| Literature DB >> 32544419 |
Sigrun Häge1, Deborah Horsch2, Anne-Charlotte Stilp3, Jintawee Kicuntod4, Regina Müller5, Stuart T Hamilton6, Ece Egilmezer7, William D Rawlinson8, Thomas Stamminger9, Eric Sonntag10, Manfred Marschall11.
Abstract
Nuclear egress is a rate-limiting step of herpesviral replication, restricting the nucleocytoplasmic transport of viral capsids. The process is regulated by two viral nuclear egress proteins (core NEC pUL50-pUL53), which recruit additional cellular and viral proteins. The multicomponent NEC mediates disassembly of the nuclear lamina barrier and the docking of nuclear capsids. The quantitation of nuclear egress has been accomplished by electron microscopic analysis, but is generally hampered by the low number of detectable cytoplasmic capsids. A newly established method for the quantitation of viral nuclear egress improves the characterization of viral mutants, host cell permissiveness and antiviral drug efficacy. In this study, various strains of human cytomegalovirus (HCMV) were used to measure the replication efficiencies in primary human fibroblasts, applying methods of cell fractionation, DNase digestion, sucrose cushions and quantitative PCR. Several stages of optimization led to a reliable quantitative assay that allowed the characterization of viral nuclear egress efficacy. Using this assay, recovery of the nuclear egress of a NEC-defective HCMV mutant was quantitatively assessed by applying an inducible NEC-expressing fibroblast culture for trans-complementation. This novel assay system can be further used to accurately quantitate and characterize the functionality of nuclear egress of HCMV or other herpesviruses. CrownEntities:
Keywords: Capsid-Release; Cytomegalovirus; Fractionation; Nuclear egress; Quantitative assay; genome-specific-qPCR
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Year: 2020 PMID: 32544419 DOI: 10.1016/j.jviromet.2020.113909
Source DB: PubMed Journal: J Virol Methods ISSN: 0166-0934 Impact factor: 2.014