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Maximizing viral detection with SIV droplet digital PCR (ddPCR) assays

  1. Author:
    Long, Samuel [ORCID]
    Berkemeier,Brian
  2. Author Address

    AIDS and Cancer Virus Program, Frederick National Laboratory for Cancer Research, Frederick, Maryland, United States of America.,
    1. Year: 2020
    2. Date: MAY 14
    3. Epub Date: 2020 05 14
  1. Journal: PloS one
    1. 15
    2. 5
    3. Pages: e0233085
  2. Type of Article: Article
  3. Article Number: e0233085
  4. ISSN: 1932-6203
  1. Abstract:

    Highly sensitive detection of HIV-1 nucleic acids is of critical importance for evaluating treatment interventions superimposed on combination antiretroviral therapy (cART) in HIV-1 infected individuals. SIV infection of rhesus macaques models many key aspects of human HIV-1 infection and plays a key role in evaluation of approaches for prevention, treatment and attempted eradication of HIV infection. Here we describe two droplet digital PCR (ddPCR) assays, a ddPCR DNA assay and an RT-ddPCR RNA assay for detecting simian immunodeficiency virus (SIV) on the RainDance platform. We demonstrate that RainDance ddPCR can tolerate significantly higher cell DNA input without inhibition on a per reaction basis (compared to both qPCR and Bio-Rad ddPCR), thus allowing a large quantity of sample to be analyzed in each reaction. In addition, the combination of a high processivity RT enzyme and RainDance ddPCR could overcome inhibition in severely inhibited (99.99% inhibition in qPCR quantification) viral RNA samples. These assays offer valuable tools for assessing low level viral production/replication and strategies for targeting residual virus in the setting of cART suppression of viral replication. The methodologies presented here can be adapted for a broad range of applications where highly sensitive nucleic acid detection is required.

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External Sources

  1. DOI: 10.1371/journal.pone.0233085
  2. PMID: 32407343
  3. WOS: 000537490700067
  4. PII : PONE-D-20-01937

Library Notes

  1. Fiscal Year: FY2019-2020
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