Virological characterization of HIV-1 RNA elements detected exclusively through the LTR region by the dual-target Aptima HIV-1 Quant Dx assay in a subset of positive patients

被引:1
作者
Sberna, Giuseppe [1 ]
Nardacci, Roberta [2 ]
Berno, Giulia [1 ]
Rozera, Gabriella [1 ]
Giombini, Emanuela [1 ]
Fabeni, Lavinia [1 ]
Specchiarello, Eliana [1 ]
Maggi, Fabrizio [1 ]
Amendola, Alessandra [1 ,3 ]
机构
[1] Natl Inst Infect Dis L Spallanzani IRCCS, Lab Virol, Rome, Italy
[2] Natl Inst Infect Dis Lazzaro Spallanzani, Lab Electron Microscopy, IRCCS, Rome, Italy
[3] Via Portuense 292, I-00149 Rome, Italy
关键词
HIV; -RNA; Viral load; Dual-target assay; LTR; Antiretroviral therapy; T-LYMPHOCYTES; PROVIRUSES;
D O I
10.1016/j.jcv.2023.105575
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Background: In a restricted subset of HIV patients with suppressed viral load (i.e., pol-undetected HIV-RNA), the Aptima HIV-1 Quant Dx Assay (Aptima), a dual-target (pol and LTR) and dual-probe test for viral load (VL) monitoring, can detect HIV-RNA exclusively through amplification of the LTR region.Objectives: To analyze the virological characteristics of the HIV-RNA elements detected only through LTR amplification (LTR-e). Study design: LTR-e isolated from plasma and peripheral blood mononuclear cells (PBMC) were evaluated for their ability to trigger productive infections. Viral pellets morphology and ultrastructural characteristics of PBMC from LTR-e patients were examined by electron microscopy. Plasma LTR-e underwent Sanger sequencing. Exosomes were examined with Aptima for LTR-e content.Results: In-vitro, LTR-e could not infect PBMC, induce cytopathic effects, or cause syncytia, even at high VL (e.g., >10,000 copies/mL). Under the electron microscope, plasma pellets and PBMC from patients with LTR-e showed atypical vesicles. Sanger sequencing of LTR-e yielded no results. Moreover, in plasma samples, LTR-e were associated with cell debris, never with exosomes.Conclusions: Differently from other dual-target but single-probe assays, Aptima unveils VL based only on LTR amplification in some HIV patients. Here, we show that LTR-e represent partial/incomplete/non-canonical transcripts unable to trigger productive infection or transmit HIV-1 infection. The recognition of VL based only on LTR-e in infected individuals is crucial as it allows to avoid inappropriate decisions in the clinical management of HIV patients, such as retesting of VL and switching of ART. Physicians and HIV-RNA dual-target assay manufacturers should consider the important implications of not recognizing this singular type of VL.
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