, 010606 plant biology & botany

Abstract

International audience; The actin cytoskeleton is a dynamic structure that provides an interactive platform for organelles and cellular components. It also serves as track for membranes and vesicles that move via myosin. The actin cytoskeleton of Symbiodinium is a well-organized reticular structure suggestive of multiple membrane interactions, very likely including those of the chloroplast. The Symbiodinium chloroplast membrane network is, in turn, a highly organized structure, suggestive of being under the control of an organizing network. We visualized the chloroplast membranes of cultured Symbiodinium sp. under various light conditions and observed changes dependent on illumination intensity. Since we suspected interaction between these two organelles, and we knew that the Symbiodinium actin cytoskeleton collapses upon treatment with either latrunculin B, an actin microfilament-disrupting agent, or butanedione monoxime, a myosin function inhibitor, we tested the Symbiodinium sp. oxygen evolution in their presence. Upon latrunculin B addition, the oxygen production decreased compared to non-treated cells; however, this was not observed after a 24 h latrunculin treatment. On the contrary, butanedione monoxime treatment caused a non-recoverable dysfunction of the chloroplast causing a severe loss in oxygen production even after long-term exposure. Using electron microscopy, we observed an alteration of the Symbiodinium sp. chloroplast distribution after latrunculin B treatment, with respect to untreated cells. Furthermore, a thorough disorganization of the chloroplast grana was observed after butanedione monoxime treatment. These data suggest that an actomyosin system would be important for chloroplast organization and distribution, and critical for normal photosynthetic function of Symbiodinium sp.

Published

2014

206. A mutation in the converter subdomain of Aspergillus nidulans MyoB blocks constriction of the actomyosin ring in cytokinesis

Author

Brianna L. Hoge, Xiao Wang, Terry W. Hill, and Loretta Jackson-Hayes

Subjects

Myosin Type II, Mutant, Wild type, Hyphae, macromolecular substances, Actomyosin, Biology, Microbiology, Filamentous actin, Actins, Aspergillus nidulans, Cell biology, Protein Structure, Tertiary, Biochemistry, Myosin, Genetics, Latrunculin, Point Mutation, Amino Acid Sequence, Conidium formation, Cytokinesis, Actin

Abstract

We have identified a mutant allele of the Aspergillus nidulans homologue of myosin II (myoB; AN4706), which prevents normal septum formation. This is the first reported myosin II mutation in a filamentous fungus. Strains expressing the myoBG843D allele produce mainly aberrant septa at 30 °C and are completely aseptate at temperatures above 37 °C. Conidium formation is greatly reduced at 30 °C and progressively impaired with increasing temperature. Sequencing of the myoBG843D allele identified a point mutation predicted to result in a glycine-to-aspartate amino acid substitution at residue 843 in the myosin II converter domain. This residue is conserved in all fungal, plant, and animal myosin sequences that we have examined. The mutation does not prevent localization of the myoBG843D gene product to contractile rings, but it does block ring constriction. MyoBG843D rings at sites of abortive septation disassemble after an extended period and dissipate into the cytoplasm. During contractile ring formation, both wild type and mutant MyoB::GFP colocalize with actin – an association that begins at the pre-ring “string” stage. Down-regulation of wild-type myoB expression under control of the alcA promoter blocks septation but does not prevent actin from aggregating at putative septation sites – the actin rings, however, do not fully coalesce. Both septation and targeting of MyoB are blocked by disruption of filamentous actin using latrunculin B. We propose a model in which myosin assembly at septation sites depends upon the presence of F-actin, but assembly of the actin component of contractile rings depends upon normal levels of myosin only for the final stages of ring compaction.

Published

2014

207. Investigating the Role of F-Actin in Human Immunodeficiency Virus Assembly by Live-Cell Microscopy

Author

Peter Koch, Ulrich S. Schwarz, Sheikh Abdul Rahman, Barbara Müller, Julian Weichsel, Hans-Georg Kräusslich, Don C. Lamb, Karl Rohr, and William J. Godinez

Subjects

Viral budding, Immunology, Arp2/3 complex, macromolecular substances, Biology, Microbiology, Filamentous actin, gag Gene Products, Human Immunodeficiency Virus, Virology, Humans, Actin, Total internal reflection fluorescence microscope, Structure and Assembly, Virus Assembly, Optical Imaging, Actin remodeling, Actin cytoskeleton, Actins, Microscopy, Fluorescence, Insect Science, Host-Pathogen Interactions, Biophysics, biology.protein, HIV-1, Latrunculin, HeLa Cells

Abstract

Human immunodeficiency virus type 1 (HIV-1) particles assemble at the plasma membrane, which is lined by a dense network of filamentous actin (F-actin). Large amounts of actin have been detected in HIV-1 virions, proposed to be incorporated by interactions with the nucleocapsid domain of the viral polyprotein Gag. Previous studies addressing the role of F-actin in HIV-1 particle formation using F-actin-interfering drugs did not yield consistent results. Filamentous structures pointing toward nascent HIV-1 budding sites, detected by cryo-electron tomography and atomic force microscopy, prompted us to revisit the role of F-actin in HIV-1 assembly by live-cell microscopy. HeLa cells coexpressing HIV-1 carrying fluorescently labeled Gag and a labeled F-actin-binding peptide were imaged by live-cell total internal reflection fluorescence microscopy (TIR-FM). Computational analysis of image series did not reveal characteristic patterns of F-actin in the vicinity of viral budding sites. Furthermore, no transient recruitment of F-actin during bud formation was detected by monitoring fluorescence intensity changes at nascent HIV-1 assembly sites. The chosen approach allowed us to measure the effect of F-actin-interfering drugs on the assembly of individual virions in parallel with monitoring changes in the F-actin network of the respective cell. Treatment of cells with latrunculin did not affect the efficiency and dynamics of Gag assembly under conditions resulting in the disruption of F-actin filaments. Normal assembly rates were also observed upon transient stabilization of F-actin by short-term treatment with jasplakinolide. Taken together, these findings indicate that actin filament dynamics are dispensable for HIV-1 Gag assembly at the plasma membrane of HeLa cells. IMPORTANCE HIV-1 particles assemble at the plasma membrane of virus-producing cells. This membrane is lined by a dense network of actin filaments that might either present a physical obstacle to the formation of virus particles or generate force promoting the assembly process. Drug-mediated interference with the actin cytoskeleton showed different results for the formation of retroviral particles in different studies, likely due to general effects on the cell upon prolonged drug treatment. Here, we characterized the effect of actin-interfering compounds on the HIV-1 assembly process by direct observation of virus formation in live cells, which allowed us to measure assembly rate constants directly upon drug addition. Virus assembly proceeded with normal rates when actin filaments were either disrupted or stabilized. Taken together with the absence of characteristic actin filament patterns at viral budding sites in our analyses, this indicates that the actin network is dispensable for HIV-1 assembly.

Published

2014

208. Expression of type I collagen and tenascin C is regulated by actin polymerization through MRTF in dedifferentiated chondrocytes

Author

Elizabeth Delve, Sneha Raju, Justin Parreno, Rita A. Kandel, Amy Jiang, Katarina Andrejevic, and Mortah Nabavi Niaki

Subjects

Myocardin related transcription factor, Biophysics, Active Transport, Cell Nucleus, macromolecular substances, Biochemistry, Chondrocyte, Collagen Type I, Polymerization, Chondrocytes, Structural Biology, Gene expression, Tenascin C, Genetics, medicine, Animals, Anilides, Fibroblast, Molecular Biology, Actin, Cell Nucleus, biology, Chemistry, Tenascin, Cell Biology, Cell Dedifferentiation, musculoskeletal system, Bridged Bicyclo Compounds, Heterocyclic, Molecular biology, Actins, medicine.anatomical_structure, Myocardin, embryonic structures, Benzamides, biology.protein, Latrunculin, Thiazolidines, Cattle, Dedifferentiation, Collagen, Type I collagen, Transcription Factors

Abstract

This study examined actin regulation of fibroblast matrix genes in dedifferentiated chondrocytes. We demonstrated that dedifferentiated chondrocytes exhibit increased actin polymerization, nuclear localization of myocardin related transcription factor (MRTF), increased type I collagen (col1) and tenascin C (Tnc) gene expression, and decreased Sox9 gene expression. Induction of actin depolymerization by latrunculin treatment or cell rounding, reduced MRTF nuclear localization, repressed col1 and Tnc expression, and increased Sox9 gene expression in dedifferentiated chondrocytes. Treatment of passaged chondrocytes with MRTF inhibitor repressed col1 and Tnc expression, but did not affect Sox9 expression. Our results show that actin polymerization regulates fibroblast matrix gene expression through MRTF in passaged chondrocytes.

Published

2014

209. Role of turgor pressure in endocytosis in fission yeast

Author

Fred Chang, Emilia Laura Munteanu, and Roshni Basu

Subjects

Time Factors, Endocytic cycle, Turgor pressure, Ingression, Biology, Endocytosis, Time-Lapse Imaging, Bulk endocytosis, Cell membrane, Cell wall, 03 medical and health sciences, 0302 clinical medicine, Cell Wall, Schizosaccharomyces, medicine, Pressure, Sorbitol, Molecular Biology, 030304 developmental biology, 0303 health sciences, Cell Membrane, Cell Biology, Articles, Actins, Cell biology, medicine.anatomical_structure, Membrane Trafficking, Latrunculin, 030217 neurology & neurosurgery

Abstract

During endocytosis, actin-dependent forces are needed to oppose internal turgor pressure for invagination of the plasma membrane. Live-cell imaging shows that addition of sorbitol to the medium significantly accelerates early steps in the endocytic process and rescues defects of endocytic mutants in fission yeast., Yeast and other walled cells possess high internal turgor pressure that allows them to grow and survive in the environment. This turgor pressure, however, may oppose the invagination of the plasma membrane needed for endocytosis. Here we study the effects of turgor pressure on endocytosis in the fission yeast Schizosaccharomyces pombe by time-lapse imaging of individual endocytic sites. Decreasing effective turgor pressure by addition of sorbitol to the media significantly accelerates early steps in the endocytic process before actin assembly and membrane ingression but does not affect the velocity or depth of ingression of the endocytic pit in wild-type cells. Sorbitol also rescues endocytic ingression defects of certain endocytic mutants and of cells treated with a low dose of the actin inhibitor latrunculin A. Endocytosis proceeds after removal of the cell wall, suggesting that the cell wall does not contribute mechanically to this process. These studies suggest that endocytosis is governed by a mechanical balance between local actin-dependent inward forces and opposing forces from high internal turgor pressure on the plasma membrane.

Published

2014

210. The calcineurin inhibitor Ascomicin interferes with the early stage of the epileptogenic process induced by Latrunculin A microperfusion in rat hippocampus

Author

Germán Sierra-Marcuño, Germán Sierra-Paredes, Carmen Freire-Cobo, and Manuel Freire

Subjects

Male, Microdialysis, Immunology, Calcineurin Inhibitors, Neuroscience (miscellaneous), AMPA receptor, Biology, Epileptogenesis, Hippocampus, Tacrolimus, Rats, Sprague-Dawley, Epilepsy, medicine, Immunology and Allergy, Animals, Infusion Pumps, Pharmacology, Glutamate receptor, Actin cytoskeleton, medicine.disease, Bridged Bicyclo Compounds, Heterocyclic, Rats, Synaptic plasticity, NMDA receptor, Latrunculin, Thiazolidines, Neuroscience

Abstract

Latrunculin A microperfusion in rat hippocampus has shown to be an effective model of acute and chronic seizures for neurochemical studies. The intervention over early synaptic plasticity changes after the epileptogenesis onset represents a big challenge on the design of a suitable therapy to impair the epilepsy development. We previously suggested that receptor location might be essential for controlling neuronal excitability, and that disruption of local cytoskeletal dynamics followed by drastic changes in the synaptic/extrasynaptic ratio of NMDA, AMPA receptors and their subsequent downstream signalling may play an important role in the pathogenesis of seizures. In the present study, we performed a pharmacological intervention in the Latrunculin model by using Ascomicin (ASC) and Phenytoin (PHT). We pointed out the inhibitory action of ASC over the protein phosphatase 2B (PP2B). PP2B pathological mechanism involves changes in actin cytoskeleton and showed to avoid those subsequent changes previously observed in PSD components. On the contrary, PHT didn’t seem to modify the F-actin depolymerization process induced, showing a similar redistribution pattern from the PSD towards the extrasynaptic site of several molecular components with more or less dependence on actin for their location, including glutamate receptors. Overall, we propose that the early intervention over changes on the synapse during the epileptogenic process might represent the best approach to avoid the onset of chronic refractory seizures our model. On this regard, the therapeutic potential of ASC, FK506 and derivatives should be further explored as a possible tool in the intervention over epilepsy and other brain diseases.

