Your search keyword '"Rush DF"' showing total 3 results

1. Cyclin B1 expression in HeLa S3 cells studied by flow cytometry.

Author

Sherwood SW, Rush DF, Kung AL, and Schimke RT

Subjects

Aphidicolin pharmacology, Cell Cycle genetics, Cell Cycle physiology, DNA genetics, DNA metabolism, Demecolcine pharmacology, Flow Cytometry, Gene Expression, HeLa Cells, Humans, Cyclins genetics, Cyclins metabolism

Abstract

Using a procedure to stain cells simultaneously for cyclin B1 protein and DNA, we have examined cyclin B1 expression by flow cytometry in human cells under a variety of perturbing and nonperturbing conditions. The method described is useful for measuring relative differences in cyclin B level (immunochemically detectable epitope) as a function of cell cycle position on an individual cell basis and thus to examine cell cycle-related changes in cyclin B expression without prior cell synchronization. We show that in HeLaS3 cells, cyclin B1 accumulates in cells only after they become 4C and have resided in G2 for a short period of time. During colcemid-induced mitotic arrest cyclin B1 continues to accumulate in HeLa S3 cells, and under specific conditions of aphidicolin-induced unbalanced cell growth induced, cyclin B accumulates to supranormal levels prior to mitosis. Flow cytometric analysis of cyclin B expression and DNA content permits detailed examination of the effects of cell cycle perturbations on cyclin B expression under a variety of conditions.

Published

1994

2. Differences in mitotic control among mammalian cells.

Author

Schimke RT, Kung AL, Rush DF, and Sherwood SW

Subjects

Animals, Antineoplastic Agents pharmacology, Aphidicolin pharmacology, Cell Cycle drug effects, Cell Cycle physiology, Cell Cycle radiation effects, Cell Line, DNA biosynthesis, Demecolcine pharmacology, Drug Resistance, Gamma Rays, Gene Amplification, Humans, Mitosis drug effects, Mitosis radiation effects, Neoplasms genetics, Mitosis physiology

Published

1991

3. Morphology of dissociated hippocampal cultures from fetal mice.

Author

Peacock JH, Rush DF, and Mathers LH

Subjects

Action Potentials, Age Factors, Animals, Axons ultrastructure, Cell Differentiation, Cell Survival, Cells, Cultured, Dendrites physiology, Dendrites ultrastructure, Hippocampus physiology, Mice, Neurons cytology, Neurons physiology, Synapses ultrastructure, Hippocampus cytology

Abstract

Dissociated hippocampal cultures from fetal mice (13--18 days gestational age) can be maintained for up to two months in culture. Cells grow as either isolated neurons or in small neuronal aggregates. Neurons remain small with a soma diameter of 15--20 micrometer even in mature cultures and develop extensively branched processes during the first two weeks in culture. After this time, processes become more difficult to visualize with phase-contrast optics because of a tendency to grow within the underlying non-neuronal cells. However, the presence of processes has been proved by silver-staining which demonstrates an organizational complexity ranging from a loosely reticulated neuropil to fascicles containing many fibers. More detailed study of individual neuronal morphology was carried out in cells filled with the fluorescent dye, Lucifer Yellow CH, in conjunction with the intracellular recording of synaptic and action potentials from dye-containing micropipettes. Dye-filled cells show a well-developed branching morphology. Process specializations include spines, beading, and basket-like endings. Processes tend to emanate from one side of the soma, either originating at the cell body or from a single trunk. Commonly there are 2--4 orders of branching, but up to 6 orders can occur (counted centrifugally from the soma). Electron microscopy revealed synapses distributed predominantly on dendrites with a smaller number on somata. Dendritic spines are present and are contacted principally by asymmetric synaptic junctions. Symmetric synapses are relatively more common on somata and proximal dendrites.

Published

1979