Characterization and Function of Putative Substrate Specificity Domain in Microvirus External Scaffolding Proteins

doi:10.1128/JVI.00301-07

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Journal of Virology, August 2007, p. 8587-8592, Vol. 81, No. 16
0022-538X/07/$08.00+0 doi:10.1128/JVI.00301-07
Copyright © 2007, American Society for Microbiology. All Rights Reserved.

Characterization and Function of Putative Substrate Specificity Domain in Microvirus External Scaffolding Proteins

Asako Uchiyama, Min Chen, and Bentley A. Fane^*

Department of Veterinary Sciences and Microbiology, University of Arizona, Tucson, Arizona

Received 12 February 2007/ Accepted 25 May 2007

Microviruses (canonical members are bacteriophages ${phi}$ X174, G4,and ${alpha}$ 3) are T=1 icosahedral virions with an assembly pathwaymediated by two scaffolding proteins. The external scaffoldingprotein D plays a major role during morphogenesis, particularlyin icosahedral shell formation. The results of previous studies,conducted with a cloned chimeric external scaffolding gene,suggest that the first ${alpha}$ -helix acts as a substrate specificitydomain, perhaps mediating the initial coat-external scaffoldingprotein interaction. However, the expression of a cloned genecould lead to protein concentrations higher than those foundin typical infections. Moreover, its induction before infectioncould alter the timing of the protein's accumulation. Both ofthese factors could drive or facilitate reactions that may notoccur under physiological conditions or before programmed celllysis. In order to elucidate a more detailed mechanistic model,a chimeric external scaffolding gene was placed directly inthe ${phi}$ X174 genome under wild-type transcriptional and translationalcontrol, and the chimeric virus, which was not viable on thelevel of plaque formation, was characterized. The results ofthe genetic and biochemical analyses indicate that ${alpha}$ -helix 1most likely mediates the nucleation reaction for the formationof the first assembly intermediate containing the external scaffoldingprotein. Mutants that can more efficiently use the chimericscaffolding protein were isolated. These second-site mutationsappear to act on a kinetic level, shortening the lag phase beforevirion production, perhaps lowering the critical concentrationof the chimeric protein required for a nucleation reaction.

* Corresponding author. Mailing address: Department of Veterinary Sciences and Microbiology, University of Arizona, Tucson, AZ 85721-0090. Phone: (520) 626-6634. Fax: (520) 621-6636. E-mail: bfane{at}u.arizona.edu

Published ahead of print on 6 June 2007.

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