the hsv-1 exonuclease, ul12, stimulates recombination by a single strand annealing mechanism1型单纯疱疹病毒核酸外切酶、ul12刺激由单一链重组退火机制.pdfVIP
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the hsv-1 exonuclease, ul12, stimulates recombination by a single strand annealing mechanism1型单纯疱疹病毒核酸外切酶、ul12刺激由单一链重组退火机制
The HSV-1 Exonuclease, UL12, Stimulates Recombination
by a Single Strand Annealing Mechanism
1 1 2 2 3
April J. Schumacher , Kareem N. Mohni , Yinan Kan , Eric A. Hendrickson , Jeremy M. Stark ,
Sandra K. Weller1*
1 Molecular, Microbial and Structural Biology Department, University of Connecticut Health Center, Farmington, Connecticut, United States of America, 2 Department of
Biochemistry, Molecular Biology, and Biophysics, University of Minnesota Medical School, Minneapolis, Minnesota, United States of America, 3 Department of Cancer
Biology, Beckman Research Institute of the City of Hope, Duarte, California, United States of America
Abstract
Production of concatemeric DNA is an essential step during HSV infection, as the packaging machinery must recognize
longer-than-unit-length concatemers; however, the mechanism by which they are formed is poorly understood. Although it
has been proposed that the viral genome circularizes and rolling circle replication leads to the formation of concatemers,
several lines of evidence suggest that HSV DNA replication involves recombination-dependent replication reminiscent of
bacteriophages l and T4. Similar to l, HSV-1 encodes a 59-to-39 exonuclease (UL12) and a single strand annealing protein
[SSAP (ICP8)] that interact with each other and can perform strand exchange in vitro. By analogy with l phage, HSV may
utilize viral and/or cellular recombination proteins during DNA replication. At least four double strand break repair pathways
are present in eukaryotic cells, and HSV-1 is known to manipulate several components of these pathways. Chromosomally
integrated reporter assays were used to measure the repair of double strand breaks in HSV-infected cells. Single strand
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