Calcium-Calmodulin Suppresses the Filamentous Actin-Binding Activity of a 135-Kilodalton Actin-Bundling Protein Isolated from Lily Pollen Tubes

Etsuo Yokota; Shoshi Muto; Teruo Shimmen

doi:10.1104/pp.123.2.645

Enolase exists in the fluid phase of cytoplasm in 3T3 cells

Journal of Cell Science ◽

10.1242/jcs.94.2.333 ◽

1989 ◽

Vol 94 (2) ◽

pp. 333-342

Author(s):

L. Pagliaro ◽

K. Kerr ◽

D.L. Taylor

Keyword(s):

Diffusion Coefficient ◽

Fluid Phase ◽

Glycolytic Enzyme ◽

Binding Activity ◽

Actin Binding ◽

Filamentous Actin ◽

3T3 Cells ◽

Ratio Imaging

We have investigated the intracellular distribution and mobility of the glycolytic enzyme enolase, using functional fluorescent analogs labeled with the succinimidyl esters of carboxyfluorescein (F1-enolase) and carboxytetramethylrhodamine (Rh-enolase) In contrast to aldolase, neither native enolase nor labeled enolase gelled filamentous actin (F-actin), as measured by falling-ball viscometry, indicating a lack of interaction between enolase and F-actin. Fluorescence redistribution after photo-bleaching (FRAP) measurements of the diffusion coefficient (D) of F1-enolase in aqueous solutions gave a value of D37,aq = 6.08 × 10(−7) cm2s-1, and no immobile fraction, consistent with a native molecular weight of 90,000. These values were not significantly different with Rh-enolase, or in the presence of F-actin, 2-phosphoglycerate or F-actin-aldolase gels, demonstrating that neither F1-enolase nor Rh-enolase binds to F-actin or aldolase in vitro. FRAP measurements of F1- and Rh-enolase microinjected into living Swiss 3T3 cells revealed spatial differences in the diffusion coefficient, but not the mobile fraction. In the perinuclear cytoplasm, we measured an apparent diffusion coefficient of 1.1 × 10(−7) cm2s-1, compared to 7.1 × 10(−8) cm2s-1 in the peripheral cytoplasm, with approximately 100% mobility of F1- or Rh-enolase in both regions. Imaging of cells co-injected with Rh-enolase and size-fractionated FITC-dextran (FD-90) revealed that Rh-enolase entered the nucleus, while FD-90 was excluded. Ratio imaging showed a relatively high nuclear ratio of Rh-enolase/FD-90, and a uniform cytoplasmic ratio, with no indication of increased concentration of enolase around stress fibers. These data demonstrate that Rh- and F1-enolase do not bind to F-actin in vitro, and are 100% mobile in vivo. Together with our recent finding that a significant fraction of aldolase binds to F-actin in vitro and is immobile in vivo, these data suggest a correlation between actin-binding activity and cytoplasmic mobility of glycolytic enzymes.

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Mechanism of Ca2+ inhibition of cytoplasmic streaming in lily pollen tubes

Journal of Cell Science ◽

10.1242/jcs.91.4.501 ◽

1988 ◽

Vol 91 (4) ◽

pp. 501-509 ◽

Cited By ~ 1

Author(s):

TADASHI KOHNO ◽

TERUO SHIMMEN

Keyword(s):

Actin Filaments ◽

Cytoplasmic Streaming ◽

Lilium Longiflorum ◽

Pollen Tubes ◽

Ionophore A23187 ◽

Filamentous Actin ◽

Actin Bundles ◽

Lily Pollen ◽

Subsequent Decrease

Using a Ca2+ ionophore, A23187, the free Ca2+ concentration ([Ca2+]) in the cytoplasm of pollen tubes of Lilium longiflorum was controlled from the cell exterior. At [Ca2+] higher than 1.0x10−5M (pCa5.0), cytoplasmic streaming was inhibited, and the inhibition was irreversible. The ATP content did not change, but actin filaments were fragmented and formed aggregates. A subsequent decrease in [Ca2+] almost stopped the progress of the actin filament fragmentation, but filamentous actin did not re-form from the fragmented actin. In a previous paper, we reported that pollen tube organelle movement along characean actin bundles was inhibited by Ca2+ at 10−5M levels and the inhibition was reversible. In the present study, the reversibility was also demonstrated using an in situ Ca2+ treatment. Organelles were isolated from pollen tubes that had been treated with high [Ca2+] and A23187. They moved along characean actin bundles in Ca2+-free medium. It is concluded that Ca2+ inhibition of cytoplasmic streaming can be attributed to both inactivation of myosin and fragmentation of actin. The irreversibility of Ca2+ inhibition in situ is attributed to the irreversible fragmentation of actin filaments.

