Cytoplasmic dynamics of myosin IIA and IIB: spatial ‘sorting’ of isoforms in locomoting cells

J. Kolega

doi:10.1242/jcs.111.15.2085

Cytoplasmic dynamics of myosin IIA and IIB: spatial ‘sorting’ of isoforms in locomoting cells

Journal of Cell Science ◽

10.1242/jcs.111.15.2085 ◽

1998 ◽

Vol 111 (15) ◽

pp. 2085-2095 ◽

Cited By ~ 8

Author(s):

J. Kolega

Keyword(s):

Cultured Cells ◽

Myosin Ii ◽

Cell Movement ◽

Leading Edge ◽

Time Lapse ◽

Living Cells ◽

Immunofluorescence Staining ◽

Spatial Sorting ◽

Time Lapse Imaging

Different isoforms of non-muscle myosin II have different distributions in vivo, even within individual cells. In order to understand how these different distributions arise, the distribution and dynamics of non-muscle myosins IIA and myosin IIB were examined in cultured cells using immunofluorescence staining and time-lapse imaging of fluorescent analogs. Cultured bovine aortic endothelia contained both myosins IIA and IIB. Both isoforms distributed along stress fibers, in linear or punctate aggregates within lamellipodia, and diffusely around the nucleus. However, the A isoform was preferentially located toward the leading edge of migrating cells when compared with myosin IIB by double immunofluorescence staining. Conversely, the B isoform was enriched in structures at the cells' trailing edges. When fluorescent analogs of the two isoforms were co-injected into living cells, the injected myosins distributed with the same disparate localizations as endogenous myosins IIA and IIB. This indicated that the ability of the myosins to ‘sort’ within the cytoplasm is intrinsic to the proteins themselves, and not a result of localized synthesis or degradation. Furthermore, time-lapse imaging of injected analogs in living cells revealed differences in the rates at which the two isoforms rearranged during cell movement. The A isoform appeared in newly formed structures more rapidly than the B isoform, and was also lost more rapidly when structures disassembled. These observations suggest that the different localizations of myosins IIA and IIB reflect different rates at which the isoforms transit through assembly, movement and disassembly within the cell. The relative proportions of different myosin II isoforms within a particular cell type may determine the lifetimes of various myosin II-based structures in that cell.

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On the Relationship Between EB-3 Profiles and Microtubules Growth in Cultured Cells

Frontiers in Molecular Biosciences ◽

10.3389/fmolb.2021.745089 ◽

2021 ◽

Vol 8 ◽

Author(s):

Arshat Urazbaev ◽

Anara Serikbaeva ◽

Anna Tvorogova ◽

Azamat Dusenbayev ◽

Sholpan Kauanova ◽

...

Keyword(s):

Growth Velocity ◽

Cultured Cells ◽

Time Lapse ◽

Living Cells ◽

Time Intervals ◽

Mean Values ◽

Microtubule Growth ◽

Dynamic Structures

Microtubules are dynamic structures undergoing rapid growth and shrinkage in living cells and in vitro. The growth of microtubules in vitro was analyzed with subpixel precision (Maurer et al., Current Biology, 2014, 24 (4), 372–384); however, to what extent these results could be applied for microtubules growing in vivo remains largely unknown. Particularly, the question is whether microtubule growth velocity in cells could be sufficiently approximated by a Gaussian distribution or its variability requires a more sophisticated description? Addressing this question, we used time-lapse microscopy and mathematical modeling, and we analyzed EB-3 comets forming on microtubules of cultured cells with subpixel precision. Parameters of comets (shape, form, and velocity) were used as topological characteristics of 3D voxel objects. Using regression analysis, we determined the real positions of the microtubule tips in time-lapse sequences. By exponential decay fitting of the restored comet intensity profile, we found that in vivo EB-3 rapidly exchanges on growing microtubule ends with a decoration time ∼ 2 s. We next developed the model showing that the best correlation between comet length and microtubule end growth velocity is at time intervals close to the decoration time. In the cells, EB comet length positively correlates with microtubule growth velocity in preceding time intervals, while demonstrating no correlation in subsequent time intervals. Correlation between comet length and instantaneous growth velocity of microtubules remains under nocodazole treatment when mean values of both parameters decrease. Our data show that the growth of microtubules in living cells is well-approximated by a constant velocity with large stochastic fluctuations.

