Stable Multi-infection of Splenocytes During SIV Infection--the Basis for Continuous Recombination

Overview

Journal Retrovirology

Publisher Biomed Central

Specialty Microbiology

Date 2012 Apr 25

PMID 22524249

Citations 3

Authors

Anke Schultz

Sieghart Sopper

Ulrike Sauermann

Andreas Meyerhans

Rodolphe Suspene

Affiliations

Soon will be listed here.

Abstract

Background: Recombination is an important mechanism in the generation of genetic diversity of the human (HIV) and simian (SIV) immunodeficiency viruses. It requires the co-packaging of divergent RNA genomes into the same retroviral capsid and subsequent template switching during the reverse transcription reaction. By HIV-specific fluorescence in situ hybridization (FISH), we have previously shown that the splenocytes from 2 chronically infected patients with Castelman's disease were multi-infected and thus fulfill the in vivo requirements to generate genetic diversity by recombination. In order to analyze when multi-infection first occurs during a lentivirus infection and how the distribution of multi-infection evolves during the disease course, we now determined the SIV copy numbers from splenocytes of 11 SIVmac251-infected rhesus macaques cross-sectionally covering the time span of primary infection throughout to end-stage immunodeficiency.

Results: SIV multi-infection of single splenocytes was readily detected in all monkeys and all stages of the infection. Single-infected cells were more frequent than double- or triple- infected cells. There was no strong trend linking the copy number distribution to plasma viral load, disease stage, or CD4 cell counts.

Conclusions: SIV multi-infection of single cells is already established during the primary infection phase thus enabling recombination to affect viral evolution in vivo throughout the disease course.

Citing Articles

Modeling of the HIV-1 Life Cycle in Productively Infected Cells to Predict Novel Therapeutic Targets.

Shcherbatova O, Grebennikov D, Sazonov I, Meyerhans A, Bocharov G Pathogens. 2020; 9(4).

PMID: 32244421 PMC: 7238236. DOI: 10.3390/pathogens9040255.

Comparison of digital PCR platforms and semi-nested qPCR as a tool to determine the size of the HIV reservoir.

Bosman K, Nijhuis M, van Ham P, Wensing A, Vervisch K, Vandekerckhove L Sci Rep. 2015; 5:13811.

PMID: 26350506 PMC: 4563360. DOI: 10.1038/srep13811.

Retroviral vectors for analysis of viral mutagenesis and recombination.

Rawson J, Mansky L Viruses. 2014; 6(9):3612-42.

PMID: 25254386 PMC: 4189041. DOI: 10.3390/v6093612.

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