Amplifying and Quantifying HIV-1 RNA in HIV Infected Individuals with Viral Loads Below the Limit of Detection by Standard Clinical Assays

Helene Mens; Mary Kearney; Ann Wiegand; Jonathan Spindler; Frank Maldarelli; John W. Mellors; John M. Coffin

doi:10.3791/2960

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Amplifying and Quantifying HIV-1 RNA in HIV Infected Individuals with Viral Loads Below the Limit of Detection by Standard Clinical Assays

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Amplifying and Quantifying HIV-1 RNA in HIV Infected Individuals with Viral Loads Below the Limit of Detection by Standard Clinical Assays

31,216 Views

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13:58 min

•

September 26, 2011

DOI:

10.3791/2960-v

DOI:

10.3791/2960-v

•

13:58 min

September 26, 2011

•

3 Views

Helene Mens¹, Mary Kearney¹, Ann Wiegand¹, Jonathan Spindler¹, Frank Maldarelli¹, John W. Mellors², John M. Coffin³

¹The virology Core at the HIV Drug Resistance Program,NCI-Frederick, ²Division of Infectious Diseases,University of Pittsburgh, ³Department of Molecular Biology and Microbiology,Tuffts University

Özet

Quantifying levels of HIV-1 RNA in plasma and sequencing single HIV-1 genomes from individuals with viral loads below the limit of detection (50-75 copies/ml) is difficult. Here we describe how to extract and quantify plasma viral RNA using a real time PCR assay that reliably measures HIV-1 RNA down to 0.3 copies/ml and how to amplify viral genomes by single genome sequencing, from samples with very low viral loads.

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Amplifying and Quantifying HIV-1 RNA in HIV Infected Individuals with Viral Loads Below the Limit of Detection by Standard Clinical Assays

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