C-terminal truncation of the transmembrane protein of an attenuated lentiviral vaccine alters its in vitro but not in vivo replication and weakens its potential pathogenicity

► CT truncation of EIAV TM decreases viral replication in cultivated equine and donkey macrophages. ► It does not influence the plasma viral load of inoculated hosts. ► The host immunity is presumably responsible for the equal in vivo replication. ► The CT truncation weakens potential pathogenicity...

Full description

Saved in:
Bibliographic Details
Published in:Virus research 2011-06, Vol.158 (1), p.235-245
Main Authors: Jiang, Cheng-Gang, Gao, Xu, Ma, Jian, Lin, Yue-Zhi, Wang, Xue-Feng, Zhao, Li-Ping, Hua, Yue-Ping, Liu, Di, Zhou, Jian-Hua
Format: Article
Language:English
Subjects:
anemia
Animals
Antibodies, Neutralizing - blood
Antibodies, Viral - blood
apoptosis
asses
Codon, Nonsense
codons
dexamethasone
drug therapy
EIAV
Equidae
Equine infectious anemia virus
genes
gp45
Horses
hosts
immunity
Infectious Anemia Virus, Equine - genetics
Infectious Anemia Virus, Equine - pathogenicity
loading
macrophages
Monocytes - virology
neutralization
neutralizing antibodies
Pathogenicity
Replication
Sequence Deletion
stop codon
transmembrane proteins
Truncation
vaccines
Vaccines, Attenuated - adverse effects
Vaccines, Attenuated - genetics
Vaccines, Attenuated - immunology
Viral Envelope Proteins - genetics
viral load
viral replication
Viral Vaccines - adverse effects
Viral Vaccines - genetics
Viral Vaccines - immunology
Virulence
Virus Replication
viruses
Citations: Items that this one cites
Items that cite this one
Online Access:Get full text
Tags: Add Tag
No Tags, Be the first to tag this record!
Description
Summary:► CT truncation of EIAV TM decreases viral replication in cultivated equine and donkey macrophages. ► It does not influence the plasma viral load of inoculated hosts. ► The host immunity is presumably responsible for the equal in vivo replication. ► The CT truncation weakens potential pathogenicity of the vaccine. Preliminary studies revealed that the gene of the gp45 transmembrane protein (TM) of the attenuated equine infectious anemia virus (EIAV) vaccine strain EIAV FDDV13 had a high frequency of a premature stop codon at position 261W, which generated a 154-residue truncation at the C-terminus. EIAV FDDV-TM36, a recombinant virus with the TM truncated at the intracytoplasmic (CT) domain due to the presence of a stop codon, was constructed based on EIAV FDDV3-8, which is a proviral derivative of the vaccine. EIAV FDDV-TM36 had a significantly reduced replication capability compared to EIAV FDDV3-8 in equine or donkey monocyte-derived macrophages and a decreased ability to induce apoptosis. However, both viruses raised a similar plasma viral load in inoculated horses and did not induce clinical symptoms of EIA. To further compare the in vivo behavior between EIAV FDDV-TM36 and EIAV FDDV3-8, inoculated horses were transiently immunosuppressed with dexamethasone. While three of the four horses inoculated with EIAV FDDV3-8 demonstrated significant increases in viral loads after the drug treatment, none of the four horses inoculated with EIAV FDDV-TM36 showed a statistically increased plasma viral load. Significantly increased neutralizing antibody levels were also observed in the group of horses inoculated with EIAV FDDV3-8, but not EIAV FDDV-TM36, after immunosuppression. Our results indicate that although the CT truncation of TM decreased viral replication in cultivated equine and donkey macrophages, the primary target cell of EIAV, and did not influence the plasma viral load of inoculated hosts, it weakened the potential pathogenicity of the vaccine. The host immunity is presumably responsible for the equal in vivo replication levels of viruses with either the CT-truncated or prototype TM.
ISSN:0168-1702
1872-7492
DOI:10.1016/j.virusres.2011.04.007