Published

2014

211. Effects of eslicarbazepine acetate on acute and chronic latrunculin A-induced seizures and extracellular amino acid levels in the mouse hippocampus

Author

Germán Sierra-Paredes, Patrício Soares-da-Silva, Germán Sierra-Marcuño, Lyndon C. Wright, Ana I. Loureiro, and Universidade de Santiago de Compostela. Departamento de Bioquímica e Bioloxía Molecular

Subjects

Male, Taurine, Glycine, Glutamic Acid, Pharmacology, Eslicarbazepine acetate, Hippocampus, gamma-Aminobutyric acid, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Mice, Oral administration, Dibenzazepines, Seizures, Extracellular, Medicine, Animals, Latrunculin A-induced seizures, Amino Acids, gamma-Aminobutyric Acid, Eslicarbazepine, Aspartic Acid, business.industry, General Neuroscience, Glutamate receptor, Glutamic acid, Bridged Bicyclo Compounds, Heterocyclic, Disease Models, Animal, chemistry, Aspartate, Acute Disease, Chronic Disease, Anticonvulsant drugs, Latrunculin, Thiazolidines, Anticonvulsants, Glutamate, business, Extracellular Space, medicine.drug, Research Article

Abstract

Background: Latrunculin A microperfusion of the hippocampus induces acute epileptic seizures and long-term biochemical changes leading to spontaneous seizures. This study tested the effect of eslicarbazepine acetate (ESL), a novel antiepileptic drug, on latrunculin A-induced acute and chronic seizures, and changes in brain amino acid extracellular levels. Hippocampi of Swiss mice were continuously perfused with a latrunculin A solution (4 μM, 1 μl/min, 7 h/day) with continuous EEG and videotape recording for 3 consecutive days. Microdialysate samples were analyzed by HPLC and fluorescence detection of taurine, glycine, aspartate, glutamate and GABA. Thereafter, mice were continuously video monitored for two months to identify chronic spontaneous seizures or behavioral changes. Control EEG recordings (8 h) were performed in all animals at least once a week for a minimum of one month. Results: Oral administration of ESL (100 mg/kg), previous to latrunculin A microperfusion, completely prevented acute latrunculin A-induced seizures as well as chronic seizures and all EEG chronic signs of paroxysmal activity. Hippocampal extracellular levels of taurine, glycine and aspartate were significantly increased during latrunculin A microperfusion, while GABA and glutamate levels remained unchanged. ESL reversed the increases in extracellular taurine, glycine and aspartate concentrations to basal levels and significantly reduced glutamate levels. Plasma and brain bioanalysis showed that ESL was completely metabolized within 1 h after administration to mainly eslicarbazepine, its major active metabolite. Conclusion: ESL treatment prevented acute latrunculin A-induced seizures as well as chronic seizures and all EEG chronic signs of paroxysmal activity, supporting a possible anti-epileptogenic effect of ESL in mice. This study was sponsored by BIAL – Portela & Cª, S.A. SI

Published

2014

212. Cell substratum adhesion during early development of Dictyostelium discoideum

Author

Danny Fuller, Eberhard Bodenschatz, Marco Tarantola, Wouter-Jan Rappel, Albert Bae, and William F. Loomis

Subjects

Talin, Integrins, Mutant, Protozoan Proteins, lcsh:Medicine, Microscopy, Atomic Force, Microbiology, Dictyostelium discoideum, Focal adhesion, Molecular Genetics, 03 medical and health sciences, Cell Movement, Cell Adhesion, Genetics, Dictyostelium, Cell adhesion, lcsh:Science, Molecular Biology, Adhesives, Cytoskeleton, Extracellular matrix proteins, Glass, Membrane proteins, Microfluidics, Shear stresses, 030304 developmental biology, 0303 health sciences, Focal Adhesions, Multidisciplinary, biology, 030302 biochemistry & molecular biology, Microbial Mutation, lcsh:R, Wild type, Biology and Life Sciences, Cell Differentiation, Cell Biology, Microfluidic Analytical Techniques, biology.organism_classification, Actin cytoskeleton, Cell biology, Mutation, Latrunculin, lcsh:Q, Single-Cell Analysis, Research Article, Developmental Biology

Abstract

Vegetative and developed amoebae of Dictyostelium discoideum gain traction and move rapidly on a wide range of substrata without forming focal adhesions. We used two independent assays to quantify cell-substrate adhesion in mutants and in wild-type cells as a function of development. Using a microfluidic device that generates a range of hydrodynamic shear stress, we found that substratum adhesion decreases at least 10 fold during the first 6 hr of development of wild type cells. This result was confirmed using a single-cell assay in which cells were attached to the cantilever of an atomic force probe and allowed to adhere to untreated glass surfaces before being retracted. Both of these assays showed that the decrease in substratum adhesion was dependent on the cAMP receptor CAR1 which triggers development. Vegetative cells missing talin as the result of a mutation in talA exhibited slightly reduced adhesive properties compared to vegetative wild-type cells. In sharp contrast to wild-type cells, however, these talA mutant cells did not show further reduction of adhesion during development such that after 5 hr of development they were significantly more adhesive than developed wild type cells. In addition, both assays showed that substrate adhesion was reduced in 0 hr cells when the actin cytoskeleton was disrupted by latrunculin. Consistent with previous observations, substrate adhesion was also reduced in 0 hr cells lacking the membrane proteins SadA or SibA as the result of mutations in sadA or sibA. However, there was no difference in the adhesion properties between wild type AX3 cells and these mutant cells after 6 hr of development, suggesting that neither SibA nor SadA play an essential role in substratum adhesion during aggregation. Our results provide a quantitative framework for further studies of cell substratum adhesion in Dictyostelium. peerReviewed

Published

2014

213. Influence of Actin Cytoskeleton on Intra-articular and Interstitial Fluid Pressures in Synovial Joints

Author

D. Scott, Anna Poli, J.R. Levick, Roger M. Mason, G. Miserocchi, K. Bertin, Poli, A, Scott, D, Bertin, K, Miserocchi, G, Mason, R, and Levick, J

Subjects

Cartilage, Articular, Cytochalasin D, Knee Joint, Metabolic Clearance Rate, Latrunculin, Biochemistry, Capillary Permeability, chemistry.chemical_compound, Osmotic Pressure, Interstitial fluid, Endothelial permeability, Synovium, Synovial Fluid, Extracellular fluid, Joint capsule, medicine, Animals, Synovial fluid, Cytochalasin, Actin, Actins, Cytoskeleton, Endothelium, Extracellular Space, Hindlimb, Kinetics, Microcirculation, Rabbits, Synovial Membrane, gamma-Globulins, Cardiology and Cardiovascular Medicine, Cell Biology, Anatomy, Actin cytoskeleton, Cartilage, medicine.anatomical_structure, chemistry, Biophysics, Synovial membrane, Articular

Abstract

Fibroblast microfilamentous actin (F-actin) influences interstitial fluid pressure via linkages to collagen in rat skin (Berg et al., 2001). The present aims were to determine whether the actin cytoskeleton of synovial endothelium, fibroblasts, and synoviocytes influences in vivo (i) fluid exchange between a joint cavity and synovial microcirculation and (ii) extracellular fluid pressures in joints. Rabbit knee joints were treated intra-articularly with the F-actin disrupting drugs cytochalasin D and latrunculin B while joint fluid pressure P(j) was recorded. In joints injected with small volumes of control solution, P(j) fell with time (-0.05 +/- 0.01 cm H2O x min(-1), mean +/- SEM, n = 9, equivalent drainage rate 3.9 microl x min(-1)). Cytochalasin or latrunculin reversed this in approximately 4 min in vivo; P(j) increased with time, e.g., +0.12 +/- 0.04 cm H2O x min(-1) at 200 microM cytochalasin (equivalent filtration rate into joint 6.6-12.5 microl x min(-1), n = 4), with a cytochalasin EC50 of 45 microM. Plasma gamma-globulin clearance into the joint cavity was also increased. Post mortem, cytochalasin did not reverse dP(j)/dt and had no more effect on P(j) than did control solution. Also, when synovial interstitial fluid pressures were measured by servonull micropipette post mortem (control -0.95 +/- 0.37 cmH2O, n = 18) cytochalasin had no significant effect on interstitial pressure over 60 min, even at 1 mM. It was concluded that synovial endothelial F-actin has an important role in the normal synovial microvascular resistance to fluid filtration and plasma gamma-globulin permeation and is thus a potential link between pro-inflammatory mediators and arthritic joint effusions. The results provided no support for the hypothesis that synoviocyte F-actin influences the swelling tendency of synovial matrix and hence extracellular fluid pressures, in contrast to the findings of Berg et al. (2001) in rat dermis.

Published

2001

214. Actin Microfilaments Facilitate the Retrograde Transport from the Golgi Complex to the Endoplasmic Reticulum in Mammalian Cells

Author

Ferran Valderrama, Teresa Babia, Jaime Renau-Piqueras, Holger Barth, Juan M. Duran, and Gustavo Egea

Subjects

Endoplasmic reticulum, Arp2/3 complex, macromolecular substances, Cell Biology, Golgi apparatus, Biology, Actin cytoskeleton, Microfilament, Biochemistry, Cell biology, symbols.namesake, Actin remodeling of neurons, Structural Biology, Genetics, symbols, biology.protein, Latrunculin, Molecular Biology, Secretory pathway

Abstract

The morphology and subcellular positioning of the Golgi complex depend on both microtubule and actin cytoskeletons. In contrast to microtubules, the role of actin cytoskeleton in the secretory pathway in mammalian cells has not been clearly established. Using cytochalasin D, we have previously shown that microfilaments are not involved in the endoplasmic reticulum–Golgi membrane dynamics. However, it has been reported that, unlike botulinum C2 toxin and latrunculins, cytochalasin D does not produce net depolymerization of actin filaments. Therefore, we have reassessed the functional role of actin microfilaments in the early steps of the biosynthetic pathway using C2 toxin and latrunculin B. The anterograde endoplasmic reticulum-to-Golgi transport monitored with the vesicular stomatitis virus-G protein remained unaltered in cells treated with cytochalasin D, latrunculin B or C2 toxin. Conversely, the brefeldin A-induced Golgi membrane fusion into the endoplasmic reticulum, the Golgi-to-endoplasmic reticulum transport of a Shiga toxin mutant form, and the subcellular distribution of the KDEL receptor were all impaired when actin microfilaments were depolymerized by latrunculin B or C2 toxin. These findings, together with the fact that COPI-coated and uncoated vesicles contain β/γ-actin isoforms, indicate that actin microfilaments are involved in the endoplasmic reticulum/Golgi interface, facilitating the retrograde Golgi-to-endoplasmic reticulum membrane transport, which could be mediated by the orchestrated movement of transport intermediates along microtubule and microfilament tracks.

Published

2001

215. Delta regulates keratinocyte spreading and motility independently of differentiation

Author

Sally Lowell and Fiona M. Watt

Subjects

Keratinocytes, Embryology, Cellular differentiation, Genetic Vectors, Motility, Biology, Transfection, Cell Movement, Cell Adhesion, medicine, Drosophila Proteins, Humans, Pseudopodia, Cytoskeleton, Cells, Cultured, Receptors, Notch, Cell Membrane, Intracellular Signaling Peptides and Proteins, Membrane Proteins, Cell Differentiation, Bridged Bicyclo Compounds, Heterocyclic, Actin cytoskeleton, Actins, Culture Media, Cell biology, Repressor Proteins, Thiazoles, medicine.anatomical_structure, Mutation, Thiazolidines, Latrunculin, Calcium, Lamellipodium, Keratinocyte, Signal Transduction, Developmental Biology

Abstract

In human interfollicular epidermis stem cells lie in clusters surrounded by their differentiated daughters, transit amplifying cells, an arrangement that reflects differences in cell cohesiveness and motility. Keratinocytes expressing a dominant negative Delta1 mutant, Delta T , lacking most of the cytoplasmic domain, acquired the motile behaviour of transit cells while retaining their stem cell identity. Conversely, overexpression of Delta1 promoted keratinocyte cohesiveness. The adhesive effects of Delta1 and Delta T were independent of SuH-dependent Notch signalling. Delta T increased motility and spreading of individual keratinocytes and stimulated lamellipodia formation. Delta and Delta T colocalised with cortical actin and redistributed on Latrunculin treatment. We propose that Delta promotes keratinocyte cohesiveness by restricting motility and discuss potential mechanisms by which Delta could interact with the actin cytoskeleton.

