Ribonucleic acids of Machupo and Lassa viruses

Abstract

Sucrose gradient velocity centrifugation, polyacrylamide gel electrophoresis and RNA-RNA hybridization were used to characterize Lassa and Machupo virion RNAs as well as virus-specific RNAs from cells infected with Pichinde and Machupo viruses. Five RNA species: 30–31S, 28S, 22–24S, 18S and 4–6S have been detected in Lassa, Machupo, and Pichinde virion RNAs. Among them 28S, 18S and 4–6S RNAs cosediment and comigrate with respectivelv cell RNAs. RNase resistance analyses suggest the presence of extensive secondary structures and complementary RNAs in Lassa, Machupo, and Pichinde virion RNAs. Annealing with poly(A)-containing RNA from infected cells has revealed that the bulk of “minus” strands of Machupo virion RNA is located in 22–24S and 28–31S fractions of sucrose gradient. Thus Machupo and Lassa viruses as well as Pichinde virus contain two genomic RNA fragments: “large” (molecular weight of about 2.2 × 10⁶) and “small” (molecular weight of about 1.3 × 10⁶). In the cells infected with Pichinde virus and treated with actinomycin D (1.0 µg/ml) synthesis of 18S,22–24S and 30–31S RNAs has been registered. At least 22–24S and 30–31S classes comprise “plus” and “minus” strands. In cells infected with Machupo virus in the presence of actinomycin D the synthesis of similar sedimentation classes of RNAs and certain amounts of 28S RNA have been detected.