|
Basic Characteristics of Mutations
|
|
Mutation Site
|
N116A |
|
Mutation Site Sentence
|
Based on the initial experiments showing a lack ofΔ105– 125 virus replication in the SCIDhu model of skin pathogenesis, the C95A, C106A, and N116A mutants were tested for replication and viral spread in human skin. |
|
Mutation Level
|
Amino acid level |
|
Mutation Type
|
Nonsynonymous substitution |
|
Gene/Protein/Region
|
gI |
|
Standardized Encoding Gene
|
ORF67
|
|
Genotype/Subtype
|
- |
|
Viral Reference
|
AB097933
|
|
Functional Impact and Mechanisms
|
|
Disease
|
Varicella Zoster Virus Infection
Cell line
|
|
Immune
|
- |
|
Target Gene
|
-
|
|
Clinical and Epidemiological Correlations
|
|
Clinical Information
|
- |
|
Treatment
|
- |
|
Location
|
- |
|
Literature Information
|
|
PMID
|
21345964
|
|
Title
|
Mutagenesis of varicella-zoster virus glycoprotein I (gI) identifies a cysteine residue critical for gE/gI heterodimer formation, gI structure, and virulence in skin cells
|
|
Author
|
Oliver SL,Sommer MH,Reichelt M,Rajamani J,Vlaycheva-Beisheim L,Stamatis S,Cheng J,Jones C,Zehnder J,Arvin AM
|
|
Journal
|
Journal of virology
|
|
Journal Info
|
2011 May;85(9):4095-110
|
|
Abstract
|
Varicella-zoster virus (VZV) is the alphaherpesvirus that causes chicken pox (varicella) and shingles (zoster). The two VZV glycoproteins gE and gI form a heterodimer that mediates efficient cell-to-cell spread. Deletion of gI yields a small-plaque-phenotype virus, DeltagI virus, which is avirulent in human skin using the xenograft model of VZV pathogenesis. In the present study, 10 mutant viruses were generated to determine which residues were required for the typical function of gI. Three phosphorylation sites in the cytoplasmic domain of gI were not required for VZV virulence in vivo. Two deletion mutants mapped a gE binding region in gI to residues 105 to 125. A glycosylation site, N116, in this region did not affect virulence. Substitution of four cysteine residues highly conserved in the Alphaherpesvirinae established that C95 is required for gE/gI heterodimer formation. The C95A and Delta105-125 (with residues 105 to 125 deleted) viruses had small-plaque phenotypes with reduced replication kinetics in vitro similar to those of the DeltagI virus. The Delta105-125 virus was avirulent for human skin in vivo. In contrast, the C95A mutant replicated in vivo but with significantly reduced kinetics compared to those of the wild-type virus. In addition to abolished gE/gI heterodimer formation, gI from the C95A or the Delta105-125 mutant was not recognized by monoclonal antibodies that detect the canonical conformation of gI, demonstrating structural disruption of gI in these viruses. This alteration prevented gI incorporation into virus particles. Thus, residues C95 and 105 to 125 are critical for gI structure required for gE/gI heterodimer formation, virion incorporation, and ultimately, effective viral spread in human skin.
|
|
Sequence Data
|
-
|
|
|