Published

2001

216. Regulation of Dendritic Spine Motility in Cultured Hippocampal Neurons

Author

Eduard Korkotian and Menahem Segal

Subjects

musculoskeletal diseases, Time Factors, Dendritic spine, Green Fluorescent Proteins, Presynaptic Terminals, Synaptophysin, Action Potentials, Motility, Pyridinium Compounds, Dendrite, Tetrodotoxin, Hippocampal formation, Biology, Hippocampus, Calcium in biology, Mice, Actin remodeling of neurons, medicine, Animals, Particle Size, ARTICLE, Cells, Cultured, Fluorescent Dyes, Neurons, Microscopy, Confocal, General Neuroscience, Temperature, Dendrites, Bridged Bicyclo Compounds, Heterocyclic, Rats, Dendritic filopodia, Cell biology, Quaternary Ammonium Compounds, Luminescent Proteins, Thiazoles, medicine.anatomical_structure, Thiazolidines, Latrunculin, Calcium, Cell Surface Extensions

Abstract

Regulation of dendritic spine motility was studied in dissociated cultures of the rat and mouse hippocampus, using green fluorescent protein-labeled neurons or neurons loaded with the calcium-sensitive dye Oregon Green-1. Cells were time-lapse-photographed on a confocal laser-scanning microscope at high resolution to detect movements as well as spontaneous fluctuations of intracellular calcium concentrations in their dendritic spines. Active presynaptic terminals attached to the spines were labeled with FM4-64, which marks a subset of synaptophysin-labeled terminals. Dendritic spines were highly motile in young, 4- to 7-d-old cells. At this age, neurons had little spontaneous calcium fluctuation or FM4-64 labeling. Within 2–3 weeks in culture, dendritic spines were much less motile, they were associated with active presynaptic terminals, and they expressed high rates of spontaneous calcium fluctuations. Irrespective of age, and even on the same dendrite, there was an inverse relationship between spine motility and presence of FM4-64-labeled terminals in contact with the imaged spines. Spine motility was blocked by latrunculin, which prevents actin polymerization, and was disinhibited by blockade of action potential discharges with tetrodotoxin. It is proposed that an active presynaptic terminal restricts motility of dendritic spines.

Published

2001

217. Myosin V-mediated vacuole distribution and fusion in fission yeast

Author

Thein Z. Win, Daniel P. Mulvihill, Jeremy S. Hyams, and Patrick J. Pollard

Subjects

Myosin Light Chains, Myosin light-chain kinase, Recombinant Fusion Proteins, Genes, Fungal, Myosin Type V, Nerve Tissue Proteins, Vacuole fusion, Vacuole, Biology, Membrane Fusion, General Biochemistry, Genetics and Molecular Biology, Phragmosome, Fungal Proteins, 03 medical and health sciences, 0302 clinical medicine, Schizosaccharomyces, Myosin, Actin, 030304 developmental biology, 0303 health sciences, Agricultural and Biological Sciences(all), Biochemistry, Genetics and Molecular Biology(all), Molecular Motor Proteins, Lipid bilayer fusion, Cell biology, Mutation, Vacuoles, Latrunculin, Calmodulin-Binding Proteins, General Agricultural and Biological Sciences, 030217 neurology & neurosurgery

Abstract

The class V myosins are actin-based motors that move a variety of cellular cargoes [1]. In budding yeast, their activity includes the relocation of a portion of the vacuole from the mother cell to the bud [2, 3]. Fission yeast cells contain numerous (approximately 80) small vacuoles. When S. pombe cells are placed in water, vacuoles fuse in response to osmotic stress [4]. Fission yeast possess two type V myosin genes, myo51(+) and myo52(+) [5]. In a myo51Delta strain, vacuoles were distributed throughout the cell, and mean vacuole diameter was identical to that seen in wild-type cells. When myo51Delta and wild-type cells were placed in water, vacuoles enlarged by fusion. In myo52Delta cells, by contrast, vacuoles were smaller and mostly clustered around the nucleus, and fusion in water was largely inhibited. When cells containing GFP-Myo52 were placed in water, Myo52 was seen to redistribute from the cell poles to the surface of the fusing vacuoles. Vacuole fusion in fission yeast was inhibited by the microtubule drug thiabendazole (TBZ) but not by the actin inhibitor latrunculin B. This is the first demonstration of the involvement of a type V myosin, possibly via an interaction with microtubules, in homotypic membrane fusion.

Published

2001

218. Translocation of the B Cell Antigen Receptor into Lipid Rafts Reveals a Novel Step in Signaling

Author

Susan K. Pierce, Paul C. Cheng, Wenxia Song, and Bruce K. Brown

Subjects

Immunology, B-cell receptor, Biological Transport, Active, Receptors, Antigen, B-Cell, macromolecular substances, Biology, Mice, Membrane Microdomains, Antigens, CD, LYN, hemic and lymphatic diseases, Tumor Cells, Cultured, Animals, Humans, Immunology and Allergy, Src family kinase, Phosphorylation, Lipid raft, Cytoskeleton, Immunoglobulin mu-Chains, Cell Membrane, Receptors, IgG, Temperature, breakpoint cluster region, Actin cytoskeleton, Actins, Cell biology, Enzyme Activation, src-Family Kinases, Mutagenesis, Site-Directed, Tyrosine, Latrunculin, lipids (amino acids, peptides, and proteins), Signal transduction, CD79 Antigens, Signal Transduction

Abstract

The cross-linking of the B cell Ag receptor (BCR) leads to the initiation of a signal transduction cascade in which the earliest events involve the phosphorylation of the immunoreceptor tyrosine-based activation motifs of Igα and Igβ by the Src family kinase Lyn and association of the BCR with the actin cytoskeleton. However, the mechanism by which BCR cross-linking initiates the cascade remains obscure. In this study, using various A20-transfected cell lines, biochemical and genetic evidence is provided that BCR cross-linking leads to the translocation of the BCR into cholesterol- and sphingolipid-rich lipid rafts in a process that is independent of the initiation of BCR signaling and does not require the actin cytoskeleton. Translocation of the BCR into lipid rafts did not require the Igα/Igβ signaling complex, was not dependent on engagement of the FcR, and was not blocked by the Src family kinase inhibitor PP2 or the actin-depolymerizing agents cytochalasin D or latrunculin. Thus, cross-linking or oligomerization of the BCR induces the BCR translocation into lipid rafts, defining an event in B cell activation that precedes receptor phosphorylation and association with the actin cytoskeleton.

Published

2001

219. An Antiprion Effect of the Anticytoskeletal Drug Latrunculin A in Yeast

Author

Gary P. Newnam, Yury O. Chernoff, Bailleul-Winslett Pa, and Renee D. Wegrzyn

Subjects

Saccharomyces cerevisiae Proteins, Prions, Saccharomyces cerevisiae, macromolecular substances, Cycloheximide, Article, Fungal Proteins, chemistry.chemical_compound, Genetics, Cytoskeleton, Molecular Biology, Heat-Shock Proteins, Actin, Fungal protein, Bridged Bicyclo Compounds, Heterocyclic, Actin cytoskeleton, Actins, Cell biology, Thiazoles, chemistry, Thiazolidines, Sodium azide, Latrunculin, Marine Toxins, Marine toxin, Peptide Termination Factors

Abstract

Prions are infectious aggregation-prone isoforms of the normal proteins, supposedly able to seed aggregation of the normal cellular counterparts. In vitro, prion proteins form amyloid fibers, resembling cytoskeletal structures. Yeast prion [PSI], which is a cytoplasmically inherited aggregated isoform of the translation termination factor Sup35p (eRF3), serves as a useful model for studying mechanisms of prion diseases and other amyloidoses. The previously described interaction between Sup35p and cytoskeletal assembly protein Slalp points to the possible relationships between prions and cytoskeletal networks. Although the Sup35PSI+ aggregates do not colocalize with actin patches, we have shown that yeast cells are efficiently cured of the [PSI] prion by prolonged incubation with latrunculin A, a drug disrupting the actin cytoskeleton. On the other hand, treatments with sodium azide or cycloheximide, agents blocking yeast protein synthesis and cell proliferation but not disrupting the cytoskeleton, do not cause a significant loss of [PSI]. Moreover, simultaneous treatment with sodium azide or cycloheximide blocks [PSI] curing by latrunculin A, indicating that prion loss in the presence of latrunculin A requires a continuation of protein synthesis during cytoskeleton disruption. The sodium azide treatment also decreases the toxic effect of latrunculin A. Latrunculin A influences neither the levels of total cellular Sup35p nor the levels of chaperone proteins, such as Hspl04 and Hsp70, which were previously shown to affect [PSI]. This makes an indirect effect of latrunculin A on [PSI] via induction of Hsps unlikely. Fluorescence microscopy detects changes in the structure and/or localization of the Sup35PSI+ aggregates in latrunculin A-treated cells. We conclude that the stable maintenance of the [PSI] prion aggregates in the protein-synthesizing yeast cells partly depends on an intact actin cytoskeleton, suggesting that anticytoskeletal treatments could be used to counteract some aggregation-related disorders.

Published

2001

220. Effects of cytochalasin D and latrunculin B on mechanical properties of cells

Author

B. Schwab, N.C. Thompson, Tetsuro Wakatsuki, and Elliot L. Elson

Subjects

Cytochalasin D, Embryo, Nonmammalian, Motility, macromolecular substances, Biology, Extracellular matrix, chemistry.chemical_compound, medicine, Animals, Fibroblast, Cells, Cultured, Actin, Dose-Response Relationship, Drug, Cell Biology, Fibroblasts, Bridged Bicyclo Compounds, Heterocyclic, Actin cytoskeleton, Actins, Cell biology, Thiazoles, medicine.anatomical_structure, Microscopy, Fluorescence, chemistry, Thiazolidines, Latrunculin, Wound healing, Chickens

Abstract

Actin microfilaments transmit traction and contraction forces generated within a cell to the extracellular matrix during embryonic development, wound healing and cell motility, and to maintain tissue structure and tone. Therefore, the state of the actin cytoskeleton strongly influences the mechanical properties of cells and tissues. Cytochalasin D and Latrunculin are commonly used reagents that, by different mechanisms, alter the state of actin polymerization or the organization of actin filaments. We have investigated the effect of a wide range of Cytochalasin D and Latrunculin B concentrations (from 40 pM to 10 microM) on the mechanical properties of the cells within fibroblast populated collagen matrices. Contractile force and dynamic stiffness were measured by uniaxial stress-strain testing. The range of effective concentrations of Cytochalasin D (200 pM-2 microM) was broader than that of Latrunculin B (20 nM-200 nM). Activating the cells by serum did not change the effective range of Cytochalasin D concentrations but shifted that of Latrunculin B upward by tenfold. Simple mathematical binding models based on the presumed mechanisms of action of Cytochalasin D and Latrunculin B simulated the concentration-dependent mechanical changes reasonably well. This study shows a strong dependence of the mechanical properties of cells and tissues on the organization and degree of polymerization of actin filaments.

Published

2001

221. Rho GTPase activity modulates Pseudomonas aeruginosa internalization by epithelial cells

Author

Tzuu-Shuh Jou, Keith E. Mostov, Joanne N. Engel, and B. I. Kazmierczak

Subjects

rac1 GTP-Binding Protein, rho GTP-Binding Proteins, RHOA, GTP', media_common.quotation_subject, Bacterial Toxins, education, Immunology, RAC1, GTPase, CDC42, Biology, Models, Biological, Microbiology, Dogs, Virology, Animals, Humans, cdc42 GTP-Binding Protein, Internalization, Cells, Cultured, media_common, Tight junction, Cytotoxins, Escherichia coli Proteins, Epithelial Cells, Cell biology, Enzyme Activation, Pseudomonas aeruginosa, biology.protein, Latrunculin, rhoA GTP-Binding Protein

Abstract

Summary The Gram-negative pathogen Pseudomonas aeruginosa invades epithelial cells in vivo and in vitro .W e have examined the pathway(s) by which epithelial cells internalize P. aeruginosa strain PA103 using Madin-Darby canine kidney (MDCK) cells. We have recently demonstrated that P. aeruginosa internalization occurs by an actin-dependent Toxin B-inhibited pathway which becomes downregulated as epithelial cells become polarized, suggesting that one or more of the Rho family GTPases is involved in bacterial internalization. Here, we demonstrate that activation of the Rho family GTPases by cytotoxic necrotizing factor 1 (CNF-1) stimulates P. aeruginosa internalization. Examination of the roles of the individual Rho family GTPases in internalization shows that expression of a constitutively active allele of RhoA (RhoAV14), but not of constitutively active Rac1 (Rac1V12) or Cdc42 (Cdc42V12), is sufficient to increase uptake of PA103pscJ. This relative increase persists when bacterial infection is established at the basolateral surface of polarized cells, suggesting that the effect of RhoAV14 is not simply due to its known ability to disrupt tight junction integrity in polarized cells. RhoAV14-mediated stimulation of bacterial uptake is actin dependent as it is abrogated by exposure to latrunculin A. We also find that endogenous Rho GTP levels in epithelial cells are increased by infection with an internalized strain of P. aeruginosa; conversely, a poorly internalized isogenic strain expressing the bacterial anti-internalization protein ExoT causes decreased Rho GTP levels. Experimental inhibition of Rho, either by expressing dominant negative RhoAN19 or by inhibiting native Rho using a membrane permeable fusion construct of a Rho-specific inhibitor, C3 ADP-ribosyltransferase, does not inhibit PA103pscJ internalization in MDCK or HeLa cells. Models consistent with these data are presented.