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Elongation factor-1 alpha is an overexpressed actin binding protein in metastatic rat mammary adenocarcinoma

Journal of Cell Science ◽

10.1242/jcs.109.11.2705 ◽

1996 ◽

Vol 109 (11) ◽

pp. 2705-2714 ◽

Cited By ~ 7

Author(s):

B.T. Edmonds ◽

J. Wyckoff ◽

Y.G. Yeung ◽

Y. Wang ◽

E.R. Stanley ◽

...

Keyword(s):

Actin Cytoskeleton ◽

Elongation Factor ◽

Metastatic Potential ◽

Cell Types ◽

Binding Activity ◽

Mammary Adenocarcinoma ◽

Actin Binding ◽

Filamentous Actin ◽

Elongation Factor 1 Alpha ◽

Elongation Factor 1

Overexpression of elongation factor-1 alpha (EF1 alpha) mRNA has been correlated with increased metastatic potential in mammary adenocarcinoma; however, this relationship was not explored at the level of protein expression. As EF1 alpha has been shown in other cell types to be a component of the actin cytoskeleton, a likely effector in metastasis, the actin binding activity of EF1 alpha from metastatic and nonmetastatic rat breast tumors and cell lines was investigated. We have shown that EF1 alpha protein is overexpressed in metastatic compared to nonmetastatic cells and whole tumors. Similarly to other EF1 alpha s, both types of tumor EF1 alpha bind to F-actin, but EF1 alpha from metastatic cells has a reduced affinity for actin. In addition, there is a high correlation between the intracellular distribution of filamentous actin and EF1 alpha in those cytoskeletal structures thought to be important for supporting the cellular motility required for metastasis. Following stimulation with EGF, there is a parallel increase in the amount of F-actin and EF1 alpha associated with the cytoskeleton. The response to EGF can be blocked with cytochalasin D indicating that the binding of EF1 alpha to the cytoskeleton is mediated by F-actin. We propose that a weakened association of EF1 alpha with actin may be related to the metastatic process via an altered organization of the actin cytoskeleton and the differential translation of mRNAs associated with the cytoskeleton.

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Cortactin, an 80/85-kilodalton pp60src substrate, is a filamentous actin-binding protein enriched in the cell cortex.

The Journal of Cell Biology ◽

10.1083/jcb.120.6.1417 ◽

1993 ◽

Vol 120 (6) ◽

pp. 1417-1426 ◽

Cited By ~ 361

Author(s):

H Wu ◽

J T Parsons

Keyword(s):

Binding Protein ◽

Cell Types ◽

Sh3 Domain ◽

Binding Activity ◽

Actin Binding ◽

Cell Cortex ◽

Filamentous Actin ◽

Actin Binding Protein ◽

Amino Terminal ◽

Multiple Copies

Two related cellular proteins, p80 and p85 (cortactin), become phosphorylated on tyrosine in pp60src-transformed cells and in cells stimulated with certain growth factors. The amino-terminal half of cortactin is comprised of multiple copies of an internal, tandem 37-amino acid repeat. The carboxyl-terminal half contains a distal SH3 domain. We report that cortactin is an F-actin-binding protein. The binding to F-actin is specific and saturable. The amino-terminal repeat region appears to be both necessary and sufficient to mediate actin binding, whereas the SH3 domain had no apparent effect on the actin-binding activity. Cortactin, present in several different cell types, is enriched in cortical structures such as membrane ruffles and lamellipodia. The properties of cortactin indicate that it may be important for microfilament-membrane interactions as well as transducing signals from the cell surface to the cytoskeleton. We suggest the name cortactin, reflecting the cortical subcellular localization and its actin-binding activity.

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Cofilin is a pH sensor for actin free barbed end formation: role of phosphoinositide binding

The Journal of Cell Biology ◽

10.1083/jcb.200804161 ◽

2008 ◽

Vol 183 (5) ◽

pp. 865-879 ◽

Cited By ~ 122

Author(s):

Christian Frantz ◽

Gabriela Barreiro ◽

Laura Dominguez ◽

Xiaoming Chen ◽

Robert Eddy ◽

...

Keyword(s):

Actin Filament ◽

Structural Changes ◽

Ph Sensor ◽

Ph Sensitive ◽

Actin Binding ◽

Filamentous Actin ◽

Filament Dynamics ◽

Ph Dependent ◽

Dynamics Simulations

Newly generated actin free barbed ends at the front of motile cells provide sites for actin filament assembly driving membrane protrusion. Growth factors induce a rapid biphasic increase in actin free barbed ends, and we found both phases absent in fibroblasts lacking H+ efflux by the Na-H exchanger NHE1. The first phase is restored by expression of mutant cofilin-H133A but not unphosphorylated cofilin-S3A. Constant pH molecular dynamics simulations and nuclear magnetic resonance (NMR) reveal pH-sensitive structural changes in the cofilin C-terminal filamentous actin binding site dependent on His133. However, cofilin-H133A retains pH-sensitive changes in NMR spectra and severing activity in vitro, which suggests that it has a more complex behavior in cells. Cofilin activity is inhibited by phosphoinositide binding, and we found that phosphoinositide binding is pH-dependent for wild-type cofilin, with decreased binding at a higher pH. In contrast, phosphoinositide binding by cofilin-H133A is attenuated and pH insensitive. These data suggest a molecular mechanism whereby cofilin acts as a pH sensor to mediate a pH-dependent actin filament dynamics.

