Transforming Sloan-Kettering viruses generated from the cloned v-ski oncogene by in vitro and in vivo recombinations Journal Article
| Authors: | Stavnezer, D.; Barkas, A. E.; Brennan, L. A.; Brodeur, D.; Li, Y. |
| Article Title: | Transforming Sloan-Kettering viruses generated from the cloned v-ski oncogene by in vitro and in vivo recombinations |
| Abstract: | The Sloan-Kettering viruses (SKVs) are replication-defective retroviruses that transform avian cells in vitro. Each of the three SKV isolates is a mixture of viruses with genomes ranging in size from 4.1 to 8.9 kilobases (kb) with a predominant genome of 5.7 kb. Using a cDNA representing a sequence, v-ski, that is SKV specific and held in common by the multiple SKV genomes, we generated a restriction map of the 5.7-kb SKV genome and molecularly cloned a ski-containing fragment from SKV proviral DNA. Southern hybridization and sequence analysis showed that the cloned DNA fragment consisted of the 1.3-kb ski sequence embedded in the p19(gag) sequence and followed by the remaining 5' half of the gag gene and small portions of both the pol and env genes. A large deletion encompassing the 3' half of gag and the 5' 80% of pol was mapped to a position about 1 kb downstream from the 3' ski-gag junction. To determine whether the cloned ski sequence had transforming activity, the ski-containing fragment and a cloned Rous-associated virus 1 (RAV-1) genome were used to construct an analog of the 5.7-kb SKV genome, RAV-SKV. Cotransfection of chicken embryo cells with RAV-SKV and RAV-1 yielded foci of transformed cells whose morphology was identical to that induced by the natural SKVs. The transformed transfected cells produced transforming virus with a 5.7-kb ski-containing genome and synthesized a gag-containing polyprotein of 110 kilodaltons (kDa). Several nonproducer clones of RAV-SKV-transformed cells were analyzed, and most were found to synthesize a 5.7-kb SKV RNA and a 110-kDa polyprotein. One clone was found to contain an 8.9-kb SKV RNA, and this clone synthesized a 125-kDa polyprotein. Since both the 5.7- and 8.9-kb genomes and the 110- and 125-kDa polyproteins had been identified in studies on the natural SKVs, the present results not only demonstrate the transforming activity of these individual SKVs but also suggest mechanisms for their generation. |
| Keywords: | nonhuman; animals; heredity; embryo; in vitro study; transfection; avian leukosis virus; oncogenes; cloning, molecular; gene mapping; oncogene; genetic engineering; cell culture; recombination, genetic; base sequence; dna, viral; radioisotope; rna, viral; retrovirus; retroviridae; chick embryo; chicken; oncogene proteins, viral; gene products, gag; genes, viral; dna transfection; priority journal; virus cell transformation; retroviridae proteins; restriction fragment |
| Journal Title: | Journal of Virology |
| Volume: | 57 |
| Issue: | 3 |
| ISSN: | 0022-538X |
| Publisher: | American Society for Microbiology |
| Date Published: | 1986-03-01 |
| Start Page: | 1073 |
| End Page: | 1083 |
| Language: | English |
| PUBMED: | 3005612 |
| PROVIDER: | scopus |
| PMCID: | PMC252841 |
| DOI: | 10.1128/JVI.57.3.1073-1083.1986 |
| DOI/URL: | |
| Notes: | Article -- Export Date: 18 August 2021 -- Source: Scopus |
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