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HIV Protocols pp 35–40Cite as

Use of Luciferase Reporter Viruses for Studying HIV Entry

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Part of the book series: Methods in Molecular Medicine™ ((MIMM,volume 17))

Abstract

HIV replication is classically measured by quantitating virus present in the supernatant of infected cells over time. Typically, cells are infected at low multiplicity of infection (MOI) and washed extensively to remove input virus. Samples of culture supernatant are then removed over approximately a two week period and frozen. Virus in the supernatants is then quantitated by reverse transcriptase assay or by ELISA for p24gag antigen. Using live virus for studying virus replication is appropriate for many applications but has several drawbacks. Generating growth curves is relatively labor-intensive, requiring frequent sampling and passaging of the infected cultures. Input virus may be carried over and mistaken for virus production at early points in the growth curve. In addition, there is the biohazard associated with working with live virus.

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Author information

Authors and Affiliations

  1. Aaron Diamond AIDS Research Center, New York, NY

    Rong Liu, Benjamin Chen & Nathaniel R. Landau

Authors
  1. Rong Liu
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  2. Benjamin Chen
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  3. Nathaniel R. Landau
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Editor information

Editors and Affiliations

  1. Walter Reed Army Institute of Research, Rockville, MD

    Nelson L. Michael MD, PhD

  2. Henry M. Jackson Foundation, Rockville, MD

    Jerome H. Kim MD

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© 1999 Humana Press Inc., Totowa, NJ

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Cite this protocol

Liu, R., Chen, B., Landau, N.R. (1999). Use of Luciferase Reporter Viruses for Studying HIV Entry. In: Michael, N.L., Kim, J.H. (eds) HIV Protocols. Methods in Molecular Medicine™, vol 17. Humana Press. https://doi.org/10.1385/0-89603-369-4:35

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  • DOI: https://doi.org/10.1385/0-89603-369-4:35

  • Publisher Name: Humana Press

  • Print ISBN: 978-0-89603-369-6

  • Online ISBN: 978-1-59259-601-0

  • eBook Packages: Springer Protocols

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