It is proposed that neoplastic cells differ from normal cells in several aspects of DNA synthesis. A long-range goal is to determine which aspects of DNA replication are altered in transformed cells in culture as compared with normal cells. DNA is not a static structure but undergoes continuous structural alterations, detected as breaks and single-strand nuclease-sensitive sites, as cells proceed through the cell cycle. DNA will be isolated from transformed fibroblasts and mutants temperature-sensitive for the transformed phenotype and examined for structural alterations in parental and replicative DNA of five subcompartments of the S-phase. Parental DNA of several subcompartments of G?1? also will be examined. G?2? DNA will be examined as a control. The interconversion of replicative intermediates, which differs in transformed and normal fibroblasts, will be examined in ts mutant cells at the permissive and nonpermissive temperatures. In contrast to frequent assumptions, the rate of DNA synthesis is not constant during the S-phase but fluctuates such that relative values of 30, 60, and 100% can occur. The fastest rates for HeLa and 2RA cells are at the beginning and end of S-phase, whereas WI-38 cells exhibit a gradual increase in rates from beginning to end of S-phase. It is proposed that single-stranded sites on DNA and the activities of DNA polymerases alpha, beta, and gamma of the single-strand specific chromatin-bound DNA polymerase and of DNA ligase are possible candidates for the factors that determine the observed variations in the rates of DNA synthesis as cells proceed through S. The measured enzyme activities will be correlated with quantitative rates of DNA synthesis determined with a flow cytometer in five S-phase compartments. (I)

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA024158-08
Application #
3166350
Study Section
Physiological Chemistry Study Section (PC)
Project Start
1978-08-01
Project End
1987-04-30
Budget Start
1986-02-01
Budget End
1987-04-30
Support Year
8
Fiscal Year
1986
Total Cost
Indirect Cost
Name
Virginia Commonwealth University
Department
Type
Overall Medical
DUNS #
City
Richmond
State
VA
Country
United States
Zip Code
23298
Collins, J M; Grogan, W M (1991) Comparisons of steady-state anisotropy of the plasma membrane of living cells with different probes. Biochim Biophys Acta 1067:171-6
Collins, J M; Grogan, W M (1991) Fluorescence quenching of a series of membrane probes measured in living cells by flow cytometry. Cytometry 12:247-51
Calderon, R O; Grogan, W M; Collins, J M (1991) Membrane structural dynamics of plasma membranes of living human prostatic carcinoma cells differing in metastatic potential. Exp Cell Res 196:192-7
Collins, J M; Dominey, R N; Grogan, W M (1990) Shape of the fluidity gradient in the plasma membrane of living HeLa cells. J Lipid Res 31:261-70
Collins, J M; Scott, R B; Grogan, W M (1990) Plasma membrane fluidity gradients of human peripheral blood leukocytes. J Cell Physiol 144:42-51
Collins, J M; Chu, A K (1990) Reduction of DNA primase activity in aging but still proliferating cells. J Cell Physiol 143:52-9
Collins, J M; Grogan, W M (1989) Comparison between flow cytometry and fluorometry for the kinetic measurement of membrane fluidity parameters. Cytometry 10:44-9
Collins, J M; Wood, S H; Chu, A K (1989) Nucleoids, a subnuclear system capable of chain elongation. Biochim Biophys Acta 1009:264-76
Collins, J M; Chu, A K (1987) Binding of the DNA polymerase alpha-DNA primase complex to the nuclear matrix in HeLa cells. Biochemistry 26:5600-7
Wood, S H; Collins, J M (1986) Preferential binding of DNA primase to the nuclear matrix in HeLa cells. J Biol Chem 261:7119-22

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