E Edelstein scite author profile

E Edelstein

3Publications

8Citation Statements Received

27Citation Statements Given

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Temple University, Westchester Institute for Human Development

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Unit Cell Hypothesis for Streptococcus faecalis

et al. 1980

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The mass doubling times of exponential-phase cultures of Streptococcus faecalis were varied from 30 to 110 min by omitting glutamine from a defined growth medium and providing different concentrations of glutamate (ranging from 300 to 14 ,Ig/ml). After Formalin fixation, cells were dried by the critical point method, and carbon-platinum replicas were prepared. The surface area and volume of cell poles seen in these replicas were estimated by a computer-assisted, three-dimensional reconstruction technique. It was found that the amount of surface area and volume of poles seen in these replicas were independent of the growth rate of culture from which the samples were taken. These observations were consistent with the unit cell model hypothesis of Donachie and Begg, in which a small number of surface sites would produce a constant amount of new cell surface regardless of the mass doubling time of the culture. However, measurements of the thickness of the cell wall taken from thin sections of the same cells showed that the cell wall increased in thickness as a function of the increase in cellular peptidoglycan content which occurs when the growth rate of this organism is slowed down by a decrease in glutamate concentration. Thus, it would seem that although the size of polar shells made by S. faecalis is invariant with growth rate, the amount of wall precursors used to construct these shells is not. MATERIALS AND METHODSCell growth. Cells of S. faecalis ATCC 9790 were allowed to go through at least six mass doublings in a chemically defined medium (14) (reaching the equivalent of 100 ,ug of dry mass per ml) before being used for study. Mass doubling times (TD) between 30 and 110 min were obtained by removing glutamine and providing a range of concentrations of glutamate (between 300 and 14 ug) (16). Electron microscopy. Formaldehyde prepared from the hydrolysis of paraformaldehyde was added 499 on August 1, 2020 by guest http://jb.asm.org/ Downloaded from 500 EDELSTEIN ET AL.

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Nucleoid structure in freeze fractures of Streptococcus faecalis: effects of filtration and chilling

Edelstein¹,

Parks²,

Tsien³

et al. 1981

J Bacteriol

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With the techniques used in this study, the nucleoid of Streptococcus faecalis could not be seen in freeze-etch preparations unless glutaraldehyde had been added to cultures of cells before they were frozen. With time, the nucleoid became visible as a network of fibers, apparently as a result ofthe aggregation of individual chromosomal elements in the presence of glutaraldehyde. When glutaraldehyde was added to undisturbed cultures, the fibers that became visible were observed in small patches that were seemingly scattered throughout the cytoplasm. However, if cells were chilled or placed on filters before glutaraldehyde was added, the fibers which then developed were seen in large central areas. The appearance of centralized nucleoids in freeze fractures of cells that had been chilled or filtered could be correlated with a decrease in the central density of the cytoplasm, as seen by light microscopy, in cells embedded in gelatin or bovine serum albumin. These observations are discussed in relation to a model for the normal structure of the nucleoid which suggests that the treatments routinely used to study the morphology-physiology of cells (chilling, filtration, and fixation) result in a reorganization of the cytoplasm, leading to an increase in the centralization of nuclear material.

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Studies on the inhibition of muscular activity in the presence of urea

Bárány

Edelstein

et al. 1965

Pfl�gers Archiv

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E Edelstein

Unit Cell Hypothesis for Streptococcus faecalis

Nucleoid structure in freeze fractures of Streptococcus faecalis: effects of filtration and chilling

Studies on the inhibition of muscular activity in the presence of urea

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