Published

2001

222. Tara, a novel F-actin binding protein, associates with the Trio guanine nucleotide exchange factor and regulates actin cytoskeletal organization

Author

Elizabeth Iannotti, Katja Seipel, Stephen J. O'Brien, Quintus G. Medley, and Michel Streuli

Subjects

Recombinant Fusion Proteins, Molecular Sequence Data, macromolecular substances, Protein Serine-Threonine Kinases, Biology, Transfection, Cell morphology, GTP-Binding Proteins, Chlorocebus aethiops, Animals, Drosophila Proteins, Guanine Nucleotide Exchange Factors, Humans, Amino Acid Sequence, Muscle, Skeletal, Cytoskeleton, Actin, Gene Library, Sequence Homology, Amino Acid, Microfilament Proteins, Actin cytoskeleton reorganization, Actin remodeling, Cell Biology, Fibroblasts, Phosphoproteins, Actin cytoskeleton, Actins, Cell biology, COS Cells, Latrunculin, Guanine nucleotide exchange factor, Sequence Alignment, Cytokinesis, HeLa Cells

Abstract

Reorganization of the actin cytoskeleton is essential to numerous cellular processes including cell locomotion and cytokinesis. This actin remodeling is regulated in part by Rho family GTPases. Previous studies implicated Trio, a Dbl-homology guanine nucleotide exchange factor with two exchange factor domains, in regulating actin cytoskeleton reorganization, cell motility and cell growth via activation of Rho GTPases. Trio is essential for mouse embryonic development and Trio-deficiency is associated with abnormal skeletal muscle and neural tissue development. Furthermore, genetic analyses in Caenorhabditis elegans and Drosophila demonstrate a role for trio-like genes in cell migration and axon guidance. Herein we characterize a novel Trio-binding protein, Tara, that is comprised of an N-terminal pleckstrin homology domain and a C-terminal coiled-coil region. Trio and Tara associate as assessed by the yeast interaction-trap assays and mammalian co-immunoprecipitation studies. Ectopically expressed Tara localizes to F-actin in a periodic pattern that is highly similar to the pattern of myosin II. Furthermore, a direct interaction between Tara and F-actin is indicated by in vitro binding studies. Cells that transiently or stably overexpress Tara display an extensively flattened cell morphology with enhanced stress fibers and cortical F-actin. Tara expression does not alter the ability of the cell to attach or to initially spread, but rather increases cell spreading following these initial events. Tara stabilizes F-actin structures as indicated by the relative resistance of Tara-expressing cells to the F-actin destabilizer Latrunculin B. We propose that Tara regulates actin cytoskeletal organization by directly binding and stabilizing F-actin, and that the localized formation of Tara and Trio complexes functions to coordinate actin remodeling.

Published

2001

223. Microtubules Are Involved in Glucose-dependent Dissociation of the Yeast Vacuolar [H+]-ATPase in Vivo

Author

Ting Xu and Michael Forgac

Subjects

G2 Phase, Vacuolar Proton-Translocating ATPases, Cell cycle checkpoint, Protein Conformation, Antineoplastic Agents, Saccharomyces cerevisiae, Microtubules, Biochemistry, Cell cycle phase, chemistry.chemical_compound, Microtubule, Molecular Biology, Cytoskeleton, Actin, biology, Nocodazole, Temperature, Cell Biology, Bridged Bicyclo Compounds, Heterocyclic, Yeast, Cell biology, Proton-Translocating ATPases, Thiazoles, Glucose, Tubulin, chemistry, biology.protein, Thiazolidines, Latrunculin

Abstract

The vacuolar [H(+)]-ATPases (V-ATPases) are composed of a peripheral V(1) domain and a membrane-embedded V(0) domain. Reversible dissociation of the V(1) and V(0) domains has been observed in both yeast and insects and has been suggested to represent a general regulatory mechanism for controlling V-ATPase activity in vivo. In yeast, dissociation of the V-ATPase is triggered by glucose depletion, but the signaling pathways that connect V-ATPase dissociation and glucose metabolism have not been identified. We have found that nocodazole, an agent that disrupts microtubules, partially blocked dissociation of the V-ATPase in response to glucose depletion in yeast. By contrast, latrunculin, an agent that disrupts actin filaments, had no effect on glucose-dependent dissociation of the V-ATPase complex. Neither nocodazole nor latrunculin blocked reassembly of the V-ATPase upon re-addition of glucose to the medium. The effect of nocodazole appears to be specifically through disruption of microtubules since glucose-dependent dissociation of the V-ATPase was not blocked by nocodazole in yeast strains bearing a mutation in tubulin that renders it resistant to nocodazole. Because nocodazole has been shown to arrest cells in the G(2) phase of the cell cycle, it was of interest to determine whether nocodazole exerted its effect on dissociation of the V-ATPase through cell cycle arrest. Glucose-dependent dissociation of the V-ATPase was examined in four yeast strains bearing temperature-sensitive mutations that arrest cells in different stages of the cell cycle. Because dissociation of the V-ATPase occurred normally at both the permissive and restrictive temperatures in these mutants, the results suggest that in vivo dissociation is not dependent upon cell cycle phase.

Published

2001

224. Involvement of actin filaments and integrins in the binding step in collagen phagocytosis by human fibroblasts

Author

Pamma D. Arora, G. Segal, Gregory P. Downey, Marc D. McKee, Christopher A. McCulloch, and Wilson Lee

Subjects

Integrins, Receptors, Collagen, media_common.quotation_subject, Integrin, macromolecular substances, Collagen receptor, chemistry.chemical_compound, Phagocytosis, Humans, Internalization, Cells, Cultured, Actin, media_common, Cytochalasin D, Integrin binding, biology, Fluorescence recovery after photobleaching, Cell Biology, Fibroblasts, Bridged Bicyclo Compounds, Heterocyclic, Molecular biology, Actins, Thiazoles, chemistry, Biophysics, biology.protein, Thiazolidines, Latrunculin, Collagen

Abstract

In physiological conditions, collagen degradation by fibroblasts occurs primarily via phagocytosis, an intracellular pathway that is thought to require collagen receptors and actin assembly for fibril internalization and degradation. Currently it is unclear which specific steps of collagen phagocytosis in fibroblasts involve actin filament assembly. As studies of phagocytosis in fibroblasts are complicated by the relatively slow rate of particle internalization compared to professional phagocytes, we have examined the role of collagen receptors and actin only in the initial collagen binding step. Prior to the binding of collagen-coated fluorescent beads by human gingival fibroblasts, a cell type that is avidly phagocytic in vitro, cells were treated with cytochalasin D (actin filament barbed-end capping) or swinholide A (actin dimer sequestering and severing) or latrunculin B (actin monomer sequestering). Bead binding and immunostaining of (alpha)(2)(beta)(1) and (alpha)(3)(beta)(1) integrin collagen receptors were measured by flow cytometry. After 1–3 hours of coincubation with beads, cytochalasin D or swinholide A eliminated actin filaments stained by rhodamine-phalloidin and inhibited collagen bead binding (reductions of 25% and 50%, respectively), possibly because of cell rounding and restricted interactions with beads. In contrast, latrunculin enhanced binding dose-dependently over controls (twofold at 1 microM) and induced the formation of brightly staining aggregates of actin and the retention of long cytoplasmic extensions. Latrunculin also reduced surface (beta)(1), (alpha)(2) and (alpha)(3) integrin staining up to 40% in bead-free and bead-loaded cells, indicating that latrunculin enhanced collagen receptor internalization. As determined by fluorescence recovery after photobleaching, latrunculin increased the mobility of surface-bound (beta)(1) integrin. The stimulatory effect of latrunculin on collagen bead binding was reduced to control levels by treatment with a (beta)(1) integrin inactivating antibody while a (beta)(1) integrin blocking antibody abrogated both bead binding and the latrunculin-induced stimulation. Immunoblotting of bead-associated proteins showed that latrunculin completely eliminated binding of (beta)-actin to collagen beads but did not affect (beta)(1) integrin binding. These data indicate that latrunculin-induced sequestration of actin monomers facilitates the disengagement of actin from (beta)(1) integrin receptors, increases collagen bead binding and enhances collagen receptor mobility. We suggest that these alterations increase the probability of adhesive bead-to-cell interactions.

Published

2001

225. Requirement of cortical actin organization for bombesin, endothelin, and EGF receptor internalization

Author

John H. Walsh, Helen Wong, J. Adrian Lunn, and Enrique Rozengurt

Subjects

medicine.medical_specialty, Cytochalasin D, Physiology, media_common.quotation_subject, education, macromolecular substances, Biology, Iodine Radioisotopes, Mice, chemistry.chemical_compound, Growth factor receptor, GTP-Binding Proteins, Epidermal growth factor, 1-(5-Isoquinolinesulfonyl)-2-Methylpiperazine, Gastrin-releasing peptide, Internal medicine, medicine, Animals, Enzyme Inhibitors, Phosphorylation, Internalization, Nucleic Acid Synthesis Inhibitors, media_common, Dose-Response Relationship, Drug, Epidermal Growth Factor, Receptors, Endothelin, Bombesin, 3T3 Cells, Cell Biology, Bridged Bicyclo Compounds, Heterocyclic, Actins, Bombesin receptor, Cell biology, ErbB Receptors, Receptors, Bombesin, Kinetics, Thiazoles, Endocrinology, Gastrin-Releasing Peptide, chemistry, Thiazolidines, Latrunculin, Signal transduction, hormones, hormone substitutes, and hormone antagonists, Signal Transduction

Abstract

The role of actin organization in occupancy-induced receptor internalization remains poorly defined. Here we report that treatment of mouse Swiss 3T3 cells with latrunculin A, a potent inhibitor of actin polymerization (including cortical actin), inhibited the internalization of the endogenous bombesin/gastrin-releasing peptide (GRP) receptor, as judged by uptake of125I-labeled GRP or fluorescent Cy3-labeled bombesin. In contrast, cells pretreated with cytochalasin D showed minimal inhibition of bombesin/GRP receptor internalization. Similarly, pretreatment of Swiss 3T3 cells with the potent Rho-kinase inhibitor HA-1077, at concentrations (10–20 μM) that abrogated bombesin-mediated stress fiber formation, did not significantly alter receptor-mediated internalization of125I-GRP. These results indicate that bombesin/GRP receptor internalization depends on latrunculin A-sensitive cortical actin rather than on rapidly turning over actin stress fibers that are disrupted by either cytochalasin D or HA-1077. The rates and total levels of internalization of the endogenously expressed endothelin A receptor and epidermal growth factor receptor were also markedly reduced by latrunculin A in Swiss 3T3 cells. The potency of latrunculin A for inhibiting G protein-coupled receptor endocytosis was comparable to that for reducing internalization of the epidermal growth factor tyrosine kinase receptor. We conclude that cortical actin structures, disrupted by latrunculin A, are necessary for occupancy-induced receptor internalization in animal cells.

