Literature DB >> 7831776

Characterization of defective-interfering RNAs of rubella virus generated during serial undiluted passage.

C A Derdeyn1, T K Frey.   

Abstract

During serial undiluted passage of rubella virus (RUB) in Vero cells, two species of defective-interfering (DI) RNAs of approximately 7000 and 800 nucleotides (nts) in length were generated (Frey, T. K., and Hemphill, M. L., Virology 164, 22-29, 1988). In this study, these DI RNAs were characterized by molecular cloning, hybridization with probes of defined sequence, and primer extension. The 7000-nt DI RNA species were found to be authentic DI RNAs which contain a single 2500- to 2700-nt deletion in the structural protein open reading frame (ORF) region of the genome. The 800-nt RNAs were found to be subgenomic DI RNAs synthesized from the large DI RNA templates. Analysis of the extent of the deletions using a reverse-transcription-PCR protocol revealed that the 3' end of the deletions did not extend beyond the 3' terminal 244 nts of the genome. The 5' end of the deletions did not extend into the nonstructural protein ORF; however, DI RNAs in which the subgenomic start site was deleted were present. Following serial undiluted passage of seven independent stocks of RUB, this was the only pattern of DI RNAs generated. DI RNAs of 2000 to 3000 nt in length were the majority DI RNA species in a persistently infected line of Vero cells, showing that other types of RUB DI RNAs can be generated and selected. However, when supernatant from the persistently infected cells was passaged, the only DI RNAs present after two passages were 7000 nts in length, indicating that this species has a selective advantage over other types of DI RNAs during serial passage.

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Year:  1995        PMID: 7831776      PMCID: PMC7130850          DOI: 10.1016/s0042-6822(95)80036-0

Source DB:  PubMed          Journal:  Virology        ISSN: 0042-6822            Impact factor:   3.616


  19 in total

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4.  Effect of antiviral antibody on maintenance of long-term rubella virus persistent infection in Vero cells.

Authors:  E S Abernathy; C Y Wang; T K Frey
Journal:  J Virol       Date:  1990-10       Impact factor: 5.103

5.  Time course of virus-specific macromolecular synthesis during rubella virus infection in Vero cells.

Authors:  M L Hemphill; R Y Forng; E S Abernathy; T K Frey
Journal:  Virology       Date:  1988-01       Impact factor: 3.616

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Journal:  Virology       Date:  1990-07       Impact factor: 3.616

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  13 in total

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Authors:  R Molenkamp; B C Rozier; S Greve; W J Spaan; E J Snijder
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4.  Rubella virus-like replicon particles: analysis of encapsidation determinants and non-structural roles of capsid protein in early post-entry replication.

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5.  Mutagenic analysis of the 3' cis-acting elements of the rubella virus genome.

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6.  Analysis of the 3' cis-acting elements of rubella virus by using replicons expressing a puromycin resistance gene.

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7.  Analysis of the selective advantage conferred by a C-E1 fusion protein synthesized by rubella virus DI RNAs.

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8.  Rubella virus capsid protein modulates viral genome replication and virus infectivity.

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9.  Effects of defined mutations in the 5' nontranslated region of rubella virus genomic RNA on virus viability and macromolecule synthesis.

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10.  C-E1 fusion protein synthesized by rubella virus DI RNAs maintained during serial passage.

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