Anna Baros scite author profile

SUMMARYEscherichia coli B[r (su °) was infected, at 30 °C, with T4Dam +, , and T4DamNx34amBL292 (33-, 55-, maturation-defective phenotype). A genetic (' transformation') assay was used to monitor transcription of genes 30 (polynucleotide ligase), 42 (deoxycytidylate hydroxymethylase), 43 (DNA polymerase), rlIA, rlIB, and e (endolysin). The principal results are: (t) All of the genes studied were transcribed exclusively from the so-called/-strand of phage DNA. (2) DNA synthesis and the maturation-defective proteins were required to turn-off transcription of genes 42, rIIA, tIIB, and 43.

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Effect of chloramphenicol and starvation for an essential amino acid on polypeptide and polyribonucleotide synthesis in Escherichia coli infected with bacteriophage T4

Witmer

Baros

Forbes

1975

Archives of Biochemistry and Biophysics

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Control of synthesis of mRNA's for T4 bacteriophage-specific dihydrofolate reductase and deoxycytidylate hydroxymethylase

Witmer¹,

Baros²,

Ende³

et al. 1976

J Virol

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A 300C, functional messengers for dCMP hydroxymethylase first appeared 3 to 6 min postinfection and reached their maximum levels at 12 min. Chloramphenicol, added before the phage, reduced the rate of mRNA accumulation. When the antibiotic was added 6 min postinfection, mRNA levels increased at their normal rate but there was no obvious repression of messenger accumulation. Delaying the addition of drug until 8 or 12 min had progressively less effect on the pattern of hydroxymethylase mRNA metabolism. When chloramphenicol was present from preinfection times or from 6 min postinfection, all hydroxymethylase mRNA's synthesized were stable; at later times, however, the ability of the drug to stabilize mRNA decreased with its ability to delay the turnoff of mRNA production. An overaccumulation of hydroxymethylase mRNA was also seen when phage-specific DNA synthesis was inhibited either by mutational lesion in an essential viral gene or by 5-fluorodeoxyuridine. By min 20 of a DNA-negative program, hydroxymethylase mRNA synthesis was repressed to the point where it no longer compensated for decay. However, a finite level of hydroxymethylase mRNA synthesis was maintained at later times of a DNA-negative infection. Such results indicate that replication of the phage chromosome is necessary but not sufficient for a complete turnoff of hydroxymethylase mRNA production. Functions controlled by the maturation-defective proteins (the products of genes 55 and 33) played only a minor role in the regulation of hydroxymethylase mRNA metabolism. Thus, we favor the hypothesis that a complete turnoff of hydroxymethylase messenger production requires one or more new proteins as well as an interval of DNA replication. The absence of DNA synthesis had no particular effect upon dihydrofolate reductase messenger production. The preinfection addition of chloramphenicol likewise had little effect on dihydrofolate reductase messenger metabolism. These latter data imply that prior synthesis of a phage-coded protein synthesis may not be required for the turnoff of reductase messenger production.

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Anna Baros

Effect of chloramphenicol and starvation for an essential amino acid on the synthesis and decay of T4 bacteriophage-specific messengers transcribed from early and quasi-late promoters

Transcriptional Control of T4 Coliphage-Specific Genes 30, 42, 43, rIIA, rIIB, and e

Effect of chloramphenicol and starvation for an essential amino acid on polypeptide and polyribonucleotide synthesis in Escherichia coli infected with bacteriophage T4

Control of synthesis of mRNA's for T4 bacteriophage-specific dihydrofolate reductase and deoxycytidylate hydroxymethylase

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