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Smurf1 regulates tumor cell plasticity and motility through degradation of RhoA leading to localized inhibition of contractility

The Journal of Cell Biology ◽

10.1083/jcb.200605135 ◽

2006 ◽

Vol 176 (1) ◽

pp. 35-42 ◽

Cited By ~ 119

Author(s):

Erik Sahai ◽

Raquel Garcia-Medina ◽

Jacques Pouysségur ◽

Emmanuel Vial

Keyword(s):

Cell Migration ◽

Tumor Cell ◽

Rho Gtpases ◽

Rho Kinase ◽

Cell Movement ◽

Leading Edge ◽

Cell Periphery ◽

Tumor Cell Migration ◽

Tumor Cell Motility

Rho GTPases participate in various cellular processes, including normal and tumor cell migration. It has been reported that RhoA is targeted for degradation at the leading edge of migrating cells by the E3 ubiquitin ligase Smurf1, and that this is required for the formation of protrusions. We report that Smurf1-dependent RhoA degradation in tumor cells results in the down-regulation of Rho kinase (ROCK) activity and myosin light chain 2 (MLC2) phosphorylation at the cell periphery. The localized inhibition of contractile forces is necessary for the formation of lamellipodia and for tumor cell motility in 2D tissue culture assays. In 3D invasion assays, and in in vivo tumor cell migration, the inhibition of Smurf1 induces a mesenchymal–amoeboid–like transition that is associated with a more invasive phenotype. Our results suggest that Smurf1 is a pivotal regulator of tumor cell movement through its regulation of RhoA signaling.

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An In Vitro Model for Assessing Corneal Keratocyte Spreading and Migration on Aligned Fibrillar Collagen

Journal of Functional Biomaterials ◽

10.3390/jfb9040054 ◽

2018 ◽

Vol 9 (4) ◽

pp. 54 ◽

Cited By ~ 7

Author(s):

Pouriska Kivanany ◽

Kyle Grose ◽

Nihan Yonet-Tanyeri ◽

Sujal Manohar ◽

Yukta Sunkara ◽

...

Keyword(s):

Growth Factor ◽

Transforming Growth Factor Beta ◽

Transforming Growth Factor ◽

Cell Movement ◽

Time Lapse ◽

Collagen Fibrils ◽

Fibrillar Collagen ◽

Freeze Injury

Background: Corneal stromal cells (keratocytes) are responsible for developing and maintaining normal corneal structure and transparency, and for repairing the tissue after injury. Corneal keratocytes reside between highly aligned collagen lamellae in vivo. In addition to growth factors and other soluble biochemical factors, feedback from the extracellular matrix (ECM) itself has been shown to modulate corneal keratocyte behavior. Methods: In this study, we fabricate aligned collagen substrates using a microfluidics approach and assess their impact on corneal keratocyte morphology, cytoskeletal organization, and patterning after stimulation with platelet derived growth factor (PDGF) or transforming growth factor beta 1 (TGFβ). We also use time-lapse imaging to visualize the dynamic interactions between cells and fibrillar collagen during wound repopulation following an in vitro freeze injury. Results: Significant co-alignment between keratocytes and aligned collagen fibrils was detected, and the degree of cell/ECM co-alignment further increased in the presence of PDGF or TGFβ. Freeze injury produced an area of cell death without disrupting the collagen. High magnification, time-lapse differential interference contrast (DIC) imaging allowed cell movement and subcellular interactions with the underlying collagen fibrils to be directly visualized. Conclusions: With continued development, this experimental model could be an important tool for accessing how the integration of multiple biophysical and biochemical signals regulate corneal keratocyte differentiation.

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Topical Review: Neuronal Migration in Cortical Development

Journal of Child Neurology ◽

10.1177/08830738040190030201 ◽

2004 ◽

Vol 19 (3) ◽

pp. 274-279

Author(s):

Shigeaki Kanatani ◽

Hidenori Tabata ◽

Kazunori Nakajima

Keyword(s):

Neuronal Migration ◽

Radial Glia ◽

Asymmetric Cell Division ◽

Time Lapse ◽

Radial Glial Cells ◽

Daughter Cells ◽

Radial Glial ◽

Time Lapse Imaging ◽

Mitotic Behavior

Cortical formation in the developing brain is a highly complicated process involving neuronal production (through symmetric or asymmetric cell division) interaction of radial glia with neuronal migration, and multiple modes of neuronal migration. It has been convincingly demonstrated by numerous studies that radial glial cells are neural stem cells. However, the processes by which neurons arise from radial glia and migrate to their final destinations in vivo are not yet fully understood. Recent studies using time-lapse imaging of neuronal migration are giving investigators an increasingly more detailed understanding of the mitotic behavior of radial glia and the migrating behavior of their daughter cells. In this review, we describe recent progress in elucidating neuronal migration in brain formation and how neuronal migration is disturbed by mutations in genes that control this process. ( J Child Neurol 2005;20:274—279).