Published

2000

226. The Actin-Driven Movement and Formation of Acetylcholine Receptor Clusters

Author

Xiaoyan Luo, Zhengshan Dai, H. Benjamin Peng, and Hongbo Xie

Subjects

Polymers, Xenopus, Gene Expression, Arp2/3 complex, Synaptic Transmission, jasplakinolide, Actin remodeling of neurons, chemistry.chemical_compound, Sarcolemma, 0302 clinical medicine, Genes, Reporter, Depsipeptides, Receptors, Cholinergic, Cells, Cultured, 0303 health sciences, Agrin, biology, Muscles, Microfilament Proteins, Microspheres, Thiazolidines, Original Article, Cortactin, actin, animal structures, Phalloidin, Green Fluorescent Proteins, Neuromuscular Junction, Antineoplastic Agents, macromolecular substances, Peptides, Cyclic, latrunculin, 03 medical and health sciences, Animals, Actin-binding protein, Actin, 030304 developmental biology, acetylcholine receptor cluster, Cell Biology, Bridged Bicyclo Compounds, Heterocyclic, Actin cytoskeleton, Molecular biology, Actins, Luminescent Proteins, Thiazoles, chemistry, biology.protein, Biophysics, Indicators and Reagents, 030217 neurology & neurosurgery

Abstract

A new method was devised to visualize actin polymerization induced by postsynaptic differentiation signals in cultured muscle cells. This entails masking myofibrillar filamentous (F)-actin with jasplakinolide, a cell-permeant F-actin–binding toxin, before synaptogenic stimulation, and then probing new actin assembly with fluorescent phalloidin. With this procedure, actin polymerization associated with newly induced acetylcholine receptor (AChR) clustering by heparin-binding growth-associated molecule–coated beads and by agrin was observed. The beads induced local F-actin assembly that colocalized with AChR clusters at bead–muscle contacts, whereas both the actin cytoskeleton and AChR clusters induced by bath agrin application were diffuse. By expressing a green fluorescent protein–coupled version of cortactin, a protein that binds to active F-actin, the dynamic nature of the actin cytoskeleton associated with new AChR clusters was revealed. In fact, the motive force generated by actin polymerization propelled the entire bead-induced AChR cluster with its attached bead to move in the plane of the membrane. In addition, actin polymerization is also necessary for the formation of both bead and agrin-induced AChR clusters as well as phosphotyrosine accumulation, as shown by their blockage by latrunculin A, a toxin that sequesters globular (G)-actin and prevents F-actin assembly. These results show that actin polymerization induced by synaptogenic signals is necessary for the movement and formation of AChR clusters and implicate a role of F-actin as a postsynaptic scaffold for the assembly of structural and signaling molecules in neuromuscular junction formation.

Published

2000

227. Actin-Dependent Regulation of Neurotransmitter Release at Central Synapses

Author

Michael A. Colicos, Yukiko Goda, and Miguel Morales

Subjects

Cytochalasin D, Recombinant Fusion Proteins, Neuroscience(all), Green Fluorescent Proteins, Presynaptic Terminals, Fluorescent Antibody Technique, Nerve Tissue Proteins, macromolecular substances, Biology, Hippocampus, Peptides, Cyclic, Synaptic Transmission, Synaptic vesicle, Exocytosis, Mice, chemistry.chemical_compound, Depsipeptides, Animals, Cytochalasin, Active zone, Neurotransmitter, Egtazic Acid, Cells, Cultured, Neurotransmitter Agents, General Neuroscience, Vesicle, Excitatory Postsynaptic Potentials, Bridged Bicyclo Compounds, Heterocyclic, Actins, Rats, Cell biology, Luminescent Proteins, Thiazoles, chemistry, Cerebellar cortex, Synapses, Thiazolidines, Latrunculin, Calcium, Marine Toxins, Synaptic Vesicles

Abstract

Depolymerization of actin by latrunculin A transiently promotes neurotransmitter release. The mean rate of mEPSCs increases by a Ca2+-independent process, without a concomitant change in the mean amplitude. The readily releasable vesicle pool size and the rate of refilling of the readily releasable pool remain unaltered by latrunculin treatment. Evoked neurotransmitter release also increases in a manner consistent with an increase in vesicle release probability. The observed enhancement of neurotransmitter release is specific to actin depolymerization mediated by latrunculin A and is not caused by cytochalasin D. Our findings indicate that actin participates in a regulatory mechanism that restrains fusion of synaptic vesicles at the active zone.

Published

2000

228. Actin-Latrunculin A Structure and Function

Author

Ilan Spector, Elena G. Yarmola, Thayumanasamy Somasundaram, Todd A. Boring, and Michael R. Bubb

Subjects

Actin remodeling, Arp2/3 complex, macromolecular substances, Cell Biology, Biology, Biochemistry, Profilin, polycyclic compounds, biology.protein, Biophysics, Latrunculin, MDia1, Actin-binding protein, Binding site, Molecular Biology, Actin

Abstract

Latrunculin A is used extensively as an agent to sequester monomeric actin in living cells. We hypothesize that additional activities of latrunculin A may be important for its biological activity. Our data are consistent with the formation of a 1:1 stoichiometric complex with an equilibrium dissociation constant of 0.2 to 0.4 micrometer and provide no evidence that the actin-latrunculin A complex participates in the elongation of actin filaments. Profilin and latrunculin A bind independently to actin, whereas binding of thymosin beta(4) to actin is inhibited by latrunculin A. Potential implications of this differential effect on actin-binding proteins are discussed. From a structural perspective, if latrunculin A binds to actin at a site that sterically influences binding by thymosin beta(4), then the observation that latrunculin A inhibits nucleotide exchange on actin implies an allosteric effect on the nucleotide binding cleft. Alternatively, if, as previously postulated, latrunculin A binds in the nucleotide cleft of actin, then its ability to inhibit binding by thymosin beta(4) is a surprising result that suggests that significant allosteric changes affect the thymosin beta(4) binding site. We show that latrunculin A and actin form a crystalline structure with orthorhombic space group P2(1)2(1)2(1) and diffraction to 3.10 A. A high resolution structure with optimized crystallization conditions should provide insight regarding these remarkable allosteric properties.

Published

2000

229. Hormone-stimulated calcium release is inhibited by cytoskeleton-disrupting toxins in AR4-2J cells

Author

Peter Feick, Irene Schulz, M. Bozem, Robert Blum, and S. Kuhlmann

Subjects

Cell Membrane Permeability, Cytochalasin D, Thapsigargin, Physiology, Bacterial Toxins, Clostridium difficile toxin B, Inositol 1,4,5-Trisphosphate, macromolecular substances, Biology, Fluorides, chemistry.chemical_compound, Cytosol, Bacterial Proteins, GTP-Binding Proteins, Tumor Cells, Cultured, Animals, Aluminum Compounds, Cytoskeleton, Pancreas, Molecular Biology, Cell Biology, Bridged Bicyclo Compounds, Heterocyclic, Actin cytoskeleton, Hormones, Rats, Bombesin receptor, Cell biology, Pancreatic Neoplasms, Thiazoles, chemistry, Type C Phospholipases, Thiazolidines, Latrunculin, Bombesin, Calcium, Intracellular

Abstract

We have studied the role of the actin cytoskeleton in bombesin-induced inositol 1,4,5-trisphosphate (IP(3))-production and Ca(2+)release in the pancreatic acinar tumour cell line AR4-2J. Intracellular and extracellular free Ca(2+)concentrations were measured in cell suspensions, using Fura-2. Disruption of the actin cytoskeleton by pretreatment of the cells with latrunculin B (10 microM), cytochalasin D (10 microM) or toxin B from Clostridium difficile (20 ng/ml) for 5-29 h led to inhibition of both, bombesin-stimulated IP(3)-production and Ca(2+)release. The toxins had no effect on binding of bombesin to its receptor, on Ca(2+)uptake into intracellular stores and on resting Ca(2+)levels. Ca(2+)mobilization from intracellular stores, induced by thapsigargin (100 nM) or IP(3)(1 microM) was not impaired by latrunculin B. In latrunculin B-pretreated cells inhibition of both, bombesin-stimulated IP(3)- production and Ca(2+)release was partly suspended in the presence of aluminum fluoride, an activator of G-proteins. Aluminum fluoride had no effect on basal IP(3)and Ca(2+)levels of control and toxin-pretreated cells. We conclude that disruption of the actin cytoskeleton impairs coupling of the bombesin receptor to its G-protein, resulting in inhibition of phospholipase C-activity with subsequent decreases in IP(3)-production and Ca(2+)release.

Published

2000

230. Disruption of actin impedes transmitter release in snake motor terminals

Author

Brian R. Villa, Robert S. Wilkinson, and John C. Cole

Subjects

Physiology, Presynaptic Terminals, Pyridinium Compounds, macromolecular substances, Biology, Synaptic Transmission, Muscle nerve, Animals, Incubation, Actin, Fluorescent Dyes, Motor Neurons, Rapid Report, Dose-Response Relationship, Drug, Vesicle, Colubridae, Anatomy, Bridged Bicyclo Compounds, Heterocyclic, Actins, Endocytosis, Electrophysiology, Quaternary Ammonium Compounds, Thiazoles, Time course, Biophysics, Thiazolidines, Latrunculin, Synaptic Vesicles, Tetanic stimulation, Immunostaining

Abstract

To investigate the role of actin in vertebrate nerve terminals, nerve-muscle preparations from garter snake (Thamnophis sirtalis) were treated with the actin-depolymerizing agent latrunculin A. Immunostaining revealed that actin filaments within presynaptic motor terminal boutons were disrupted by the drug. In preparations loaded with the optical probe FM1-43, destaining was reduced by latrunculin treatment, suggesting that transmitter release was partially blocked. Latrunculin treatment did not influence the amplitude or time course of spontaneous miniature endplate potentials (MEPPs). Similarly, endplate potentials (EPPs) evoked at low frequency were comparable in control and latrunculin-treated curarized preparations. Brief tetanic stimulation of the muscle nerve (25 Hz, 90 s) depressed EPP amplitudes in both control and latrunculin-treated preparations. After tetanus, EPPs elicited at 0. 2 Hz in control preparations recovered rapidly (0-5 min) and completely (usually potentiating to above pre-tetanus levels; 130 +/- 11 %, mean +/- s.e.m.). In contrast, EPPs evoked in latrunculin-treated preparations recovered slowly (8-10 min) and incompletely (84 +/- 8 %). The influence of latrunculin on post-tetanic EPPs depended on its concentration in the bath (KD = 3. 1 microM) and on time of incubation. These observations argue that actin filaments facilitate transmitter release rather than impede it. Specifically, actin may facilitate mobilization of vesicles towards the releasable pools.

Published

2000

231. Evidence for direct membrane retrieval following cortical granule exocytosis inXenopus oocytes and eggs

Author

William M. Bement, Craig A. Mandato, Hélène A. Benink, and Brad B. Swelstad

Subjects

Endosome, Cortical granule exocytosis, Xenopus, Cortical granule, Latrunculin, Animal Science and Zoology, General Medicine, Biology, Endocytosis, biology.organism_classification, Actin cytoskeleton, Exocytosis, Cell biology

Abstract

Rapid exocytosis is typically followed by rapid resorption of exocytosed membrane; however, whether membrane retrieval occurs via indirect endocytosis of numerous small vesicles or direct resealing of the original, larger exocytotic vesicles is controversial. Here we show that cortical granule (CG) exocytosis in Xenopus oocytes and eggs is followed by rapid formation of endosomes as large as the CGs. Large endosomes are translucent, and their formation has the same developmental and pharmacological profile as CG exocytosis. Time course analyses show that large endosomes are not derived from small endosomes. Large endosome formation is trig- gered by stimuli that do not trigger increases in intracellular-free calcium and is insensitive to perturbation of microtubules by treatment with nocodazole. Perturbation of the f-actin cytoskel- eton with latrunculin, however, sharply reduces large endosome formation. We conclude that CG membrane is directly retrieved in Xenopus oocytes and eggs and suggest that this retrieval is not directly dependent on an increase in intracellular-free calcium, but is dependent on the actin cytoskeleton. J. Exp. Zool. 286:767-775, 2000. © 2000 Wiley-Liss, Inc.

Published

2000

232. Insulin-induced actin filament remodeling colocalizes actin with phosphatidylinositol 3-kinase and GLUT4 in L6 myotubes

Author

Amira Klip, Peter Tong, Karen Yaworsky, Zayna A. Khayat, and Robert J. Bloch

Subjects

Monosaccharide Transport Proteins, Biological Transport, Active, Muscle Proteins, Arp2/3 complex, macromolecular substances, Biology, Models, Biological, Cell Line, Phosphatidylinositol 3-Kinases, chemistry.chemical_compound, Actin remodeling of neurons, Animals, Insulin, Cytoskeleton, Actin, Cytochalasin D, Organelles, Glucose Transporter Type 4, Muscles, Cell Membrane, Actin remodeling, Cell Biology, Actins, Rats, rac GTP-Binding Proteins, Cell biology, chemistry, biology.protein, Latrunculin, MDia1, GLUT4

Abstract

We examined the temporal reorganization of actin microfilaments by insulin and its participation in the localization of signaling molecules and glucose transporters in L6 myotubes expressing myc-tagged glucose transporter 4 (GLUT4myc). Scanning electron microscopy revealed a dynamic distortion of the dorsal cell surface (membrane ruffles) upon insulin treatment. In unstimulated cells, phalloidin-labeled actin filaments ran parallel to the longitudinal axis of the cell. Immunostaining of the p85 regulatory subunit of phosphatidylinositol 3-kinase was diffusely punctate, and GLUT4myc was perinuclear. After 3 minutes of insulin treatment, actin reorganized to form structures; these structures protruded from the dorsal surface of the myotubes by 10 minutes and condensed in the myoplasm into less prominent foci at 30 minutes. The p85 polypeptide colocalized with these structures at all time points. Actin remodeling and p85 relocalization to actin structures were prevented by cytochalasin D or latrunculin B. GLUT4myc recruitment into the actin-rich projections was also observed, but only after 10 minutes of insulin treatment. Irrespective of insulin stimulation, the majority of p85 and a portion (45%) of GLUT4 were recovered in the Triton X-100-insoluble material that was also enriched with actin. In contrast, vp165, a transmembrane aminopeptidase that morphologically colocalized with GLUT4 vesicles, was fully soluble in Triton X-100 extracts of both insulin-treated and control myotubes. Transient transfection of dominant inhibitory Rac1 (N17) into L6 myotubes prevented formation of dorsal actin structures and blocked insulin-induced GLUT4myc translocation to the cell surface. We propose that insulin-dependent formation of actin structures facilitates the association of PI3-K (p85) with GLUT4 vesicles and, potentially, the arrival of GLUT4 at the cell surface.

