![Fig. 2. Analysis of viral parameters in parental U937 and resistant RU cells after H-1 virus infection. (A) The survival of U937 and RU cells was determined by counting viable cells 4 days after infection with H-1 virus (MOI = 100 pfu/cell), using the Trypan blue exclusion method, and expressed as a percentage of the value measured in mock-infected cultures. Results from a typical experiment are shown. (B) Infectious particles recovered 48 hours after inoculation of 106 cells with H-1 virus (5 pfu/cell) were measured by plaque-assay. Data shown are from a typical experiment. Similar relative values were obtained in three independent experiments (SD < 22%). (C) The virus uptake was assayed after infection with [3H]thymidine-labeled H-1 virus (2 × 103 pfu [105 cpm]/106 cells), followed by a washing step with 1 mmol/L EDTA to remove noninternalized particles (upper part). Internalized [35S]methionine-labeled capsids were revealed by autoradiography after immunoprecipitation and SDS-PAGE analysis of VP1 and VP2 proteins extracted 2 hours after infection with H-1 virus (4 × 106 pfu [106 cpm]/106 cell) and washing with EDTA (lower part). (D) Amplification of viral DNA was determined by Southern blotting. After virus (10 pfu/cell) or mock infection, cultures were incubated for 40 hours in complete medium. DNA samples extracted by the Hirt procedure were analyzed by agarose gel electrophoresis, blotted, and hybridized with a virus-specific 32P-labeled DNA probe. RFI and RFII refer to viral DNA replicative forms of monomer and dimer length, respectively. Viral DNA species were positioned relative to HindIII-digested phage λ DNA used as size markers and revealed by ethidium bromide staining. (E) The viral transcripts were detected by Northern blotting. At 48 hours postinfection (10 pfu/cell), total RNA was isolated by the guanidinium thiocyanate method, fractionated by agarose/formaldehyde gel electrophoresis, blotted, and hybridized with a virus-specific 32P-labeled DNA probe. (F ) The accumulation of viral proteins was determined by immunoprecipitation. At 36 hours postinfection (5 pfu/cell) cultures were incubated for 2 hours in the presence of [35S]methionine and processed for immunoprecipitation with antiserums directed against the viral products NS-1 or VP-1 and VP-2, SDS-PAGE, and autoradiography.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/89/5/10.1182_blood.v89.5.1642/3/bl_0021f2a.jpeg?Expires=1724241507&Signature=Ek115C1v5spMKqBbEEKylPx41P6F3W9VAAwZTcZsE39WpvpPNNeySslKptOz97lYZmCVNYsYSaceH5NTONstYPNGizipm2o~aN-GRBDMA5iQHOjfcffOmvPiqkiBnwdxWy4lGLuEMdgh89DYphhxzkUTjMyBKsHXSiVjdplaCt49-M0-tFfT38tJI1qUfMwNlplGm4srVC6cvU8esHrsT1cloDrav3JMqvp2qXwI-Oyug-xVjct4cGuTLy8dG3Lvu9vKkktTPwczKmaiDtHbmtbAKUwE1v86oeYjlp2SwG5J0Dj1n-p9izLY3Zrp6fBdpBlVMoAPe8op5hC~6YJ2zw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Analysis of viral parameters in parental U937 and resistant RU cells after H-1 virus infection. (A) The survival of U937 and RU cells was determined by counting viable cells 4 days after infection with H-1 virus (MOI = 100 pfu/cell), using the Trypan blue exclusion method, and expressed as a percentage of the value measured in mock-infected cultures. Results from a typical experiment are shown. (B) Infectious particles recovered 48 hours after inoculation of 106 cells with H-1 virus (5 pfu/cell) were measured by plaque-assay. Data shown are from a typical experiment. Similar relative values were obtained in three independent experiments (SD < 22%). (C) The virus uptake was assayed after infection with [3H]thymidine-labeled H-1 virus (2 × 103 pfu [105 cpm]/106 cells), followed by a washing step with 1 mmol/L EDTA to remove noninternalized particles (upper part). Internalized [35S]methionine-labeled capsids were revealed by autoradiography after immunoprecipitation and SDS-PAGE analysis of VP1 and VP2 proteins extracted 2 hours after infection with H-1 virus (4 × 106 pfu [106 cpm]/106 cell) and washing with EDTA (lower part). (D) Amplification of viral DNA was determined by Southern blotting. After virus (10 pfu/cell) or mock infection, cultures were incubated for 40 hours in complete medium. DNA samples extracted by the Hirt procedure were analyzed by agarose gel electrophoresis, blotted, and hybridized with a virus-specific 32P-labeled DNA probe. RFI and RFII refer to viral DNA replicative forms of monomer and dimer length, respectively. Viral DNA species were positioned relative to HindIII-digested phage λ DNA used as size markers and revealed by ethidium bromide staining. (E) The viral transcripts were detected by Northern blotting. At 48 hours postinfection (10 pfu/cell), total RNA was isolated by the guanidinium thiocyanate method, fractionated by agarose/formaldehyde gel electrophoresis, blotted, and hybridized with a virus-specific 32P-labeled DNA probe. (F ) The accumulation of viral proteins was determined by immunoprecipitation. At 36 hours postinfection (5 pfu/cell) cultures were incubated for 2 hours in the presence of [35S]methionine and processed for immunoprecipitation with antiserums directed against the viral products NS-1 or VP-1 and VP-2, SDS-PAGE, and autoradiography.