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Individual neuronal subtypes control initial myelin sheath growth and stabilization

Neural Development ◽

10.1186/s13064-020-00149-3 ◽

2020 ◽

Vol 15 (1) ◽

Author(s):

Heather N. Nelson ◽

Anthony J. Treichel ◽

Erin N. Eggum ◽

Madeline R. Martell ◽

Amanda J. Kaiser ◽

...

Keyword(s):

Spinal Cord ◽

Central Nervous System ◽

Nervous System ◽

Myelin Sheath ◽

Time Lapse ◽

Marked Individual ◽

Larval Zebrafish ◽

Sheath Formation ◽

Time Lapse Imaging

Abstract Background In the developing central nervous system, pre-myelinating oligodendrocytes sample candidate nerve axons by extending and retracting process extensions. Some contacts stabilize, leading to the initiation of axon wrapping, nascent myelin sheath formation, concentric wrapping and sheath elongation, and sheath stabilization or pruning by oligodendrocytes. Although axonal signals influence the overall process of myelination, the precise oligodendrocyte behaviors that require signaling from axons are not completely understood. In this study, we investigated whether oligodendrocyte behaviors during the early events of myelination are mediated by an oligodendrocyte-intrinsic myelination program or are over-ridden by axonal factors. Methods To address this, we utilized in vivo time-lapse imaging in embryonic and larval zebrafish spinal cord during the initial hours and days of axon wrapping and myelination. Transgenic reporter lines marked individual axon subtypes or oligodendrocyte membranes. Results In the larval zebrafish spinal cord, individual axon subtypes supported distinct nascent sheath growth rates and stabilization frequencies. Oligodendrocytes ensheathed individual axon subtypes at different rates during a two-day period after initial axon wrapping. When descending reticulospinal axons were ablated, local spinal axons supported a constant ensheathment rate despite the increased ratio of oligodendrocytes to target axons. Conclusion We conclude that properties of individual axon subtypes instruct oligodendrocyte behaviors during initial stages of myelination by differentially controlling nascent sheath growth and stabilization.

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Actomyosin-based Retrograde Flow of Microtubules in the Lamella of Migrating Epithelial Cells Influences Microtubule Dynamic Instability and Turnover and Is Associated with Microtubule Breakage and Treadmilling

The Journal of Cell Biology ◽

10.1083/jcb.139.2.417 ◽

1997 ◽

Vol 139 (2) ◽

pp. 417-434 ◽

Cited By ~ 315

Author(s):

Clare M. Waterman-Storer ◽

E.D. Salmon

Keyword(s):

Epithelial Cells ◽

Dynamic Instability ◽

Leading Edge ◽

Unknown Origin ◽

Time Lapse ◽

Lung Epithelial Cells ◽

Retrograde Flow ◽

Microtubule Dynamic ◽

Lung Epithelial ◽

Time Lapse Imaging

We have discovered several novel features exhibited by microtubules (MTs) in migrating newt lung epithelial cells by time-lapse imaging of fluorescently labeled, microinjected tubulin. These cells exhibit leading edge ruffling and retrograde flow in the lamella and lamellipodia. The plus ends of lamella MTs persist in growth perpendicular to the leading edge until they reach the base of the lamellipodium, where they oscillate between short phases of growth and shortening. Occasionally “pioneering” MTs grow into the lamellipodium, where microtubule bending and reorientation parallel to the leading edge is associated with retrograde flow. MTs parallel to the leading edge exhibit significantly different dynamics from MTs perpendicular to the cell edge. Both parallel MTs and photoactivated fluorescent marks on perpendicular MTs move rearward at the 0.4 μm/min rate of retrograde flow in the lamella. MT rearward transport persists when MT dynamic instability is inhibited by 100-nM nocodazole but is blocked by inhibition of actomyosin by cytochalasin D or 2,3-butanedione–2-monoxime. Rearward flow appears to cause MT buckling and breaking in the lamella. 80% of free minus ends produced by breakage are stable; the others shorten and pause, leading to MT treadmilling. Free minus ends of unknown origin also depolymerize into the field of view at the lamella. Analysis of MT dynamics at the centrosome shows that these minus ends do not arise by centrosomal ejection and that ∼80% of the MTs in the lamella are not centrosome bound. We propose that actomyosin-based retrograde flow of MTs causes MT breakage, forming quasi-stable noncentrosomal MTs whose turnover is regulated primarily at their minus ends.