Published

2000

233. Effects of latrunculin reveal requirements for the actin cytoskeleton during secretion from mast cells

Author

A. Pendleton and A. Koffer

Subjects

chemistry.chemical_element, macromolecular substances, Cell Biology, Biology, Calcium, Actin cytoskeleton, Exocytosis, Cell biology, chemistry, Structural Biology, Latrunculin, Secretion, Cytoskeleton, Marine toxin, Actin

Abstract

To investigate the role of the actin cytoskeleton in exocytosis, we have tested the effects of latrunculin B, a microfilament-disrupting drug, on secretion from intact and permeabilised rat peritoneal mast cells. The toxin strongly inhibited secretion from intact cells (attached or in suspension) responding to a polybasic agonist, compound 48/80. However, this effect was revealed only after a profound depletion of actin filaments. This was achieved by a long (1 h) exposure of cells to the drug before activation, together with its presence during activation. Maximal inhibition of secretion by such treatment was 85% at 40 microgram/ml latrunculin B. These results indicate that minimal actin structures are essential for the exocytotic response. In contrast, stimulus-induced cell spreading was prevented by latrunculin (5 microgram/ml) applied either before or after activation. The effects of the toxin on intact cells were fully reversible. The responses of permeabilised cells were affected differentially: secretion induced by calcium was more sensitive to latrunculin than that induced by GTP-gamma-S. The calcium response, therefore, is more dependent upon the integrity of the actin cytoskeleton than the response induced by GTP-gamma-S. Again, maximal inhibitory effects (approximately 65 and 25% at 40 microgram/ml) were observed only when cells were exposed to the toxin both before and after permeabilisation. Since the permeabilised cells system focuses on the final steps of exocytosis, the incomplete inhibition suggests that actin plays a modulatory rather than a central role at this stage.

Published

2000

234. Physode formation in embryos of Phyllospora comosa and Hormosira banksii (Phaeophyceae)

Author

Margaret N. Clayton and Monica E. A. Schoenwaelder

Subjects

Phyllospora comosa, Endoplasmic reticulum, Hormosira, Plant Science, Aquatic Science, Biology, Golgi apparatus, biology.organism_classification, chemistry.chemical_compound, symbols.namesake, Rhizoid, chemistry, Cytoplasm, Botany, symbols, Latrunculin, Cytochalasin

Abstract

Phenolic compounds, packaged within vesicles known as physodes, are a major cytoplasmic constituent of eggs and zygotes of the Australasian fucoids Hormosira banksii (Turner) Decaisne and Phyllospora comosa (Labillardiere) C Agardh. Light and transmission electron microscopy in conjunction with the actin inhibitors cytochalasin and latrunculin and the Golgi disruptor Brefeldin were used to investigate physode biogenesis in Hormosira and Phyllospora zygotes and embryos. Our results show that physodes are formed in the perinuclear region of the cell. Contrary to many early reports, no evidence was found that physode genesis is associated with chloroplasts. Instead, the Golgi apparatus and the endoplasmic reticulum are implicated in physode formation. Physodes are produced in large quantities around the nucleus just before periods of active wall deposition, particularly during rhizoid initiation and crosswall formation. Subsequently, they move from their central location to the sites of wall deposition.

Published

2000

235. Melanosome and erythrosome positioning regulates cAMP-induced movement in chromatophores from spotted triplefin,Grahamina capito

Author

Helén Nilsson

Subjects

Forskolin, General Medicine, Biology, Actin cytoskeleton, Chromatophore, Cell biology, chemistry.chemical_compound, chemistry, Organelle, Latrunculin, Animal Science and Zoology, Actin, Intracellular, Melanosome

Abstract

This study investigated regulation of uniform positioning of melanosomes and erythrosomes in chromatophores from spotted triplefin Grahamina capito from New Zealand, by modulating levels of intracellular cAMP. Elevated cAMP levels, caused by forskolin treatment, in- hibited aggregation and induced rapid dispersion of melanosomes and erythrosomes. The dispersing organelles moved to and accumulated at the cell periphery, leading to an abnormal hyperdispersed state with a melanosome- or erythrosome-depleted cell center. Minutes after hyperdispersion, these organelles reversed direction and moved towards the center again to finally distribute throughout the cells. When chromatophores with initially dispersed melanosomes or erythrosomes were treated with forskolin, no hyperdispersion was seen, but the erythrosomes aggregated slowly. Disassembly of actin by latrunculin resulted in a similar but constant hyperdispersed melanosome and erythrosome distribution. The results show that cAMP not only disperses but also aggregates melanosomes and erythrosomes, and that it is the intracellular position of these organelles that determine the direc- tionality of the cAMP-induced movement. To ascertain the even distribution in the dispersed state, regulatory components associated with the actin cytoskeleton in the cell periphery might modify activity of cytoplasmic dynein or kinesin upon contact with dispersing melanosomes or erythrosomes. J. Exp. Zool. 287:191-198, 2000. © 2000 Wiley-Liss, Inc.

Published

2000

236. New anti-actin drugs in the study of the organization and function of the actin cytoskeleton

Author

Ilan Spector, Nava R. Shochet, Michael R. Bubb, and Filip Braet

Subjects

Histology, Swinholide A, Cell, Actin remodeling, macromolecular substances, Biology, Actin cytoskeleton, Pectenotoxin II, Cell biology, Medical Laboratory Technology, medicine.anatomical_structure, medicine, Latrunculin, Anatomy, Cytoskeleton, Instrumentation, Actin

Abstract

The high degree of structural and molecular complexity of the actin-based cytoskeleton, combined with its ability to reorganize rapidly and locally in response to stimuli, and its force-generating properties, have made it difficult to assess how the different actin structures are assembled in cells, and how they regulate cell behavior. An obvious approach to study the relationships between actin organization, dynamics, and functions is the specific perturbation of actin structures using pharmacological means. Until recently there were only a few agents available that interfered with cellular activities by binding to actin and most of our knowledge concerning the involvement of actin in basic cellular processes was based on the extensive use of the cytochalasins. In recent years we have identified an increasing number of actin-targeted marine natural products, including the latrunculins, jasplakinolides (jaspamides), swinholide A, misakinolide A, halichondramides, and pectenotoxin II, which are discussed in this article. All these marine-sponge-derived compounds are unusual macrolides and can be classified into several major families, each with its own distinct chemical structures. We describe the current state of knowledge concerning the actin-binding properties of these compounds and show that each class of drugs alters the distribution patterns of actin in a unique way, and that even within a chemical class, structurally similar compounds can have different biochemical properties and cellular effects. We also discuss the effects of these new drugs on fenestrae formation in liver endothelial cells as an example of their usefulness as powerful tools to selectively unmask actin-mediated dynamic processes.

Published

1999

237. The Platelet Cytoskeleton Regulates the Affinity of the Integrin αIIbβ3 for Fibrinogen

Author

Gaston Vilaire, Bohumil Bednar, Sally H. Zigmond, Michael E. Cunningham, and Joel S. Bennett

Subjects

Blood Platelets, Fibrinogen, Fibrinogen binding, Actin remodeling, Platelet Glycoprotein GPIIb-IIIa Complex, macromolecular substances, Cell Biology, Cofilin, Biology, Actin cytoskeleton, Biochemistry, Actins, Cell biology, chemistry.chemical_compound, chemistry, biology.protein, Humans, Latrunculin, Cytochalasin, Actin-binding protein, Molecular Biology, Cytoskeleton, Cytochalasin D

Abstract

Agonist-generated inside-out signals enable the platelet integrin alpha(IIb)beta(3) to bind soluble ligands such as fibrinogen. We found that inhibiting actin polymerization in unstimulated platelets with cytochalasin D or latrunculin A mimics the effects of platelet agonists by inducing fibrinogen binding to alpha(IIb)beta(3). By contrast, stabilizing actin filaments with jasplakinolide prevented cytochalasin D-, latrunculin A-, and ADP-induced fibrinogen binding. Cytochalasin D- and latrunculin A-induced fibrinogen was inhibited by ADP scavengers, suggesting that subthreshold concentrations of ADP provided the stimulus for the actin filament turnover required to see cytochalasin D and latrunculin A effects. Gelsolin, which severs actin filaments, is activated by calcium, whereas the actin disassembly factor cofilin is inhibited by serine phosphorylation. Consistent with a role for these factors in regulating alpha(IIb)beta(3) function, cytochalasin D- and latrunculin A-induced fibrinogen binding was inhibited by the intracellular calcium chelators 1,2-bis(2-aminophenoxy)ethane-N,N,N', N'-tetraacetic acid acetoxymethyl ester and EGTA acetoxymethyl ester and the Ser/Thr phosphatase inhibitors okadaic acid and calyculin A. Our results suggest that the actin cytoskeleton in unstimulated platelets constrains alpha(IIb)beta(3) in a low affinity state. We propose that agonist-stimulated increases in platelet cytosolic calcium initiate actin filament turnover. Increased actin filament turnover then relieves cytoskeletal constraints on alpha(IIb)beta(3), allowing it to assume the high affinity conformation required for soluble ligand binding.

Published

1999

238. Diatom gliding is the result of an actin-myosin motility system

Author

Ilan Spector, Thomas F. Schultz, Richard Wetherbee, Nicole Poulsen, and Timothy P. Spurck

Subjects

Gliding motility, fungi, Motility, macromolecular substances, Cell Biology, Biology, Actin cytoskeleton, Cell biology, chemistry.chemical_compound, Nocodazole, chemistry, Structural Biology, Myosin, Latrunculin, Cytochalasin, Actin

Abstract

Diatoms are a group of unicellular microalgae that are encased in a highly ornamented siliceous cell wall, or frustule. Pennate diatoms have bilateral symmetry and many genera possess an elongated slit in the frustule called the raphe, a feature synonymous with their ability to adhere and glide over a substratum, a process little understood. We have used cytoskeleton-disrupting drugs to investigate the roles of actin, myosin, and microtubules in diatom gliding or motility. No effect on diatom gliding was observed using the cytochalasins, known actin inhibitors, or the microtubule-inhibitors oryzalin and nocodazole. The latrunculins are a new group of anti-actin drugs, and we show here that they are potent inhibitors of diatom gliding, resulting in the complete disassociation of the raphe-associated actin cables. The recovery of actin staining and motility following latrunculin treatment was extremely fast. Cells exposed to latrunculin for 12 h recovered full function and actin staining within 5 sec of the drug being removed, demonstrating that the molecular components required for this motility system are immediately available. Butanedione monoxime (BDM), a known myosin inhibitor, also reversibly inhibited diatom gliding in a manner similar to the latrunculins. This work provides evidence that diatom gliding is based on an actin/myosin motility system.

Published

1999

239. New actin mutants allow further characterization of the nucleotide binding cleft and drug binding sites

Author

Lisa D. Belmont, David G. Drubin, and G. M. L. Patterson

Subjects

Models, Molecular, Phalloidin, Receptors, Drug, Genes, Fungal, Arp2/3 complex, Saccharomyces cerevisiae, macromolecular substances, Biology, chemistry.chemical_compound, Adenosine Triphosphate, Actin-binding protein, Binding site, Cells, Cultured, Actin, Pyrans, Nucleotides, Actin remodeling, Cell Biology, Bridged Bicyclo Compounds, Heterocyclic, Actins, Endocytosis, Cell biology, Thiazoles, Phenotype, chemistry, Biochemistry, Mutagenesis, Site-Directed, biology.protein, Thiazolidines, Latrunculin, MDia1

Abstract

We have generated 9 site-specific mutations in Saccharomyces cerevisiae actin. These mutants display a variety of phenotypes when expressed in vivo, including slow actin filament turnover, slow fluid-phase endocytosis, and defects in actin organization. Actin mutation D157E confers resistance to the actin-sequestering drug, latrunculin A. Latrunculin A inhibits nucleotide exchange on wild-type yeast actin but not on D157E actin, suggesting that this residue is part of the latrunculin A binding site. We have refined our earlier map of the phalloidin binding site on actin, demonstrating a requirement for residue G158 in addition to D179 and R177. The nine new actin mutants as well as a large collection of existing actin mutants were also used to identify the putative binding site of another actin binding drug, tolytoxin, on actin. The actin alleles that result in decreased sensitivity to this drug cluster at a site near the nucleotide-binding pocket. Actin purified from one of these mutants has a reduced affinity for tolytoxin. In addition, tolytoxin causes a 2.4-fold increase in the t1/2 of ATP exchange, further suggesting that this drug binds near the nucleotide-binding pocket of actin. We note that the binding sites for latrunculin A, phalloidin, and tolytoxin all map close to the actin nucleotide binding pocket.

