Tracking HIV-1-Infected Cell Clones Using Integration Site-Specific qPCR

Author:

Brandt Leah D.ORCID,Guo ShuangORCID,Joseph Kevin W.,Jacobs Jana L.,Naqvi Asma,Coffin John M.,Kearney Mary F.,Halvas Elias K.,Wu Xiaolin,Hughes Stephen H.,Mellors John W.

Abstract

Efforts to cure HIV-1 infection require better quantification of the HIV-1 reservoir, particularly the clones of cells harboring replication-competent (intact) proviruses, termed repliclones. The digital droplet PCR assays commonly used to quantify intact proviruses do not differentiate among specific repliclones, thus the dynamics of repliclones are not well defined. The major challenge in tracking repliclones is the relative rarity of the cells carrying specific intact proviruses. To date, detection and accurate quantification of repliclones requires in-depth integration site sequencing. Here, we describe a simplified workflow using integration site-specific qPCR (IS-qPCR) to determine the frequencies of the proviruses integrated in individual repliclones. We designed IS-qPCR to determine the frequencies of repliclones and clones of cells that carry defective proviruses in samples from three donors. Comparing the results of IS-qPCR with deep integration site sequencing data showed that the two methods yielded concordant estimates of clone frequencies (r = 0.838). IS-qPCR is a potentially valuable tool that can be applied to multiple samples and cell types over time to measure the dynamics of individual repliclones and the efficacy of treatments designed to eliminate them.

Funder

National Cancer Institute

Bill and Melinda Gates Foundation

National Institute of Allergy and Infectious Diseases

American Cancer Society

Office of AIDS Research

Leidos

Publisher

MDPI AG

Subject

Virology,Infectious Diseases

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