TY - JOUR
T1 - Impact of HIV-1 backbone on neutralization sensitivity
T2 - Neutralization profiles of heterologous envelope glycoproteins expressed in native subtype C and CRF01-AE backbone
AU - Chenine, Agnès Laurence
AU - Wieczorek, Lindsay
AU - Sanders-Buell, Eric
AU - Wesberry, Maggie
AU - Towle, Teresa
AU - Pillis, Devin M.
AU - Molnar, Sebastian
AU - McLinden, Robert
AU - Edmonds, Tara
AU - Hirsch, Ivan
AU - O'Connell, Robert
AU - McCutchan, Francine E.
AU - Montefiori, David C.
AU - Ochsenbauer, Christina
AU - Kappes, John C.
AU - Kim, Jerome H.
AU - Polonis, Victoria R.
AU - Tovanabutra, Sodsai
PY - 2013/11/29
Y1 - 2013/11/29
N2 - Standardized assays to assess vaccine and antiviral drug efficacy are critical for the development of protective HIV-1 vaccines and drugs. These immune assays will be advanced by the development of standardized viral stocks, such as HIV-1 infectious molecular clones (IMC), that i) express a reporter gene, ii) are representative of globally diverse subtypes and iii) are engineered to easily exchange envelope (env) genes for expression of sequences of interest. Thus far, a subtype B IMC backbone expressing Renilla luciferase (LucR), and into which the ectodomain of heterologous env coding sequences can be expressed has been successfully developed but as execution of HIV-1 vaccine efficacy trials shifts increasingly to non-subtype B epidemics (Southern African and Southeast Asia), non-subtype B HIV-1 reagents are needed to support vaccine development. Here we describe two IMCs derived from subtypes C and CRF01-AE HIV-1 primary isolates expressing LucR (IMC.LucR) that were engineered to express heterologous gp160 Envs. 18 constructs expressing various subtypes C and CRF01-AE Envs, mostly acute, in subtype-matched and -unmatched HIV backbones were tested for functionality and neutralization sensitivity. Our results suggest a possible effect of non-env HIV-1 genes on the interaction of Env and neutralizing antibodies and highlight the need to generate a library of IMCs representative of the HIV-1 subtype spectrum to be used as standardized neutralization assay reagents for assessing HIV-1 vaccine efficacy.
AB - Standardized assays to assess vaccine and antiviral drug efficacy are critical for the development of protective HIV-1 vaccines and drugs. These immune assays will be advanced by the development of standardized viral stocks, such as HIV-1 infectious molecular clones (IMC), that i) express a reporter gene, ii) are representative of globally diverse subtypes and iii) are engineered to easily exchange envelope (env) genes for expression of sequences of interest. Thus far, a subtype B IMC backbone expressing Renilla luciferase (LucR), and into which the ectodomain of heterologous env coding sequences can be expressed has been successfully developed but as execution of HIV-1 vaccine efficacy trials shifts increasingly to non-subtype B epidemics (Southern African and Southeast Asia), non-subtype B HIV-1 reagents are needed to support vaccine development. Here we describe two IMCs derived from subtypes C and CRF01-AE HIV-1 primary isolates expressing LucR (IMC.LucR) that were engineered to express heterologous gp160 Envs. 18 constructs expressing various subtypes C and CRF01-AE Envs, mostly acute, in subtype-matched and -unmatched HIV backbones were tested for functionality and neutralization sensitivity. Our results suggest a possible effect of non-env HIV-1 genes on the interaction of Env and neutralizing antibodies and highlight the need to generate a library of IMCs representative of the HIV-1 subtype spectrum to be used as standardized neutralization assay reagents for assessing HIV-1 vaccine efficacy.
UR - http://www.scopus.com/inward/record.url?scp=84896694686&partnerID=8YFLogxK
U2 - 10.1371/journal.pone.0076104
DO - 10.1371/journal.pone.0076104
M3 - Article
C2 - 24312165
AN - SCOPUS:84896694686
SN - 1932-6203
VL - 8
JO - PLoS ONE
JF - PLoS ONE
IS - 11
M1 - e76104
ER -