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Osmotic stress and the yeast cytoskeleton: phenotype-specific suppression of an actin mutation.

The Journal of Cell Biology ◽

10.1083/jcb.118.3.561 ◽

1992 ◽

Vol 118 (3) ◽

pp. 561-571 ◽

Cited By ~ 157

Author(s):

S Chowdhury ◽

K W Smith ◽

M C Gustin

Keyword(s):

Osmotic Stress ◽

Actin Filament ◽

Physiological Process ◽

Actin Binding ◽

Temperature Sensitive ◽

Filamentous Actin ◽

Cortical Actin ◽

Yeast Saccharomyces Cerevisiae ◽

Rhodamine Phalloidin ◽

Diploid Cells

In the yeast Saccharomyces cerevisiae, actin filaments function to direct cell growth to the emerging bud. Yeast has a single essential actin gene, ACT1. Diploid cells containing a single copy of ACT1 are osmosensitive (Osms), i.e., they fail to grow in high osmolarity media (D. Shortle, unpublished observations cited by Novick, P., and D. Botstein. 1985. Cell. 40:415-426). This phenotype suggests that an underlying physiological process involving actin is osmosensitive. Here, we demonstrate that this physiological process is a rapid and reversible change in actin filament organization in cells exposed to osmotic stress. Filamentous actin was stained using rhodamine phalloidin. Increasing external osmolarity caused a rapid loss of actin filament cables, followed by a slower redistribution of cortical actin filament patches. In the recovery phase, cables and patches were restored to their original levels and locations. Strains containing an act1-1 mutation are both Osms and temperature-sensitive (Ts) (Novick and Botstein, 1985). To identify genes whose products functionally interact with actin in cellular responses to osmotic stress, we have isolated extragenic suppressors which revert only the Osms but not the Ts phenotype of an act1-1 mutant. These suppressors identify three genes, RAH1-RAH3. Morphological and genetic properties of a dominant suppressor mutation suggest that the product of the wild-type allele, RAH3+, is an actin-binding protein that interacts with actin to allow reassembly of the cytoskeleton following osmotic stress.

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Purification and characterization of a nonpolymerizing long-pitch actin dimer

Biochemistry and Cell Biology ◽

10.1139/o06-091 ◽

2006 ◽

Vol 84 (5) ◽

pp. 695-702 ◽

Cited By ~ 1

Author(s):

Braden Sweeting ◽

John F. Dawson

Keyword(s):

Critical Concentration ◽

Dnase I ◽

Actin Binding ◽

Wild Type ◽

Filamentous Actin ◽

Rhodamine Phalloidin ◽

Fold Reduction ◽

Crystallization Conditions ◽

Self Association ◽

Pointed End

Atomic resolution structures of filamentous actin have not been obtained owing to the self-association of actin under crystallization conditions. Obtaining short filamentous actin complexes of defined lengths is therefore a highly desirable goal. Here we report the production and isolation of a long-pitch actin dimer employing chemical crosslinking between wild-type actin and Q41C/C374A mutant actin. The Q41C/C374A mutant actin possessed altered polymerization properties, with a 2-fold reduction in the rate of elongation and an increased critical concentration relative to wild-type actin. The Q41C/C374A mutant actin also displayed an increase in the IC50 for DNase I, a pointed-end actin-binding protein. The long-pitch dimer was bound by DNase I to prevent polymerization and purified. It was found that each actin dimer is bound by 2 DNase I molecules, 1 likely bound to each of the actin protomers. The long-pitch dimer bound by DNase I did not form short F actin structures, as assessed by the binding of rhodamine–phalloidin.

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αE-catenin actin-binding domain alters actin filament conformation and regulates binding of nucleation and disassembly factors

Molecular Biology of the Cell ◽

10.1091/mbc.e13-07-0388 ◽

2013 ◽

Vol 24 (23) ◽

pp. 3710-3720 ◽

Cited By ~ 62

Author(s):

Scott D. Hansen ◽

Adam V. Kwiatkowski ◽

Chung-Yueh Ouyang ◽

HongJun Liu ◽

Sabine Pokutta ◽

...

