Analysis of the functional and host range-determining regions of the murine ectropic and amphotropic retrovirus envelope proteins.

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J Virol. 1993 August; 67(8): 4712-4721

Analysis of the functional and host range-determining regions of the murine ectropic and amphotropic retrovirus envelope proteins.

R A Morgan, O Nussbaum, D D Muenchau, L Shu, L Couture and W F Anderson

Molecular Hematology Branch, National Heart, Lung, and Blood Institute, Bethesda, Maryland 20892.

ABSTRACT

A series of Moloney murine leukemia virus (Mo-MuLV) envelopegene constructs were analyzed for biological activity. Threeclasses of recombinant envelopes were examined: insertions,deletions, and chimeras. Insertion (4 to 5 amino acids) anddeletion (31 to 62 amino acids) mutants spanned most of theSU (gp70)-coding region and were all biologically inactive.Radioimmunoprecipitation demonstrated that the mutant envelopeproteins were incorrectly processed. The Pr80env envelope precursorproteins failed to obtain the proper posttranslational modificationsand were not cleaved into SU (gp70) and TM (p15E), suggestingthat disruption of Pr80env structure prevents intracellulartransport and processing. To analyze the functional domainsof the SU portion of the Env protein, we assembled several chimericconstructs. In these constructs, portions of the ecotropic Mo-MuLVenvelope gene were replaced with corresponding sequences fromthe 4070A amphotropic MuLV envelope. Using a retroviral vectorpseudotyping assay, 5 of 12 chimeric envelope proteins wereshown to be biologically active. Host range was determined byretroviral vector transduction of the appropriate cell, by viralinterference studies, and by the productive infection of Chinesehamster ovary cells expressing the murine ecotropic receptor.These results permit assignment of the amino acids responsiblefor host range determination. Ecotropic host range is determinedby the first 88 amino acids of the Mo-MuLV SU, while the amphotropichost range-determining region spans the first 157 amino acidsof the 4070A SU.

J Virol. 1993 August; 67(8): 4712-4721

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