Lois Fanshier scite author profile

Cells producing Rous sarcoma virus contain virus-specific ribonucleic acid (RNA) which can be identified by hybridization to single-stranded deoxyribonucleic acid (DNA) synthesized with RNA-directed DNA polymerase. Hybridization was detected by either fractionation on hydroxyapatite or hydrolysis with single strand-specific nucleases. Similar results were obtained with both procedures. The hybrids formed between enzymatically synthesized DNA and viral RNA have a high order of thermal stability, with only minor evidence of mismatched nucleotide sequences. Virus-specific RNA is present in both nuclei and cytoplasm of infected cells. This RNA is remarkably heterogeneous in size, including molecules which are probably restricted to the nucleus and which sediment in their native state more rapidly than the viral genome. The nature of the RNA found in cytoplasmic fractions varies from preparation to preparation, but heterogeneous RNA (ca. 4-50S), smaller than the viral genome, is always present in substantial amounts. MATERIALS AND METHODS Materials. The sources of most reagents have been described (13, 15). Conidia of N. crassa were purchased from Miles Laboratories, Inc.; dimethylsulfoxide from Matheson, Coleman and Bell; Takadiastase (Sanzyme) was a gift from Sankyo Ltd., Tokyo, Japan. Diastase powder obtained from Sigma also contains S-1 nuclease, but the data in the present communication pertain only to the Sankyo material. All cell cultures were prepared from embryos known to be free from carrier infection with avian leukosis virus (embryonated eggs obtained from Kimber Farms, Berkeley, Calif.). Electrophoretically purified deoxyribonuclease was purchased from Worthington Biochemicals and treated with iodoacetate by the method of Zimmerman and Sandeen (34) to inactivate traces of contaminating ribonuclease. The alkylated preparations were tested for ribonuclease with 32p_ labeled 70S RSV RNA, which was denatured (11, 12) after exposure to the enzyme and was analyzed by rate-zonal centrifugation. 891

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The low molecular weight RNAs of Rous sarcoma virus

Bishop

et al. 1970

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Identification of nucleotide sequences which may encode the oncogenic capacity of avian retrovirus MC29

Sheiness¹,

Fanshier²,

Bishop³

1978

J Virol

136

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The retrovirus strain MC29 induces a variety of tumors in chickens, including myelocytomatosis and carcinomas of the kidney and liver. In addition, the virus can transform cultures of embryonic avian macrophages and fibroblasts. We have characterized the genome of MC29 virus and have identified nucleotide sequences that may encode the oncogenic potential of the virus. MC29 virus can replicate only with the assistance of a related helper virus. The defect in replication is apparently a consequence of a deletion in one or more viral genes: the haploid genome of the MC29 virus has a molecular weight of ca. 1.7 x 106, whereas the genome of the helper virus MCAV has a molecular weight of ca. 3.1 x 106. Although MC29 virus transforms fibroblasts in culture, its genome has no detectable homology with the gene src that is responsible for transformation of fibroblasts by avian sarcoma viruses. We prepared radioactive single-stranded DNA complementary to nucleotide sequences present in the genome of MC29 virus but not in the genome of MCAV (cDNAMc29). If they are contiguous, these sequences (ca. 1,500 nucleotides) are sufficiently complex to encode at least one protein. Homologous sequences were not detectable in several strains of avian sarcoma viruses or in an endogenous virus of chickens. Our findings confirm and extend recent reports from other laboratories and lead to the conclusion that MC29 virus may contain a previously unidentified gene(s) that is capable of transforming several distinct target cells. The evolutionary origins of this putative gene and its location on the viral genome can be explored with cDNAMC29.

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Deoxyribonucleic Acid Polymerase Associated with Rous Sarcoma Virus and Avian Myeloblastosis Virus: Properties of the Enzyme and Its Product

Garapin

McDonnell

Levinson

et al. 1970

J Virol

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Deoxyribonucleic acid (DNA) polymerase activity can be elicited in purified preparations of avian myeloblastosis virus and Rous sarcoma virus (Schmidt-Ruppin strain) by treatment with nonionic detergent. The enzyme(s) and its synthetic products appear to be virion-associated. Enzymatic activity can be inhibited by pretreatment with either ribonuclease (8to 10-fold inhibition) or actinomycin D (twofold inhibition). By contrast, rifampin has little, if any effect. The enzyme(s) synthesizes two primary products, a ribonucleic acid (RNA): DNA hybrid and DNA which is free of RNA. The results of both zonal and equilibrium centrifugation indicate that nascent chains of DNA are associated with the 70S viral RNA. It is concluded that at least two enzymatic activities are under study: transcription of DNA from viral RNA, and subsequent, additional synthesis of DNA, utilizing product of the initial reaction as template.

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Tolerance and immunity in chickens after congenital and contact infection with an avian leukosis virus

et al. 1962

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Lois Fanshier

Virus-Specific Ribonucleic Acid in Cells Producing Rous Sarcoma Virus: Detection and Characterization

The low molecular weight RNAs of Rous sarcoma virus

Identification of nucleotide sequences which may encode the oncogenic capacity of avian retrovirus MC29

Deoxyribonucleic Acid Polymerase Associated with Rous Sarcoma Virus and Avian Myeloblastosis Virus: Properties of the Enzyme and Its Product

Tolerance and immunity in chickens after congenital and contact infection with an avian leukosis virus

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