Your search keyword '"Polynucleotide Ligases biosynthesis"' showing total 5 results

1. Activation of 2',5'-oligo(A) polymerase and protein kinase of interferon-treated HeLa cells by 2'-O-methylated poly (inosinic acid) . poly(cytidylic acid), Correlations with interferon-inducing activity.

Author

Minks MA, West DK, Benvin S, Greene JJ, Ts'o PO, and Baglioni C

Subjects

2',5'-Oligoadenylate Synthetase, Adenine Nucleotides biosynthesis, Adenosine Triphosphate metabolism, Enzyme Activation, HeLa Cells enzymology, Humans, Interferons biosynthesis, Methylation, Oligonucleotides biosynthesis, Oligoribonucleotides biosynthesis, Polynucleotide Adenylyltransferase metabolism, Protein Kinases metabolism, HeLa Cells drug effects, Interferons pharmacology, Poly I-C pharmacology, Polynucleotide Ligases biosynthesis, Protein Kinases biosynthesis

Abstract

An oligonucleotide polymerase and a protein kinase which require double-stranded RNA (dsRNA) for activation are induced in HeLa cells by human fibroblast interferon. The polymerase synthesizes a series of oligonucleotides from ATP, whereas the kinase phosphorylates a polypeptide of Mr = 72,000 and the alpha subunit of initiation factor eIF-2. Partially or fully 2'-O-methylated derivatives of poly(inosinic acid) . poly(cytidylic acid) (rIn . rCn) were used to determine the structural requirements of dsRNA in the activation of these two enzymes. While fully methylated polymers failed to activate either enzyme, partially methylated polymers activated the enzymes in specific manners. The activation of the kinase by the rIn . rCn analogues was affected more severely by the level of methylation than was the activation of the polymerase. Moreover, fully methylated analogues blocked the activation of the kinase by rIn . rCn but not the activation of the polymerase. These observations are consistent with a biphasic model for enzyme activation similar to that proposed for interferon induction, which required the recognition of a relatively small region of rIn . rCn as the last step. Differences in the activation of the polymerase and kinase are explicable on the basis of the polymerase requirement for a smaller recognition region of the rIn . rCn duplex than the kinase. Dependence of polymerase activation on the level of methylation shows striking similarities with the interferon inducing activities of these analogues, suggesting a possible relationship between polymerase activation and interferon induction.

Published

1980

2. Mechanism of pppA(2'p5'A)n2'p5'AOH synthesis in extracts of interferon-treated HeLa cells.

Author

Minks MA, Benvin S, and Baglioni C

Subjects

2',5'-Oligoadenylate Synthetase, Enzyme Induction, HeLa Cells drug effects, HeLa Cells enzymology, Humans, Kinetics, Nucleotides pharmacology, Adenine Nucleotides biosynthesis, Interferons pharmacology, Oligonucleotides biosynthesis, Oligoribonucleotides biosynthesis, Polynucleotide Ligases biosynthesis

Abstract

Treatment of HeLa cells with interferon results in the induction of an enzymatic activity designated 2'5'oligo(A) polymerase. The polymerase requires continuous presence of double-stranded RNA (dsRNA) for activity, since degradation of dsRNA abolishes synthesis of the oligomeric series pppA(2'p5'A)n. These oligonucleotides are formed initially at a constant rate with dimer synthesized faster than trimer, and the latter faster than tetramer. After 45 min, accumulation of the dimer declines whereas that of other oligomers still proceeds at a linear rate. These results suggest that an oligomer remains associated with the enzyme for possible consecutive additions of adenylate, since no significant accumulation of dimer precedes synthesis of trimer. The relative amounts of the different oligomers found at the end of a reaction may reflect an increasing probability of release as the oligomers are elongated. The accumulation of dimer, however, decreases when it becomes a substrate for adenylate addition; incorporation of isolated dimer into 2'5'-oligo(A) was directly shown. Other nucleotides with a blocked p5'A terminus, like A5'ppppp5'A and NADH, can serve as adenylate acceptors in the presence of dsRNA. The adenosine triphosphates 2'-dATP and 3'-dATP are not incorporated efficiently into 2'5'-oligo(A) and inhibit its synthesis.

