Novel Method for Simultaneous Quantification of Phenotypic Resistance to Maturation, Protease, Reverse Transcriptase, and Integrase HIV Inhibitors Based on 3′Gag(p2/p7/p1/p6)/PR/RT/INT-Recombinant Viruses: a Useful Tool in the Multitarget Era of Antiretroviral Therapy | Zendy

Jan Weber | Zendy; Ana Vázquez | Zendy; Dane Winner | Zendy; Justine D. Rose | Zendy; Doug Wylie | Zendy; Ariel M. Rhea | Zendy; Kenneth R. Henry | Zendy; Jennifer Pappas | Zendy; Alison Wright | Zendy; N. A. Mohamed | Zendy; Richard Gibson | Zendy; Benigno Rodrı́guez | Zendy; Vincent Soriano | Zendy; Kevin King | Zendy; Eric J. Arts | Zendy; Paul D. Olivo | Zendy; Miguel E. QuiñonesMateu | Zendy

Open Access

Novel Method for Simultaneous Quantification of Phenotypic Resistance to Maturation, Protease, Reverse Transcriptase, and Integrase HIV Inhibitors Based on 3′Gag(p2/p7/p1/p6)/PR/RT/INT-Recombinant Viruses: a Useful Tool in the Multitarget Era of Antiretroviral Therapy

Author(s) -

Jan Weber,

Ana Vázquez,

Dane Winner,

Justine D. Rose,

Doug Wylie,

Ariel M. Rhea,

Kenneth R. Henry,

Jennifer Pappas,

Alison Wright,

N. A. Mohamed,

Richard Gibson,

Benigno Rodrı́guez,

Vincent Soriano,

Kevin King,

Eric J. Arts,

Paul D. Olivo,

Miguel E. QuiñonesMateu

Publication year - 2011

Publication title -

antimicrobial agents and chemotherapy

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 2.07

H-Index - 259

eISSN - 1070-6283

pISSN - 0066-4804

DOI - 10.1128/aac.00396-11

Subject(s) - integrase , reverse transcriptase , virology , biology , rnase h , recombinant dna , virus , microbiology and biotechnology , polymerase chain reaction , gene , genetics , human immunodeficiency virus (hiv)

Twenty-six antiretroviral drugs (ARVs), targeting five different steps in the life cycle of the human immunodeficiency virus type 1 (HIV-1), have been approved for the treatment of HIV-1 infection. Accordingly, HIV-1 phenotypic assays based on common cloning technology currently employ three, or possibly four, different recombinant viruses. Here, we describe a system to assess HIV-1 resistance to all drugs targeting the three viral enzymes as well as viral assembly using a single patient-derived, chimeric virus. Patient-derived p2-INT (gag -p2/NCp7/p1/p6/pol -PR/RT/IN) products were PCR amplified as a single fragment (3,428 bp) or two overlapping fragments (1,657 bp and 2,002 bp) and then recombined into a vector containing a near-full-length HIV-1 genome with theSaccharomyces cerevisiae uracil biosynthesis gene (URA3) replacing the 3,428 bp p2-INT segment (Dudley et al., Biotechniques 46:458–467, 2009). P2-INT-recombinant viruses were employed in drug susceptibility assays to test the activity of protease (PI), nucleoside/nucleotide reverse transcriptase (NRTI), nonnucleoside reverse transcriptase (NNRTI), and integrase strand-transfer (INSTI) inhibitors. Using a single standardized test (ViralARTS HIV), this new technology permits the rapid and automated quantification of phenotypic resistance for all known and candidate antiretroviral drugs targeting all viral enzymes (PR, RT, including polymerase and RNase H activities, and IN), some of the current and potential assembly inhibitors, and any drug targeting Pol or Gag precursor cleavage sites (relevant for PI and maturation inhibitors) This novel assay may be instrumental (i) in the development and clinical assessment of novel ARV drugs and (ii) to monitor patients failing prior complex treatment regimens.

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