Literature DB >> 29046447

Functional Carboxy-Terminal Fluorescent Protein Fusion to Pseudorabies Virus Small Capsid Protein VP26.

Ian B Hogue1,2, Jolie Jean1, Andrew D Esteves1, Nikhila S Tanneti1, Julian Scherer1, Lynn W Enquist3.   

Abstract

Fluorescent protein fusions to herpesvirus capsids have proven to be a valuable method to study virus particle transport in living cells. Fluorescent protein fusions to the amino terminus of small capsid protein VP26 are the most widely used method to visualize pseudorabies virus (PRV) and herpes simplex virus (HSV) particles in living cells. However, these fusion proteins do not incorporate to full occupancy and have modest effects on virus replication and pathogenesis. Recent cryoelectron microscopy studies have revealed that herpesvirus small capsid proteins bind to capsids via their amino terminus, whereas the carboxy terminus is unstructured and therefore may better tolerate fluorescent protein fusions. Here, we describe a new recombinant PRV expressing a carboxy-terminal VP26-mCherry fusion. Compared to previously characterized viruses expressing amino-terminal fusions, this virus expresses more VP26 fusion protein in infected cells and incorporates more VP26 fusion protein into virus particles, and individual virus particles exhibit brighter red fluorescence. We performed single-particle tracking of fluorescent virus particles in primary neurons to measure anterograde and retrograde axonal transport, demonstrating the usefulness of this novel VP26-mCherry fusion for the study of viral intracellular transport.IMPORTANCE Alphaherpesviruses are among the very few viruses that are adapted to invade the mammalian nervous system. Intracellular transport of virus particles in neurons is important, as this process underlies both mild peripheral nervous system infection and severe spread to the central nervous system. VP26, the small capsid protein of HSV and PRV, was one of the first herpesvirus proteins to be fused to a fluorescent protein. Since then, these capsid-tagged virus mutants have become a powerful tool to visualize and track individual virus particles. Improved capsid tags will facilitate fluorescence microscopy studies of virus particle intracellular transport, as a brighter particle will improve localization accuracy of individual particles and allow for shorter exposure times, reducing phototoxicity and improving the time resolution of particle tracking in live cells.
Copyright © 2017 American Society for Microbiology.

Entities:  

Keywords:  fluorescence; fluorescent image analysis; fluorescent protein; herpes simplex virus; herpesviruses; neuron; neurotropic viruses; neurovirulence; pseudorabies virus; video microscopy

Mesh:

Substances:

Year:  2017        PMID: 29046447      PMCID: PMC5730785          DOI: 10.1128/JVI.01193-17

Source DB:  PubMed          Journal:  J Virol        ISSN: 0022-538X            Impact factor:   5.103


  36 in total

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7.  Extensive subunit contacts underpin herpesvirus capsid stability and interior-to-exterior allostery.

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8.  Improper tagging of the non-essential small capsid protein VP26 impairs nuclear capsid egress of herpes simplex virus.

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9.  Role of Us9 phosphorylation in axonal sorting and anterograde transport of pseudorabies virus.

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Review 10.  Fluorescent Protein Approaches in Alpha Herpesvirus Research.

Authors:  Ian B Hogue; Jens B Bosse; Esteban A Engel; Julian Scherer; Jiun-Ruey Hu; Tony Del Rio; Lynn W Enquist
Journal:  Viruses       Date:  2015-11-19       Impact factor: 5.048

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2.  Establishment of a Fosmid Library for Pseudorabies Virus SC Strain and Application in Viral Neuronal Tracing.

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3.  The Cholesterol Transport Inhibitor U18666A Interferes with Pseudorabies Virus Infection.

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4.  Pseudorabies Virus UL24 Abrogates Tumor Necrosis Factor Alpha-Induced NF-κB Activation by Degrading P65.

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  4 in total

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