Published

1999

240. Effects of rhizopodin and latrunculin B on the morphology and on the actin cytoskeleton of mammalian cells

Author

Hans Reichenbach, Florenz Sasse, Heinrich Lünsdorf, and Thomas M. A. Gronewold

Subjects

Histology, PTK2, Fluorescent Antibody Technique, Antineoplastic Agents, macromolecular substances, Biology, Kidney, Cell morphology, Cell Line, Pathology and Forensic Medicine, Mice, Multinucleate, medicine, Animals, Oxazoles, Cytoskeleton, Protein kinase C, Cell Biology, Fibroblasts, Bridged Bicyclo Compounds, Heterocyclic, Actin cytoskeleton, Actins, Cell biology, Microscopy, Electron, Thiazoles, medicine.anatomical_structure, Cell culture, Thiazolidines, Latrunculin, Macrolides

Abstract

The effects of the novel myxobacterial compound rhizopodin on mammalian cells were studied and compared with those of latrunculin B. Both substances induced adherently growing L929 mouse fibroblasts and PtK2 potoroo kidney cells to produce long, narrow, branched extensions or runners. Rhizopodin was more efficient than latrunculin B in that respect (minimal inhibitory concentration with L929 cells 5 nM vs 50 nM), and, in contrast to latrunculin B, its effects were permanent. Rhizopodin-treated cells became much larger than normal cells and were multinucleate, yet stayed alive and biochemically active for several weeks. Latrunculin B-treated cells returned to a quasi-normal state within 3-4 days. But latrunculin B acted faster, with the first effects becoming visible almost immediately upon the addition of the drug, while the first rhizopodin effects were seen 10 min later. Both substances caused reorganization of the actin cytoskeleton. When 100 nM rhizopodin was added to PtK2 cells, the stress fibers began to decay after just 10 min and had disappeared completely after about 3 h. Later there was a gradual restitution of F-actin. Long F-actin fibers were seen within the runners, and only there; in fact, these fibers may be responsible for the development and extension of the runners. The microtubuli network adjusted itself to the new cell morphology, but was not directly impaired by the compound.

Published

1999

241. Microtubules, but not actin microfilaments, regulate vacuole motility and morphology in hyphae ofPisolithus tinctorius

Author

Danielle Davies, Louise Cole, G. J. Hyde, Anne E. Ashford, and Lara Perasso

Subjects

Cell Biology, Vacuole, Biology, Microfilament, Cell biology, Nocodazole, chemistry.chemical_compound, chemistry, Structural Biology, Microtubule, Ultrastructure, Latrunculin, Endomembrane system, Cytoskeleton

Abstract

While it is now recognised that transport within the endomembrane system may occur via membranous tubules, spatial regulation of this process is poorly understood. We have investigated the role of the cytoskeleton in regulating the motility and morphology of the motile vacuole system in hyphae of the fungus Pisolithus tinctorius by studying (1) the effects of anti-microtubule (oryzalin, nocodazole) and anti-actin drugs (cytochalasins, latrunculin) on vacuolar activity, monitored by fluorescence microscopy of living cells; and (2) the ultrastructural relationship of microtubules, actin microfilaments, and vacuoles in hyphae prepared by rapid-freezing and freeze-substitution. Anti-microtubule drugs reduced the tubular component of the vacuole system in a dose-dependent and reversible manner, the extent of which correlated strongly with the degree of disruption of the microtubule network (monitored by immunofluorescence microscopy). The highest doses of anti-microtubule drugs completely eliminated tubular vacuoles, and only spherical vacuoles were observed. In contrast, anti-actin drugs did not reduce the frequency of tubular vacuoles or the motility of these vacuoles, even though immunofluorescence microscopy confirmed perturbation of microfilament organisation. Electron microscopy showed that vacuoles were always accompanied by microtubules. Bundles of microtubules were found running in parallel along the length of tubular vacuoles and individual microtubules were often within one microtubule diameter of a vacuole membrane. Our results strongly support a role for microtubules, but not actin microfilaments, in the spatial regulation of vacuole motility and morphology in fungal hyphae. Cell Motil. Cytoskeleton 42:114–124, 1999. © 1999 Wiley-Liss, Inc.

Published

1999

242. Structure and dynamics of actin filament solutions in the presence of latrunculin A

Author

Boyoung Cha, Andre F. Palmer, and Denis Wirtz

Subjects

chemistry.chemical_classification, Diffusing-wave spectroscopy, Polymers and Plastics, macromolecular substances, Polymer, Condensed Matter Physics, Filamentous actin, Viscoelasticity, Protein filament, chemistry, Polymer chemistry, polycyclic compounds, Materials Chemistry, Biophysics, Latrunculin, Physical and Theoretical Chemistry, Elasticity (economics), Actin

Abstract

We study the polymerization kinetics and linear rheology of actin filaments in the absence and in the presence of latrunculin A. Filamentous actin is a semiflexible polymer, and latrunculin A is an organic, actin-binding molecule. Using diffusing wave spectroscopy (DWS), we monitor the thermally excited motion of monodisperse polystyrene microspheres in semidilute solutions of actin filaments. From these measurements, we extract the microspheres mean-square displacement, which is related to the viscoelastic nature of the actin solutions. These optical measurements, along with mechanical measurements, suggest that despite its depolymerizing effect, latrunculin A promotes the strengthening of actin networks. DWS shows that while the scaling nature of the viscoelastic properties of actin filaments is essentially unmodified in the presence of latrunculin A at small time scales, the elasticity of actin solutions becomes enhanced for increasing latrunculin concentrations at large time scales. Complementary electron-microscopy measurements help uncover the structural origin of this enhanced elasticity at small time scales.

Published

1998

243. Keratins significantly contribute to cell stiffness and impact invasive behavior

Author

Anatol Fritsch, Thomas M. Magin, Josef A. Käs, and Kristin Seltmann

Subjects

Epithelial-Mesenchymal Transition, Indoles, Cell, Biophysics, Motility, Fluorescent Antibody Technique, macromolecular substances, Matrix (biology), Colony-Forming Units Assay, Mice, Downregulation and upregulation, Cell Movement, Keratin, medicine, Animals, Neoplasm Invasiveness, Epithelial–mesenchymal transition, Cytoskeleton, Cell Shape, Skin, chemistry.chemical_classification, Multidisciplinary, biology, integumentary system, Vinculin, Biological Sciences, Cell biology, Biomechanical Phenomena, medicine.anatomical_structure, chemistry, biology.protein, Latrunculin, Keratins, Wound healing, Genetic Engineering

Abstract

Cell motility and cell shape adaptations are crucial during wound healing, inflammation and malignant progression. These processes require the remodeling of the keratin cytoskeleton, to facilitate cell-cell and matrix adhesion. However, the role of keratins for biomechanical properties and invasion of epithelial cells are only partially understood. Here, we address this issue in murine keratinocytes lacking all keratins upon genome engineering. In contrast to prediction, keratin-free cells show an about 60% higher cell deformability even for small deformations. This is compared to less pronounced softening effects for actin depolymerization induced via latrunculin A. To relate these findings with functional consequences, we use invasion and three-dimensional growth assays. These reveal higher invasiveness of keratin-free cells. Re-expression of a small amount of the keratin pair K5/K14 in keratin-free cells reverses the above phenotype for the invasion but does not with respect to cell deformability. Our data shows a novel role of keratins as major player of cell stiffness influencing invasion with implications for epidermal homeostasis and pathogenesis. This study supports the view that downregulation of keratins observed during epithelial-mesenchymal transition directly contributes to the migratory and invasive behavior of tumor cells. (see K. Seltmann et al., PNAS, in press).

Published

2013

244. The effects of actomyosin inhibitors on cytoskeletal distributions in the lens

Author

G Won and V Choh

Subjects

Myosin light-chain kinase, Confocal, macromolecular substances, General Medicine, Anatomy, Biology, law.invention, Ophthalmology, Confocal microscopy, law, Myosin, Ultrastructure, Biophysics, Latrunculin, Cytoskeleton, Actin

Abstract

Purpose Previous work indicates that inhibitors of actin, myosin, and myosin light chain kinase are associated with a softening of the lens. The softening of lenses did not affect the optical quality, despite the application of inhibitors that, based on Western blot analysis, affect the cytoskeleton of lens fibre cells. Inhibitors can impart their effects biochemically or structurally, therefore, in the present study, the cytoskeletal distribution of inhibitor-treated lenses was examined using confocal microscopy. Methods Lenses of 7-day-old White Leghorn chickens were treated (15 mins) with 10 µM of either a vehicle (dimethyl sulfoxide) or an inhibitor (1-(5-iodonaphthalene-1-sulfonyl)-1H-hexahydro-1,4-diazepine hydrochloride [ML-7], a myosin light chain kinase inhibitor; 1-phenyl-1,2,3,4-tetrahydro-4-hydroxypyrrolo[2.3-b]-7-methylquinolin-4-one [blebbistatin], a myosin II inhibitor; latrunculin, an actin inhibitor). After treatment, lenses were incubated in antibodies against the appropriate cytoskeletal proteins, and mounted onto slides in toto for examination under confocal microscopy. Images taken from the confocal microscope were analyzed using nearest neighbour analysis for irregularity. Results Myosin distributions were highly regular, with a nearest neighbour value (Rn) of 2.02. Blebbistatin treatment resulted in a less regular arrangement (Rn=1.65), approaching a random distribution. Actin distributions in the latrunculin-treated lenses were disorganized, showing irregular spatial distributions between vertices (Rn=1.53) compared to those in vehicle treated lenses (Rn=1.91). Conclusion Inhibitors were shown to affect the distributions of actin and myosin, which indicates that these inhibitors impart their effects by altering cytoskeletal ultrastructure.

Published

2013

245. Organization and regulation of intracellular plasma membrane-connected HIV-1 assembly compartments in macrophages

Author

Petra Mlcochova, Annegret Pelchen-Matthews, and Mark Marsh

Subjects

Phosphatidylinositol 4,5-Diphosphate, Physiology, HIV Infections, MDM, Plant Science, Monocytes, Polymerization, Cell membrane, Phosphatidylinositol Phosphates, Structural Biology, Image Processing, Computer-Assisted, Coloring Agents, 0303 health sciences, Agricultural and Biological Sciences(all), Compartment, 030302 biochemistry & molecular biology, Actin cytoskeleton, Lipids, Cell biology, Pleckstrin homology domain, medicine.anatomical_structure, Thiazolidines, General Agricultural and Biological Sciences, Biotechnology, Fluorescence Recovery After Photobleaching, Research Article, Endosome, Cell Survival, Green Fluorescent Proteins, Biology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Live cell imaging, medicine, Humans, Ecology, Evolution, Behavior and Systematics, Actin, 030304 developmental biology, Biochemistry, Genetics and Molecular Biology(all), Macrophages, Virus Assembly, Cell Membrane, Fluorescence recovery after photobleaching, Cell Biology, Intracellular Membranes, Bridged Bicyclo Compounds, Heterocyclic, Actins, Cell Compartmentation, IPMC, HIV-1, Latrunculin, Developmental Biology

Abstract

Background In HIV-1-infected human monocyte-derived macrophages (MDMs), virus particles assemble primarily on intracellularly sequestered plasma membrane domains termed intracellular plasma membrane-connected compartments (IPMCs). Despite their clear role in virus formation, little is known of the organization, composition, dynamics or function of these compartments. Results We have used amphipathic membrane dyes to reveal the complex three-dimensional structure of IPMCs in whole MDMs and to visualize connections between IPMCs and the cell surface. The observation of similar IPMC structures in both infected and uninfected cells indicates that these compartments are not induced by virus infection, but are present constitutively in MDMs. By expressing a phospholipase Cδ pleckstrin homology domain linked to green fluorescent protein, we demonstrate that IPMCs contain phosphatidylinositol 4,5-bisphosphate. Live cell imaging of cells expressing this probe shows that IPMCs are dynamic, but relatively stable, sub-domains of the plasma membrane. As recent electron microscopy studies indicated that portions of IPMCs are coated with β2 integrin-containing focal adhesion-like complexes linked to actin, we investigated whether the actin cytoskeleton is required for the organization of IPMCs. In MDMs treated with the actin polymerization inhibitor latrunculin, the normally compact IPMCs dispersed into smaller structures that remained connected to the plasma membrane. Moreover, latrunculin enhanced the release of preformed, mature HIV-1 particles from infected MDMs. Conclusions IPMCs are constitutive features of MDMs that are continuous with the plasma membrane and are used as unique sites for the assembly of new virions following infection by HIV-1. A functionally intact actin cytoskeleton is required to maintain the organization of the IPMCs and, in HIV-1-infected cells, perturbation of the actin cytoskeleton influences both the organization of the compartment and the release of sequestered virus.

