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Open AccessJournal ArticleDOI

Cytoplasmic filaments of Amoeba proteus. I. The role of filaments in consistency changes and movement.

Thomas D. Pollard, +1 more
- 01 Aug 1970 - 
- Vol. 46, Iss: 2, pp 267-289
TLDR
The role of filaments in consistency changes and movement in a motile cytoplasmic extract of Amoeba proteus was investigated by correlating light and electron microscopic observations with viscosity measurements and the structural relationship of the 70 A and the 160 A Filaments in the motile extract suggest that both types of Filaments may be required for movement.
Abstract
The role of filaments in consistency changes and movement in a motile cytoplasmic extract of Amoeba proteus was investigated by correlating light and electron microscopic observations with viscosity measurements. The extract is prepared by the method of Thompson and Wolpert (1963). At 0°C, this extract is nonmotile and similar in structure to ameba cytoplasm, consisting of groundplasm, vesicles, mitochondria, and a few 160 A filaments. The extract undergoes striking ATP-stimulated streaming when warmed to 22°C. Two phases of movement are distinguished. During the first phase, the apparent viscosity usually increases and numerous 50–70 A filaments appear in samples of the extract prepared for electron microscopy, suggesting that the increase in viscosity in caused, at least in part, by the formation of these thin filaments. During this initial phase of ATP-stimulated movement, these thin filaments are not detectable by phase-contrast or polarization microscopy, but later, in the second phase of movement, 70 A filaments aggregate to form birefringent microscopic fibrils. A preparation of pure groundplasm with no 160 A filaments or membranous organelles exhibits little or no ATP-stimulated movement, but 50–70 A filaments form and aggregate into birefringent fibrils. This observation and the structural relationship of the 70 A and the 160 A filaments in the motile extract suggest that both types of filaments may be required for movement. These two types of filaments, 50–70 A and 160 A, are also present in the cytoplasm of intact amebas. Fixed cells could not be used to study the distribution of these filaments during natural ameboid movement because of difficulties in preserving the normal structure of the ameba during preparation for electron microscopy.

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Presence of modified fibroblasts in granulation tissue and their possible role in wound contraction.

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Actin and myosin and cell movement.

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Intracellular localization of messenger RNAs for cytoskeletal proteins

TL;DR: Actin mRNA distribution may result in increased concentration of actin filaments in lamellipodia of motile cells, demonstrating that cytoplasmic mRNAs are localized in specific, nonrandom cellular patterns and that localized concentrations of specific proteins may result from corresponding localization of their respective m RNAs.
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Isolation and properties of actin, myosin, and a new actinbinding protein in rabbit alveolar macrophages.

TL;DR: Actin, myosin, and a high molecular weight actin-binding protein were extracted from rabbit alveolar macrophages with low ionic strength sucrose solutions containing ATP, EDTA, and dithiothreitol and collected by ultracentrifugation.
References
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Journal ArticleDOI

A simplified lead citrate stain for use in electron microscopy.

TL;DR: This communication reports the use of a commercially available lead citratO to eliminate the lead citrate stain in electron microscopy.
Journal ArticleDOI

Formation of arrowhead complexes with heavy meromyosin in a variety of cell types.

TL;DR: The significance of HMM-filament binding is discussed in view of the finding that arrowhead complexes form in types of cells not usually thought to contain actin filaments.
Journal ArticleDOI

Cytoplasmic fibrils in living cultured cells. A light and electron microscope study.

TL;DR: In this paper, the structure and behavior of the stress fibers of cultured rat embryo cells are described by a combined light and electron microscopic study, and it is concluded that the filamentous structure shown within the cytoplasm of glutaraldehyde/osmium-fixed cells is a generally accurate representation of the structure of the living cell.
Journal ArticleDOI

Cytoplasmic microfilaments in streaming Nitella cells

TL;DR: The plant Nitella was selected for study with respect to the ultrastructural basis for rotational streaming, and the relationships of microfilaments in this material to similar structures in other materials is discussed.
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