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International network for comparison of HIV neutralization assays: the NeutNet report II. | LitMetric

AI Article Synopsis

  • Neutralizing antibodies are critical for assessing vaccine-induced immunity against HIV-1, but there is a lack of clarity on which assays accurately measure protective immunity.
  • An international study (NeutNet Phase II) involving 13 laboratories evaluated polyclonal reagents using nine plasma samples across an 8 virus panel, comparing results with a previous phase that used monoclonal antibodies.
  • The findings revealed that the PSV assay was generally more sensitive than the PBMC assay, with significant differences in sensitivities depending on the specific virus and the plasma used for testing.

Article Abstract

Background: Neutralizing antibodies provide markers for vaccine-induced protective immunity in many viral infections. By analogy, HIV-1 neutralizing antibodies induced by immunization may well predict vaccine effectiveness. Assessment of neutralizing antibodies is therefore of primary importance, but is hampered by the fact that we do not know which assay(s) can provide measures of protective immunity. An international collaboration (NeutNet) involving 18 different laboratories previously compared different assays using monoclonal antibodies (mAbs) and soluble CD4 (Phase I study).

Methods: In the present study (Phase II), polyclonal reagents were evaluated by 13 laboratories. Each laboratory evaluated nine plasmas against an 8 virus panel representing different genetic subtypes and phenotypes. TriMab, a mixture of three mAbs, was used as a positive control allowing comparison of the results with Phase I in a total of nine different assays. The assays used either uncloned virus produced in peripheral blood mononuclear cells (PBMCs) (Virus Infectivity Assays, VIA), or Env (gp160)-pseudotyped viruses (pseudoviruses, PSV) produced in HEK293T cells from molecular clones or from uncloned virus. Target cells included PBMC and genetically engineered cell lines in either single- or multiple-cycle infection format. Infection was quantified by using a range of assay read-outs including extra- or intra-cellular p24 antigen detection, luciferase, beta-galactosidase or green fluorescent protein (GFP) reporter gene expression.

Findings: Using TriMab, results of Phase I and Phase II were generally in agreement for six of the eight viruses tested and confirmed that the PSV assay is more sensitive than PBMC (p = 0.014). Comparisons with the polyclonal reagents showed that sensitivities were dependent on both virus and plasma.

Conclusions: Here we further demonstrate clear differences in assay sensitivities that were dependent on both the neutralizing reagent and the virus. Consistent with the Phase I study, we recommend parallel use of PSV and VIA for vaccine evaluation.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3348930PMC
http://journals.plos.org/plosone/article?id=10.1371/journal.pone.0036438PLOS

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