Affiliation:
1. Department of Microbiology and Immunology, SUNY Upstate Medical University, Syracuse, New York 13210
Abstract
ABSTRACT
Recombinant viruses were constructed to have an
Escherichia coli
replicon containing a mutagenesis marker, the
supF
gene, integrated within the thymidine kinase locus (
tk
) of herpes simplex virus type 1. These viruses expressed either wild-type or mutant DNA polymerase (Pol) and were tested in a mutagenesis assay for the fidelity of their replication of the
supF
gene. A mutation frequency of approximately 10
−4
was observed for wild-type strain KOS-derived recombinants in their replication of the
supF
gene. However, recombinants derived from the PAA
r
5 Pol mutant, which has been demonstrated to have an antimutator phenotype in replicating the
tk
gene, had three- to fourfold increases in
supF
mutation frequency (
P
< 0.01), a result similar to that exhibited when the
supF
gene was induced to replicate as episomal DNA (Y. T. Hwang, B.-Y. Liu, C.-Y. Hong, E. J. Shillitoe, and C. B. C. Hwang, J. Virol. 73:5326-5332, 1999). Thus, the PAA
r
5 Pol mutant had an antimutator function in replicating the
tk
gene and was less accurate in replicating the
supF
gene than was the wild-type strain. The spectra of mutations and distributions of substituted bases within the
supF
genes that replicated as genomic DNA were different from those in the genes that replicated as episomal DNA. Therefore, the differences in sequence contents between the two target genes influenced the accuracy of the Pol during viral replication. Furthermore, the replication mode of the target gene also affected the mutational spectrum.
Publisher
American Society for Microbiology
Subject
Virology,Insect Science,Immunology,Microbiology
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