Spatiotemporal dynamics of HSV genome nuclear entry and compaction state transitions using bioorthogonal chemistry and super-resolution microscopy

Eiki Sekine; Nora Schmidt; David Gaboriau; Peter O'Hare

doi:10.1371/journal.ppat.1006721

Spatiotemporal dynamics of HSV genome nuclear entry and compaction state transitions using bioorthogonal chemistry and super-resolution microscopy

PLoS Pathog. 2017 Nov 9;13(11):e1006721. doi: 10.1371/journal.ppat.1006721. eCollection 2017 Nov.

Authors

Eiki Sekine¹, Nora Schmidt¹, David Gaboriau², Peter O'Hare¹

Affiliations

¹ Section of Virology, Department of Medicine, Imperial College, St Mary's Medical School, London, United Kingdom.
² Department of Medicine, Facility for Imaging by Light Microscopy, National Heart and Lung Institute, Imperial College, London, United Kingdom.

Abstract

We investigated the spatiotemporal dynamics of HSV genome transport during the initiation of infection using viruses containing bioorthogonal traceable precursors incorporated into their genomes (HSVEdC). In vitro assays revealed a structural alteration in the capsid induced upon HSVEdC binding to solid supports that allowed coupling to external capture agents and demonstrated that the vast majority of individual virions contained bioorthogonally-tagged genomes. Using HSVEdC in vivo we reveal novel aspects of the kinetics, localisation, mechanistic entry requirements and morphological transitions of infecting genomes. Uncoating and nuclear import was observed within 30 min, with genomes in a defined compaction state (ca. 3-fold volume increase from capsids). Free cytosolic uncoated genomes were infrequent (7-10% of the total uncoated genomes), likely a consequence of subpopulations of cells receiving high particle numbers. Uncoated nuclear genomes underwent temporal transitions in condensation state and while ICP4 efficiently associated with condensed foci of initial infecting genomes, this relationship switched away from residual longer lived condensed foci to increasingly decondensed genomes as infection progressed. Inhibition of transcription had no effect on nuclear entry but in the absence of transcription, genomes persisted as tightly condensed foci. Ongoing transcription, in the absence of protein synthesis, revealed a distinct spatial clustering of genomes, which we have termed genome congregation, not seen with non-transcribing genomes. Genomes expanded to more decondensed forms in the absence of DNA replication indicating additional transitional steps. During full progression of infection, genomes decondensed further, with a diffuse low intensity signal dissipated within replication compartments, but frequently with tight foci remaining peripherally, representing unreplicated genomes or condensed parental strands of replicated DNA. Uncoating and nuclear entry was independent of proteasome function and resistant to inhibitors of nuclear export. Together with additional data our results reveal new insight into the spatiotemporal dynamics of HSV genome uncoating, transport and organisation.

MeSH terms

Capsid Proteins / metabolism*
Cell Line
Cell Nucleus / genetics
Cell Nucleus / metabolism*
DNA Replication / genetics
Genome, Viral*
Herpesvirus 1, Human / physiology*
Humans
Microscopy / methods
Virion / metabolism*
Virus Replication / physiology*
Virus Uncoating / genetics

Substances

Capsid Proteins

Grants and funding

This work was funded in part by grants from the Biotechnology and Biological Sciences Research Council, GB which support the Facility for Light Microscopy Imperial College London to DG (http://www.bbsrc.ac.uk/) and by a PhD studentship from the Wellcome Trust, UK (https://wellcome.ac.uk/) to ES. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.