Published

1980

3. Mechanisms of action of human interferons. Induction of 2'5'-oligo(A) polymerase.

Author

Baglioni C and Maroney PA

Subjects

2',5'-Oligoadenylate Synthetase, Adenine Nucleotides biosynthesis, Cycloheximide pharmacology, Dactinomycin pharmacology, Deoxyadenosines pharmacology, Enzyme Induction, HeLa Cells drug effects, HeLa Cells enzymology, Humans, Kinetics, Leukocytes, Oligoribonucleotides biosynthesis, Interferons pharmacology, Polynucleotide Ligases biosynthesis

Abstract

Interferons induce an enzymatic activity that polymerizes ATP into 2'5'-oligoadenylate. This enzyme, designated 2'5'-oligo(A) polymerase, is induced in HeLa cells by type I interferon with a faster kinetics than by type II (immune) interferon. Cells treated with type I interferon in the presence of cycloheximide show elevated levels of polymerase when the inhibitor or protein synthesis is removed and actinomycin D is added to the cultures to prevent further synthesis of mRNA. This suggests that, in the presence of cycloheximide, interferon can activate transcription of mRNA for the 2'5'-oligo(A) polymerase, which is subsequently translated upon removal of this inhibitor. In contrast, cells treated with type II interferon in the same way do not show increased levels of polymerase. This indicates that type II interferon cannot activate transcription of a stable mRNA for the polymerase when protein synthesis is inhibited. This observation and the different kinetics of induction of 2'5'-oligo(A) polymerase suggest major differences in the mechanism of action of the different types of interferon, with type I being a "direct" inducer of the polymerase and type II an "indirect" inducer. The commitment of HeLa cells to the induction of 2'5'-oligo(A) polymerase declines if the cells are exposed to type I interferon in the presence of an inhibitor of RNA synthesis. This suggests that transcription of specific mRNAs is transiently activated by interferon and that repeated interaction of interferon with its receptor may be required for prolonged transcription of the mRNA for 2'5'-oligo(A) polymerase.

Published

1980

4. Covalent attachment of polyribonucleotides to polydeoxyribonucleotides catalyzed by deoxyribonucleic acid ligase.

Author

Nath K and Hurwitz J

Subjects

Adenine Nucleotides metabolism, Adenosine Monophosphate metabolism, Alkaline Phosphatase, DNA metabolism, DNA Viruses, Exonucleases metabolism, Kinetics, Phosphorus Radioisotopes, Poly U metabolism, Polynucleotide Ligases biosynthesis, Polynucleotides metabolism, RNA metabolism, Structure-Activity Relationship, Templates, Genetic, Thymine Nucleotides pharmacology, Tritium, Uracil Nucleotides metabolism, Coliphages enzymology, Deoxyribonucleotides metabolism, Escherichia coli enzymology, Polynucleotide Ligases metabolism, Ribonucleotides metabolism

Published

1974

5. Biosynthesis of mammalian DNA ligase.

Author

Teraoka H and Tsukada K

Subjects

Animals, Carcinoma, Ehrlich Tumor enzymology, Cattle, DNA Ligases isolation & purification, Electrophoresis, Polyacrylamide Gel, Fluorometry, Half-Life, Molecular Weight, Rabbits, Thymus Gland enzymology, DNA Ligases biosynthesis, Polynucleotide Ligases biosynthesis

Abstract

A monospecific antibody against calf thymus DNA ligase composed of a single polypeptide with Mr = 130,000 cross-reacts with rodent and calf thymus DNA ligases. The antibody precipitates a single Mr = 200,000 polypeptide from detergent lysates of [3H] leucine-labeled mouse Ehrlich tumor cells and calf thymocytes. Pulse-chase experiments show that the Mr = 200,000 polypeptide in Ehrlich tumor cells has a half-life of about 0.5 h. In addition to the Mr = 200,000 polypeptide, a Mr = 130,000 polypeptide is detected in the partially purified enzyme preparations from radiolabeled Ehrlich tumor cells. These results suggest that DNA ligase is synthesized in mammalian cells as a Mr = 200,000 polypeptide and that the Mr = 200,000 polypeptide is degraded to a Mr = 130,000 polypeptide by a limited proteolysis in vitro.

Published

1985