Ultrastructure of the yeast actin cytoskeleton and its association with the plasma membrane.

Mulholland, Jon; Preuss, Daphne; Moon, Anne; Wong, Alice S.T.; Drubin, David G.; Botstein, David

doi:10.1083/jcb.125.2.381

Cited by 347 publications

(296 citation statements)

References 32 publications

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“…We did not detect any actin cable-like structures in our preparations, nor are cables apparent in intact spheroplasts, which lack obvious cell polarity. Our results extend upon a previous model in which actin filaments wind around finger-like invaginations of the plasma membrane (Mulholland et al, 1994). We show that actin patches are conical or mound-like structures rising out of the plasma membrane and suggest that they are composed of short filaments arranged into an apparently cross-linked scaffold that surrounds a membrane core.…”

Section: Ultrastructure Of Cortical Actin Patches In Yeastsupporting

confidence: 76%

“…However, actin filaments do not show up well in the crowded yeast cytoplasm, except for rare actin cables in Saccharomyces cerevisiae and pathogenic yeasts (Adams and Pringle, 1984;Kopecka et al, 2001;Yamaguchi et al, 2002), cytoplasmic "filasomes" distinct from cortical patches in fission yeast (Kanbe et al, 1989;Takagi et al, 2003), and aberrant filamentous actin structures in mutant budding yeast defective in endocytosis (Sekiya-Kawasaki et al, 2003). Immunolabeled thin sections have in some cases revealed finger-like invaginations of the plasma membrane apparently entwined in an actin helix (Mulholland et al, 1994). However, these structures are two-dimensional and thus provide limited information about geometry and spatial relations within cortical actin patches.…”

Section: Introductionmentioning

confidence: 99%

“…An ultrastructural analysis of the cortical actin cytoskeleton would provide a powerful basis for understanding the function of actin in endocytosis by allowing highresolution visual comparisons of actin and membrane structures in wild-type and mutant yeast strains. Attempts have been made to visualize yeast actin filaments by thinsection electron microscopy (Adams and Pringle, 1984;Mulholland et al, 1994). However, actin filaments do not show up well in the crowded yeast cytoplasm, except for rare actin cables in Saccharomyces cerevisiae and pathogenic yeasts (Adams and Pringle, 1984;Kopecka et al, 2001;Yamaguchi et al, 2002), cytoplasmic "filasomes" distinct from cortical patches in fission yeast (Kanbe et al, 1989;Takagi et al, 2003), and aberrant filamentous actin structures in mutant budding yeast defective in endocytosis (Sekiya-Kawasaki et al, 2003).…”

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Actin and Septin Ultrastructures at the Budding Yeast Cell Cortex

Rodal

Kozubowski

Goode

et al. 2005

MBoC

174

162

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Budding yeast has been a powerful model organism for studies of the roles of actin in endocytosis and septins in cell division and in signaling. However, the depth of mechanistic understanding that can be obtained from such studies has been severely hindered by a lack of ultrastructural information about how actin and septins are organized at the cell cortex. To address this problem, we developed rapid-freeze and deep-etch techniques to image the yeast cell cortex in spheroplasted cells at high resolution. The cortical actin cytoskeleton assembles into conical or mound-like structures composed of short, cross-linked filaments. The Arp2/3 complex localizes near the apex of these structures, suggesting that actin patch assembly may be initiated from the apex. Mutants in cortical actin patch components with defined defects in endocytosis disrupted different stages of cortical actin patch assembly. Based on these results, we propose a model for actin function during endocytosis. In addition to actin structures, we found that septin-containing filaments assemble into two kinds of higher order structures at the cell cortex: rings and ordered gauzes. These images provide the first high-resolution views of septin organization in cells. INTRODUCTIONBudding yeast has been used for over 20 yr as a model organism to study cytoskeletal function because the genes encoding many components of the cytoskeleton are conserved and because yeast cells are readily amenable to parallel genetic, biochemical, and cell biological analyses. Despite rapid advances in defining the components of the yeast cytoskeleton, its ultrastructure has been difficult to image at the resolution of the electron microscope, with the exception of microtubules (O'Toole et al., 1999). This may be due to the low abundance of the cytoskeleton in yeast relative to mammalian cells, to the presence of a cell wall that complicates extraction procedures, and to high ribosome density in the yeast cytoplasm. As a result, there has been a conspicuous deficit in our understanding of the higher order organization of actin and septin polymers in vivo (Pruyne and Bretscher, 2000). Thus, although it is possible to rapidly identify and mutate cytoskeletal proteins in yeast, there is no method by which to examine the ultrastructural consequences of these mutations. This gap could be filled by developing an approach to image the yeast cytoskeleton at high resolution.The yeast actin cytoskeleton is organized into three distinct structures: motile cortical patches that are polarized in the growing bud, actin cables that run along the motherdaughter cell axis, and a contractile cytokinetic ring at the neck of dividing cells (reviewed in Pruyne and Bretscher, 2000). Cortical actin patches contain many of the actin-associated proteins common to all eukaryotes (Goode and Rodal, 2001) and are composed of actin filaments that undergo rapid turnover (Ayscough et al., 1997). Actin is essential for yeast endocytosis (Kubler and Riezman, 1993). A number of recent studies suggest that act...