Keyword(s):

Actin Filament ◽

Actin Filaments ◽

Binding Domain ◽

Actin Binding ◽

Filamentous Actin ◽

Filament Structure ◽

Actin Binding Domain ◽

Filament Bundles ◽

Underlying Mechanisms ◽

Cell Cell

The actin-binding protein αE-catenin may contribute to transitions between cell migration and cell–cell adhesion that depend on remodeling the actin cytoskeleton, but the underlying mechanisms are unknown. We show that the αE-catenin actin-binding domain (ABD) binds cooperatively to individual actin filaments and that binding is accompanied by a conformational change in the actin protomer that affects filament structure. αE-catenin ABD binding limits barbed-end growth, especially in actin filament bundles. αE-catenin ABD inhibits actin filament branching by the Arp2/3 complex and severing by cofilin, both of which contact regions of the actin protomer that are structurally altered by αE-catenin ABD binding. In epithelial cells, there is little correlation between the distribution of αE-catenin and the Arp2/3 complex at developing cell–cell contacts. Our results indicate that αE-catenin binding to filamentous actin favors assembly of unbranched filament bundles that are protected from severing over more dynamic, branched filament arrays.

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Structure of the Lifeact–F-actin complex

PLoS Biology ◽

10.1371/journal.pbio.3000925 ◽

2020 ◽

Vol 18 (11) ◽

pp. e3000925 ◽

Cited By ~ 1

Author(s):

Alexander Belyy ◽

Felipe Merino ◽

Oleg Sitsel ◽

Stefan Raunser

Keyword(s):

Hypervariable Region ◽

Binding Pocket ◽

Actin Binding ◽

Filamentous Actin ◽

Activity Measurements ◽

High Resolution Structure ◽

D Loop ◽

Hydrophobic Binding

Lifeact is a short actin-binding peptide that is used to visualize filamentous actin (F-actin) structures in live eukaryotic cells using fluorescence microscopy. However, this popular probe has been shown to alter cellular morphology by affecting the structure of the cytoskeleton. The molecular basis for such artefacts is poorly understood. Here, we determined the high-resolution structure of the Lifeact–F-actin complex using electron cryo-microscopy (cryo-EM). The structure reveals that Lifeact interacts with a hydrophobic binding pocket on F-actin and stretches over 2 adjacent actin subunits, stabilizing the DNase I-binding loop (D-loop) of actin in the closed conformation. Interestingly, the hydrophobic binding site is also used by actin-binding proteins, such as cofilin and myosin and actin-binding toxins, such as the hypervariable region of TccC3 (TccC3HVR) from Photorhabdus luminescens and ExoY from Pseudomonas aeruginosa. In vitro binding assays and activity measurements demonstrate that Lifeact indeed competes with these proteins, providing an explanation for the altering effects of Lifeact on cell morphology in vivo. Finally, we demonstrate that the affinity of Lifeact to F-actin can be increased by introducing mutations into the peptide, laying the foundation for designing improved actin probes for live cell imaging.

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Modulation of Nuclear Localization of the Influenza Virus Nucleoprotein through Interaction with Actin Filaments

Journal of Virology ◽

10.1128/jvi.73.3.2222-2231.1999 ◽

1999 ◽

Vol 73 (3) ◽

pp. 2222-2231 ◽

Cited By ~ 82

Author(s):

Paul Digard ◽

Debra Elton ◽

Konrad Bishop ◽

Elizabeth Medcalf ◽

Alan Weeds ◽

...

Keyword(s):

Influenza Virus ◽

Nuclear Localization ◽

Virus Genome ◽

Actin Binding ◽

Filamentous Actin ◽

Nuclear Localization Signals ◽

Infected Cells ◽

Cytoplasmic Accumulation ◽

High Level

ABSTRACT The influenza virus genome is transcribed in the nuclei of infected cells but assembled into progeny virions in the cytoplasm. This is reflected in the cellular distribution of the virus nucleoprotein (NP), a protein which encapsidates genomic RNA to form ribonucleoprotein structures. At early times postinfection NP is found in the nucleus, but at later times it is found predominantly in the cytoplasm. NP contains several sequences proposed to act as nuclear localization signals (NLSs), and it is not clear how these are overridden to allow cytoplasmic accumulation of the protein. We find that NP binds tightly to filamentous actin in vitro and have identified a cluster of residues in NP essential for the interaction. Complexes containing RNA, NP, and actin could be formed, suggesting that viral ribonucleoproteins also bind actin. In cells, exogenously expressed NP when expressed at a high level partitioned to the cytoplasm, where it associated with F-actin stress fibers. In contrast, mutants unable to bind F-actin efficiently were imported into the nucleus even under conditions of high-level expression. Similarly, nuclear import of NLS-deficient NP molecules was restored by concomitant disruption of F-actin binding. We propose that the interaction of NP with F-actin causes the cytoplasmic retention of influenza virus ribonucleoproteins.

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