Transient inhibition of DNA synthesis results in increased dihydrofolate reductase synthesis and subsequent increased DNA content per cell

Author:

Johnston R N,Feder J,Hill A B,Sherwood S W,Schimke R T

Abstract

We examined the role that blockage of cells in the cell cycle may play in the stimulation of gene amplification and enhancement of drug resistance. We found that several different inhibitors of DNA synthesis, which were each able to block cells at the G1-S-phase boundary, induced an enhanced cycloheximide-sensitive synthesis of an early S-phase cell cycle-regulated enzyme, dihydrofolate reductase, and of other proteins as well. This response was specific, in that blockage at the G2 phase did not result in overproduction of the enzyme. When the cells were released from drug inhibition, DNA synthesis resumed, resulting in a cycloheximide-sensitive elevation in DNA content per cell. We speculate that the excess DNA synthesis (which could contribute to events detectable later as gene amplification) is a consequence of the accumulation of S-phase-specific proteins in the affected cells, which may then secondarily influence the pattern of DNA replication.

Publisher

American Society for Microbiology

Subject

Cell Biology,Molecular Biology

Reference27 articles.

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2. Phenotypic expression in E. coli of a DNA sequence coding for mouse dihydrofolate reductase;Chang A. C. Y.;Nature (London),1978

3. Effect of methotrexate on dihydrofolate reductase activity in methotrexate-resistant human KB cells;Domin B. A.;Mol. Pharmacol.,1982

4. Transcription factor Spl recognizes a DNA sequence in the mouse dihydrofolate reductase promoter;Dynan W. S.;Nature (London),1986

5. Transcriptional regulation of mouse dihydrofolate reductase in the cell cycle;Farnham P. J.;J. Biol. Chem.,1985

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