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Section: Ultrastructure Of Cortical Actin Patches In Yeastsupporting

confidence: 76%

Section: Introductionmentioning

confidence: 99%

mentioning

confidence: 99%

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Actin and Septin Ultrastructures at the Budding Yeast Cell Cortex

Rodal

Kozubowski

Goode

et al. 2005

MBoC

174

162

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“…At cytokinesis, the actin cytoskeleton is reorganized and actin patches are relocalized to the mother-daughter neck where the cell wall is modified for cell separation. The mechanisms by which actin mediates polarized secretion are not well understood, but it has been shown that cortical actin patches are associated with the cell surface through an invagination of the plasma membrane (Mulholland et al, 1994) and it has been suggested that components of the secretory pathway (endoplasmic reticulum [ER] and Golgi) could be transported into the bud to direct localized growth presumably via an actin-dependent mechanism (Preuss et al, 1992).A variety of proteins have been shown to be required for either bud emergence or for bud site selection (for recent reviews see Bretscher et al, 1994;Chant, 1994; Welch and Drubin, 1994). CDC42, encoding a small GTP-binding protein, and several genes encoding its regulators are involved in bud emergence: cells mutated in these genes arrest as large unbudded cells with a disorganized actin cytoskeleton and delocalized chitin.…”

mentioning

confidence: 99%

BED1, a gene encoding a galactosyltransferase homologue, is required for polarized growth and efficient bud emergence in Saccharomyces cerevisiae.

Mondésert

Reed

1996

The Journal of Cell Biology

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Abstract. The ellipsoidal shape of the yeast Saccharomyces cerevisiae is the result of successive isotropic/apical growth switches that are regulated in a cell cycledependent manner. It is thought that growth polarity is governed by the remodeling of the actin cytoskeleton that is itself under the control of the cell cycle machinery. The cell cycle and the morphogenesis cycle are tightly coupled and it has been recently suggested that a morphogenesis/polarity checkpoint control monitors bud emergence in order to maintain the coupling of these two events (Lew, D. J., and S. I. Reed. 1995. J. Cell BioL 129:739-749). During a screen based on the inability of cells impaired in the budding process to survive when the morphogenesis checkpoint control is abolished, we identified and characterized BED1, a new gene that is required for efficient budding. Cells carrying a disrupted allele of BED1 no longer have the wild-type ellipsoidal shape characteristic of S. cerevisiae, are larger than wild-type cells, are deficient in bud emergence, and depend upon an intact morphogenesis checkpoint control to survive. These cells show defects in polarized growth despite the fact that the actin cytoskeleton appears normal. Our results suggest that Bedl is a type II membrane protein localized in the endoplasmic reticulum. BED1 is significantly homologous to gma12 ÷, a S. pombe gene coding for an et-l,2-galactosyltransferase, suggesting that glycosylation of specific proteins or lipids could be important for signaling in the switch to polarized growth and in bud emergence.T HE ellipsoidal shape of the yeast Saccharomyces cerevisiae reflects cell cycle-regulated polarized growth. At specific times during the cell cycle, cell growth is either isotropic or polarized toward the bud (for review see Lew and Reed, 1995b). A correlation between local deposition of new cell wall components and actin localization has been established (Adams and Pringle, 1984;Kilmartin and Adams, 1984), leading to the proposal that actin directs secretory vesicles to specific regions of the plasma membrane to allow localized cell surface growth during bud initiation and bud growth. During most of the G1 phase, growth is isotropic and cortical actin patches are delocalized throughout the cell. The attainment of a critical cell size and concomitant execution of START lead to the formation of an actin ring at the pre-bud site and the orientation of actin filaments toward this site. Subsequent to START, growth is almost completely restricted to the emerging bud. During bud growth, cortical actin patches are localized to the bud. Initially, bud growth occurs primarily at the distal tip. At some point, though, there is a switch to isotropic growth first in the bud, then also tranAddress all correspondence to S. I. Reed, Department of Molecular Biology, MB7, The Scripps Research Institute, 10666 North Torrey Pines Road, La Jolla, California 92037. Tel.: (619) 554-6188. siently in the mother cell at mitosis. At cytokinesis, the actin cytoskeleton is reorganized and...

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“…Immunoelectron microscopy indicated that at least some of the actin patches represent coils of actin filaments surrounding membrane invaginations (Mulholland et al, 1994). These structures might anchor the cytoskeleton to the plasma membrane.…”

Section: Saccharomyces Cerevisiaementioning

confidence: 99%

Interdependence of Filamentous Actin and Microtubules for Asymmetric Cell Division

Schaerer-Brodbeck¹,

Riezman²

2000

Biological Chemistry

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Asymmetric cell divisions are crucial to the generation of cell fate diversity. They contribute to unequal distribution of cellular factors to the daughter cells. Asymmetric divisions are characterized by a 90º rotation of the mitotic spindle. There is increasing evidence that a tight cooperation between cortical, filamentous actin and astral microtubules is indispensable for successful spindle rotation. Over the past years, the dynactin complex has emerged as a key candidate to mediate actin/microtubule interaction at the cortex. This review discusses our current understanding of how spindle rotation is accomplished by the interplay of filamentous actin and microtubules in a variety of experimental systems.

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Ultrastructure of the yeast actin cytoskeleton and its association with the plasma membrane.

Cited by 347 publications

References 32 publications

Actin and Septin Ultrastructures at the Budding Yeast Cell Cortex

Actin and Septin Ultrastructures at the Budding Yeast Cell Cortex

BED1, a gene encoding a galactosyltransferase homologue, is required for polarized growth and efficient bud emergence in Saccharomyces cerevisiae.

Interdependence of Filamentous Actin and Microtubules for Asymmetric Cell Division

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