Published

2013

246. A new F-actin structure in fungi: actin ring formation around the cell nucleus of Cryptococcus neoformans

Author

Masashi Yamaguchi, Marie Kopecká, and Susumu Kawamoto

Subjects

Phalloidine, macromolecular substances, 02 engineering and technology, Microtubules, YEPD, 03 medical and health sciences, chemistry.chemical_compound, Structural Biology, medicine, Radiology, Nuclear Medicine and imaging, Dimethyl Sulfoxide, Cytoskeleton, Instrumentation, Actin, 030304 developmental biology, Cryptococcus neoformans, Cell Nucleus, 0303 health sciences, biology, Rhodamines, Nocodazole, Free Radical Scavengers, 021001 nanoscience & nanotechnology, biology.organism_classification, Bridged Bicyclo Compounds, Heterocyclic, Actins, Tubulin Modulators, 3. Good health, Actin Cytoskeleton, Microscopy, Electron, medicine.anatomical_structure, chemistry, Biochemistry, Microscopy, Fluorescence, Biophysics, Latrunculin, Thiazolidines, Marine Toxins, 0210 nano-technology, Nucleus, Intracellular

Abstract

The F-actin cytoskeleton of Cryptococcus neoformans is known to comprise actin cables, cortical patches and cytokinetic ring. Here, we describe a new F-actin structure in fungi, a perinuclear F-actin collar ring around the cell nucleus, by fluorescent microscopic imaging of rhodamine phalloidin-stained F-actin. Perinuclear F-actin rings form in Cryptococcus neoformans treated with the microtubule inhibitor Nocodazole or with the drug solvent dimethyl sulfoxide (DMSO) or grown in yeast extract peptone dextrose (YEPD) medium, but they are absent in cells treated with Latrunculin A. Perinuclear F-actin rings may function as 'funicular cabin' for the cell nucleus, and actin cables as intracellular 'funicular' suspending nucleus in the central position in the cell and moving nucleus along the polarity axis along actin cables.

Published

2012

247. Acoustic detection of melanosome transport in Xenopus laevis melanophores

Author

Elisabeth Norström, Christoph Langhammer, Rickard Frost, Sofia Svedhem, Joachim Sturve, Margareta Wallin, and Lovisa J Bodin

Subjects

Biophysics, Xenopus, Melanophores, Biology, Biochemistry, Microtubules, law.invention, chemistry.chemical_compound, Xenopus laevis, Confocal microscopy, law, Organelle, Animals, Melanocyte-Stimulating Hormones, Molecular Biology, Cells, Cultured, Cytoskeleton, Melanosome, Melanins, Melanosomes, Nocodazole, Biological Transport, Cell Biology, Acoustics, biology.organism_classification, Chromatophore, Cell biology, chemistry, Melanosome transport, Quartz Crystal Microbalance Techniques, Latrunculin

Abstract

Organelle transport studies are often performed using melanophores from lower vertebrates due to the ease of inducing movements of pigment granules (melanosomes) and visualizing them by optical microscopy. Here, we present a novel methodology to monitor melanosome translocation (which is a light-sensitive process) in the dark using the quartz crystal microbalance with dissipation monitoring (QCM-D) technique. This acoustic sensing method was used to study dispersion and aggregation of melanosomes in Xenopus laevis melanophores. Reversible sensor responses, correlated to optical reflectance measurements, were obtained by alternating addition and removal of melatonin (leading to melanosome aggregation) and melanocyte-stimulating hormone (MSH) (leading to melanosome dispersion). By confocal microscopy, it was shown that a vertical redistribution of melanosomes occurred during the dispersion/aggregation processes. Furthermore, the transport process was studied in the presence of cytoskeleton-perturbing agents disrupting either actin filaments (latrunculin) or microtubules (nocodazole). Taken together, these experiments suggest that the acoustic responses mainly originate from melanosome transport along actin filaments (located close to the cell membrane), as expected based on the penetration depth of the QCM-D technique. The results clearly indicate the potential of QCM-D for studies of intracellular transport processes in melanophores.

Published

2012

248. Interactions of Isolated C-terminal Fragments of Neural Wiskott-Aldrich Syndrome Protein (N-WASP) with Actin and Arp2/3 Complex

Author

Jean-François Gaucher, Louis Renault, Chloé Maugé, Dominique Didry, Bérengère Guichard, Marie-France Carlier, Cibles Thérapeutiques et conception de médicaments (CiTCoM - UMR 8038), Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS)-Université de Paris (UP), Laboratoire d'Enzymologie et Biochimie Structurales (LEBS), Centre National de la Recherche Scientifique (CNRS), Laboratoire de Biologie Structurale et Radiobiologie (LBSR), Commissariat à l'énergie atomique et aux énergies alternatives (CEA), Institut de Biologie Intégrative de la Cellule (I2BC), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Université Paris-Saclay-Centre National de la Recherche Scientifique (CNRS), and Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS)-Université Paris Cité (UPCité)

Subjects

Repetitive Sequences, Amino Acid, Wiskott-Aldrich Syndrome Protein, Neuronal, Arp2/3 complex, macromolecular substances, Crystallography, X-Ray, Biochemistry, Actin-Related Protein 2-3 Complex, 03 medical and health sciences, Actin filament branching, otorhinolaryngologic diseases, Animals, Humans, Actin-binding protein, Protein Structure, Quaternary, Molecular Biology, ComputingMilieux_MISCELLANEOUS, 030304 developmental biology, 0303 health sciences, biology, 030302 biochemistry & molecular biology, Wiskott–Aldrich syndrome protein, Cell Biology, Actins, Protein Structure, Tertiary, [SDV.BBM.BP]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Biophysics, stomatognathic diseases, Profilin, Multiprotein Complexes, biology.protein, Biophysics, Latrunculin, Cattle, Rabbits, MDia1, biological phenomena, cell phenomena, and immunity, Molecular Biophysics, Protein Binding

Abstract

Wiskott-Aldrich syndrome proteins (WASP) are a family of proteins that all catalyze actin filament branching with the Arp2/3 complex in a variety of actin-based motile processes. The constitutively active C-terminal domain, called VCA, harbors one or more WASP homology 2 (WH2) domains that bind G-actin, whereas the CA extension binds the Arp2/3 complex. The VCA·actin·Arp2/3 entity associates with a mother filament to form a branched junction from which a daughter filament is initiated. The number and function of WH2-bound actin(s) in the branching process are not known, and the stoichiometry of the VCA·actin·Arp2/3 complex is debated. We have expressed the tandem WH2 repeats of N-WASP, either alone (V) or associated with the C (VC) and CA (VCA) extensions. We analyzed the structure of actin in complex with V, VC, and VCA using protein crystallography and hydrodynamic and spectrofluorimetric methods. The partial crystal structure of the VC·actin 1:1 complex shows two actins in the asymmetric unit with extensive actin-actin contacts. In solution, each of the two WH2 domains in V, VC, and VCA binds G-actin in 1:2 complexes that participate in barbed end assembly. V, VC, and VCA enhance barbed end depolymerization like profilin but neither nucleate nor sever filaments, in contrast with other WH2 repeats. VCA binds the Arp2/3 complex in a 1:1 complex even in the presence of a large excess of VCA. VCA·Arp2/3 binds one actin in a latrunculin A-sensitive fashion, in a 1:1:1 complex, indicating that binding of the second actin to VCA is weakened in the ternary complex.

Published

2012

249. Thoracic aortic aneurysm (TAAD)-causing mutation in actin affects formin regulation of polymerization

Author

Elesa W. Wedemeyer, Heather L. Bartlett, Alyson R. Pierick, Lindsey E. Malloy, Sarah E. Bergeron, Kuo-Kuang Wen, Melissa McKane, Nicole D. Vanderpool, and Peter A. Rubenstein

Subjects

Saccharomyces cerevisiae Proteins, Mutation, Missense, Arp2/3 complex, macromolecular substances, Saccharomyces cerevisiae, Biochemistry, Models, Biological, parasitic diseases, Humans, Actin-binding protein, Molecular Biology, biology, Microfilament Proteins, Actin remodeling, food and beverages, Cell Biology, Actin cytoskeleton, Bridged Bicyclo Compounds, Heterocyclic, Molecular biology, Actins, Cell biology, Aortic Aneurysm, carbohydrates (lipids), Actin Cytoskeleton, Profilin, Amino Acid Substitution, Protein Structure and Folding, biology.protein, Latrunculin, Thiazolidines, MDia1, ACTA2

Abstract

More than 30 mutations in ACTA2, which encodes α-smooth muscle actin, have been identified to cause autosomal dominant thoracic aortic aneurysm and dissection. The mutation R256H is of particular interest because it also causes patent ductus arteriosus and moyamoya disease. R256H is one of the more prevalent mutations and, based on its molecular location near the strand-strand interface in the actin filament, may affect F-actin stability. To understand the molecular ramifications of the R256H mutation, we generated Saccharomyces cerevisiae yeast cells expressing only R256H yeast actin as a model system. These cells displayed abnormal cytoskeletal morphology and increased sensitivity to latrunculin A. After cable disassembly induced by transient exposure to latrunculin A, mutant cells were delayed in reestablishing the actin cytoskeleton. In vitro, mutant actin exhibited a higher than normal critical concentration and a delayed nucleation. Consequently, we investigated regulation of mutant actin by formin, a potent facilitator of nucleation and a protein needed for normal vascular smooth muscle cell development. Mutant actin polymerization was inhibited by the FH1-FH2 fragment of the yeast formin, Bni1. This fragment strongly capped the filament rather than facilitating polymerization. Interestingly, phalloidin or the presence of wild type actin reversed the strong capping behavior of Bni1. Together, the data suggest that the R256H actin mutation alters filament conformation resulting in filament instability and misregulation by formin. These biochemical effects may contribute to abnormal histology identified in diseased arterial samples from affected patients.

Published

2012

250. Inhibition of interdomain motion in g-actin by the natural product latrunculin: a molecular dynamics study

Author

Sandra Rennebaum, Amedeo Caflisch, University of Zurich, and Caflisch, Amedeo

Subjects

1303 Biochemistry, Protein Conformation, Motility, Arp2/3 complex, macromolecular substances, Molecular Dynamics Simulation, Biochemistry, Protein filament, 1315 Structural Biology, Adenosine Triphosphate, Structural Biology, 10019 Department of Biochemistry, 1312 Molecular Biology, Animals, Humans, Actin-binding protein, Cytoskeleton, Molecular Biology, Actin, Binding Sites, biology, Chemistry, Actin remodeling, Water, Bridged Bicyclo Compounds, Heterocyclic, Actins, Protein Structure, Tertiary, Biophysics, biology.protein, 570 Life sciences, Latrunculin, Thiazolidines, Rabbits, Protein Multimerization

Abstract

As part of the cytoskeleton, actin is essential for the morphology, motility, and division of eukaryotic cells. Recent X-ray fiber diffraction studies have shown that the conformation of monomeric actin is flattened upon incorporation into the filament by a relative rotation of its two major domains. The antiproliferative activity of latrunculin, a macrolide toxin produced by sponges, seems to be related to its binding to monomeric actin and inhibition of polymerization. Yet, the mechanism of inhibition is not known in detail. Here, multiple explicit water molecular dynamics simulations show that latrunculin binding hinders the conformational transition related to actin polymerization. In particular, the presence of latrunculin at the interface of the two major domains of monomeric actin reduces the correlated displacement of Domain 2 with respect to Domain 1. Moreover, higher rotational flexibility between the two major domains is observed in the absence of ATP as compared to ATP-bound actin, offering a possible explanation as to why actin polymerizes more favorably in the absence of nucleotides. Proteins 2012; © 2012 Wiley Periodicals, Inc.

Published

2012