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Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance

A tier 2 SHIV-MK38 strain was obtained after two in vivo passages of tier 1 SHIV-MK1. SHIV-MK38#818, cloned from the MK38 strain, was neutralisation-resistant, like the parental MK38 strain, to SHIV-infected monkey plasma (MP), HIV-1-infected human pooled plasma (HPP), and KD247 monoclonal antibody...

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Autores principales: Pisil, Yalcin, Yazici, Zafer, Shida, Hisatoshi, Matsushita, Shuzo, Miura, Tomoyuki
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2020
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7157653/
https://www.ncbi.nlm.nih.gov/pubmed/32138199
http://dx.doi.org/10.3390/pathogens9030181
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author Pisil, Yalcin
Yazici, Zafer
Shida, Hisatoshi
Matsushita, Shuzo
Miura, Tomoyuki
author_facet Pisil, Yalcin
Yazici, Zafer
Shida, Hisatoshi
Matsushita, Shuzo
Miura, Tomoyuki
author_sort Pisil, Yalcin
collection PubMed
description A tier 2 SHIV-MK38 strain was obtained after two in vivo passages of tier 1 SHIV-MK1. SHIV-MK38#818, cloned from the MK38 strain, was neutralisation-resistant, like the parental MK38 strain, to SHIV-infected monkey plasma (MP), HIV-1-infected human pooled plasma (HPP), and KD247 monoclonal antibody (mAb) (anti-V3 gp120 env). We investigated the mechanisms underlying the resistance of #818, specifically the amino acid substitutions that confer resistance to MK1. We introduced amino acid substitutions in the MK1 envelope by in vitro mutagenesis and then compared the neutralisation resistance to MP, HPP, and KD247 mAb with #818 in a neutralisation assay using TZM-bl cells. We selected 11 substitutions in the V1, V2, C2, V4, C4, and V5 regions based on the alignment of env of MK1 and #818. The neutralisation resistance of the mutant MK1s with 7 of 11 substitutions in the V1, C2, C4, and V5 regions did not change significantly. These substitutions did not alter any negative charges or N-glycans. The substitutions N169D and K187E, which added negative charges, and S190N in the V2 region of gp120 and A389T in V4, which created sites for N-glycan, conferred high neutralisation resistance. The combinations N169D+K187E, N169D+S190N, and N169D+A389T resulted in MK1 neutralisation resistance close to that of #818. The combinations without 169D were neutralisation-sensitive. Therefore, N169D is the most important substitution for neutralisation resistance. This study demonstrated that although the V3 region sequences of #818 and MK1 are the same, V3 binding antibodies cannot neutralise #818 pseudovirus. Instead, mutations in the V2 and V4 regions inhibit the neutralisation of anti-V3 antibodies. We hypothesised that 169D and 190N altered the MK1 Env conformation so that the V3 region is buried. Therefore, the V2 region may block KD247 from binding to the tip of the V3 region.
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spelling pubmed-71576532020-05-01 Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance Pisil, Yalcin Yazici, Zafer Shida, Hisatoshi Matsushita, Shuzo Miura, Tomoyuki Pathogens Article A tier 2 SHIV-MK38 strain was obtained after two in vivo passages of tier 1 SHIV-MK1. SHIV-MK38#818, cloned from the MK38 strain, was neutralisation-resistant, like the parental MK38 strain, to SHIV-infected monkey plasma (MP), HIV-1-infected human pooled plasma (HPP), and KD247 monoclonal antibody (mAb) (anti-V3 gp120 env). We investigated the mechanisms underlying the resistance of #818, specifically the amino acid substitutions that confer resistance to MK1. We introduced amino acid substitutions in the MK1 envelope by in vitro mutagenesis and then compared the neutralisation resistance to MP, HPP, and KD247 mAb with #818 in a neutralisation assay using TZM-bl cells. We selected 11 substitutions in the V1, V2, C2, V4, C4, and V5 regions based on the alignment of env of MK1 and #818. The neutralisation resistance of the mutant MK1s with 7 of 11 substitutions in the V1, C2, C4, and V5 regions did not change significantly. These substitutions did not alter any negative charges or N-glycans. The substitutions N169D and K187E, which added negative charges, and S190N in the V2 region of gp120 and A389T in V4, which created sites for N-glycan, conferred high neutralisation resistance. The combinations N169D+K187E, N169D+S190N, and N169D+A389T resulted in MK1 neutralisation resistance close to that of #818. The combinations without 169D were neutralisation-sensitive. Therefore, N169D is the most important substitution for neutralisation resistance. This study demonstrated that although the V3 region sequences of #818 and MK1 are the same, V3 binding antibodies cannot neutralise #818 pseudovirus. Instead, mutations in the V2 and V4 regions inhibit the neutralisation of anti-V3 antibodies. We hypothesised that 169D and 190N altered the MK1 Env conformation so that the V3 region is buried. Therefore, the V2 region may block KD247 from binding to the tip of the V3 region. MDPI 2020-03-03 /pmc/articles/PMC7157653/ /pubmed/32138199 http://dx.doi.org/10.3390/pathogens9030181 Text en © 2020 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Pisil, Yalcin
Yazici, Zafer
Shida, Hisatoshi
Matsushita, Shuzo
Miura, Tomoyuki
Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance
title Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance
title_full Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance
title_fullStr Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance
title_full_unstemmed Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance
title_short Specific Substitutions in Region V2 of gp120 env confer SHIV Neutralisation Resistance
title_sort specific substitutions in region v2 of gp120 env confer shiv neutralisation resistance
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7157653/
https://www.ncbi.nlm.nih.gov/pubmed/32138199
http://dx.doi.org/10.3390/pathogens9030181
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