MIKA, LEONARD A. (U. S. Army Chemical Corps, Frederick, Md.), and JAMES B. PIRSCH. Replication of variola virus in suspended cultures of mammalian cells. Appl. Microbiol. 9:545-548. 1961.-The studies reported here describe the successful propagation of variola virus in spinner cultures of mammalian cells, and the factors which influence its growth. Five established cell lines were used for the propagation of variola virus in a spinner culture system. Low doses of virus did initiate an infection but virus yields did not approach those obtained when an intermediate inoculum was used. Although the nonviable cell population remained low during the course of infection with an intermediate amount of virus, with an inoculum of 105 infectious units per ml or higher, the percentage of nonviable cells increased rapidly and by the sixth day after infection the population was totally nonviable. Intracellular replication of variola virus occurred early and rapidly in a spinner culture of guinea pig lung cells, whereas the liberation of virus into the suspending medium was a more gradual process. Several complete medium changes tend to maintain a suitable environment for the infected cell culture resulting in fairly high and constant viral titers over a period of 7 days. The propagation of variola virus in monolayer cultures of various tissue cells has been investigated by
The studies reported here describe the successful propagation of variola virus in spinner cultures of mammalian cells, and the factors which influence its growth. Five established cell lines were used for the propagation of variola virus in a spinner culture system. Low doses of virus did initiate an infection but virus yields did not approach those obtained when an intermediate inoculum was used. Although the nonviable cell population remained low during the course of infection with an intermediate amount of virus, with an inoculum of 10
5
infectious units per ml or higher, the percentage of nonviable cells increased rapidly and by the sixth day after infection the population was totally nonviable. Intracellular replication of variola virus occurred early and rapidly in a spinner culture of guinea pig lung cells, whereas the liberation of virus into the suspending medium was a more gradual process. Several complete medium changes tend to maintain a suitable environment for the infected cell culture resulting in fairly high and constant viral titers over a period of 7 days.
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