J Gen Virol 48 (1980), 341-350; DOI 10.1099/0022-1317-48-2-341
© 1980 Society for General Microbiology
Quantification of Newly Synthesized Virus RNA in Moloney Murine Leukaemia Virus-infected Cells
Naomi Guttman-Bass,
Howard Cedar and
Amos Panet
Departments of Virology and Molecular Biology, The Hebrew University-Hadassah Medical School, Jerusalem, Israel
A technique for the isolation and characterization of newly transcribed murine leukaemia virus RNA in chronically infected cells has been developed. Cellular RNA was pulse labelled with 3H-uridine and virus-specific sequences were annealed with an excess of mercurated complementary DNA. Based on the affinity between mercurated cDNA and sulphydryl-Sepharose, the hybrid was specifically selected by affinity column chromatography. The specificity of this method was dependent on the purity of the cDNA and it was necessary to remove non-viral sequences from the cDNA in order to isolate virus-specific RNA. Between 0.5 and 0.8% of the labelled RNA in Moloney MuLV-infected rat cells and 1.5% of the labelled RNA in Moloney MuLV-infected NIH Swiss mouse cells were virus-specific. Using this methodology, the effect of the cell cycle on the transcriptional activity of proviral genes was investigated. Cultures of Moloney MuLV-infected rat cells arrested in G0 phase of the cell cycle released reduced quantities of virus, but continued to synthesize virus RNA. The pools of virus RNA and p30 antigen in the G0-arrested cells equalled the pools in actively dividing cells. These results suggested that post-transcriptional events controlled virus production in the G0-arrested cells.
Received 25 October 1979;
accepted 10 January 1980.
Copyright © 1980 by the Society for General Microbiology.
