Translation of cucumber necrosis virus RNA in vitro
Johnston, Julie C. and Rochon, D’Ann M.,, 71, 2233-2241 (1990),
doi = https://doi.org/10.1099/0022-1317-71-10-2233,
publicationName = Microbiology Society,
issn = 0022-1317,
abstract= The in vitro translation products directed by cucumber necrosis virus (CNV) RNA were analysed in both rabbit reticulocyte lysate and wheatgerm extract cell-free translation systems. In rabbit reticulocyte lysates, one major protein of approximate M r 34·6K was produced. In wheatgerm extracts, four proteins of approximate Mr values 41·6K, 34·6K, 24K and 20K were produced. The genomic locations of the CNV in vitro translation products were determined using several experimental approaches including, first, hybrid-arrested translation using negative-sense RNA corresponding to selected regions of the CNV genome, second, in vitro translation of synthetic positive-sense CNV transcripts and third, in vitro translation of CNV virion RNA fractionated according to size. Together these experiments demonstrated that the protein of Mr 34·6K is derived from the 5′-proximal coding region, the 41·6K protein is derived from an internal coding region, and that at least one but probably both the 24K and 20K proteins are derived from the 3′-terminal coding region. In addition, immunoprecipitation of in vitro translation products using anti-CNV polyclonal serum demonstrated that the 41·6K protein is the coat protein. The templates for the expression of CNV cistrons were investigated by in vitro translation of sucrose gradient-fractionated CNV virion RNA as well as in vitro translation of positive-sense synthetic transcripts.,
language=,
type=