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In Vivo Time-Lapse Imaging of Neuronal Development inXenopus

Cold Spring Harbor Protocols ◽

10.1101/pdb.top077156 ◽

2013 ◽

Vol 2013 (9) ◽

pp. pdb.top077156 ◽

Cited By ~ 4

Author(s):

Edward S. Ruthazer ◽

Anne Schohl ◽

Neil Schwartz ◽

Aydin Tavakoli ◽

Marc Tremblay ◽

...

Keyword(s):

Neuronal Development ◽

Time Lapse ◽

Time Lapse Imaging

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Scribble, Lgl1, and myosin II form a complex in vivo to promote directed cell migration

Molecular Biology of the Cell ◽

10.1091/mbc.e19-11-0657 ◽

2020 ◽

Vol 31 (20) ◽

pp. 2234-2248

Author(s):

Maha Abedrabbo ◽

Shoshana Ravid

Keyword(s):

Cell Migration ◽

Cell Adhesion ◽

Myosin Ii ◽

Leading Edge ◽

Directed Cell Migration ◽

Lethal Giant Larvae ◽

And Migration ◽

Migrating Cells

Here we show that Scribble (Scrib), Lethal giant larvae 1 (Lgl1), and myosin II form a complex in vivo and colocalize at the cell leading edge of migrating cells, and this colocalization is interdependent. Scrib and Lgl1 are required for proper cell adhesion, polarity, and migration.

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Examining seizure-induced effects on the dendritic growth of immature neurons, using in vivo time-lapse imaging of the intact juvenile brain

Clinical Neurophysiology ◽

10.1016/j.clinph.2007.03.028 ◽

2007 ◽

Vol 118 (7) ◽

pp. e186

Author(s):

D. Sesath Hewapathirane ◽

Simon Chen ◽

Wesley Yen ◽

Kurt Haas

Keyword(s):

Dendritic Growth ◽

Time Lapse ◽

Immature Neurons ◽

Time Lapse Imaging

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Cytostructural dynamics of spreading and translocating cells.

The Journal of Cell Biology ◽

10.1083/jcb.95.1.127 ◽

1982 ◽

Vol 95 (1) ◽

pp. 127-136 ◽

Cited By ~ 54

Author(s):

T Soranno ◽

E Bell

Keyword(s):

Cell Nucleus ◽

Compression Wave ◽

Radial Stress ◽

Leading Edge ◽

Time Lapse ◽

Living Cells ◽

Stress Fibers ◽

Immunofluorescent Staining ◽

Transitional Stage ◽

Compression Waves

Cytostructural changes during fibroblast spreading and translocation and during the transition between the two states have been studied in living cells and in the same cells after fixation and immunofluorescent staining. In time-lapse sequences we observe that birefringent arcs, sometimes circles, concentric with the cell perimeter, form near the periphery of a spreading cell, or that arcs form near the leading edge of a locomoting cell. The arcs move toward the nucleus, where they disappear. In spreading cells, radial stress fibers extend from the region of the cell nucleus to the periphery. The arcs or circles and the stress fibers are visualized in the same cells after fixation and staining with fluorescein-conjugated antiactin antibodies. Stained images of spreading cells show the arcs and stress fibers in the same plane of focus. At points of intersection with arcs, stress fibers are bent toward the substrate on which the cell is moving. During a transitional stage between spreading and translocation the cytostructure undergoes reproducible changes. Arcs and circle cease to form. The radial stress fibers elongate, spiral around the nucleus, and move to the periphery as a band of filaments. We interpret the moving arcs as condensations of a microfilament network that move toward the nucleus as compression waves. As elements of the net are brought close together by the compression wave, contraction may occur and facilitate the condensations.

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