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一种酵母糖蛋白对广泛中和性的人类免疫缺陷病毒抗体2G12表现出高亲和力结合,并抑制gp120与2G12和DC-SIGN的相互作用。

A yeast glycoprotein shows high-affinity binding to the broadly neutralizing human immunodeficiency virus antibody 2G12 and inhibits gp120 interactions with 2G12 and DC-SIGN.

作者信息

Luallen Robert J, Fu Hu, Agrawal-Gamse Caroline, Mboudjeka Innocent, Huang Wei, Lee Fang-Hua, Wang Lai-Xi, Doms Robert W, Geng Yu

机构信息

ProSci Inc., 12170 Flint Place, Poway, CA 92064, USA.

出版信息

J Virol. 2009 May;83(10):4861-70. doi: 10.1128/JVI.02537-08. Epub 2009 Mar 4.

Abstract

The human immunodeficiency virus type 1 (HIV-1) envelope (Env) protein contains numerous N-linked carbohydrates that shield conserved peptide epitopes and promote trans infection by dendritic cells via binding to cell surface lectins. The potent and broadly neutralizing monoclonal antibody 2G12 binds a cluster of high-mannose-type oligosaccharides on the gp120 subunit of Env, revealing a conserved and highly exposed epitope on the glycan shield. To find an effective antigen for eliciting 2G12-like antibodies, we searched for endogenous yeast proteins that could bind to 2G12 in a panel of Saccharomyces cerevisiae glycosylation knockouts and discovered one protein that bound weakly in a Delta pmr1 strain deficient in hyperglycosylation. 2G12 binding to this protein, identified as Pst1, was enhanced by adding the Delta mnn1 deletion to the Delta pmr1 background, ensuring the exposure of terminal alpha1,2-linked mannose residues on the D1 and D3 arms of high-mannose glycans. However, optimum 2G12 antigenicity was found when Pst1, a heavily N-glycosylated protein, was expressed with homogenous Man(8)GlcNAc(2) structures in Delta och1 Delta mnn1 Delta mnn4 yeast. Surface plasmon resonance analysis of this form of Pst1 showed high affinity for 2G12, which translated into Pst1 efficiently inhibiting gp120 interactions with 2G12 and DC-SIGN and blocking 2G12-mediated neutralization of HIV-1 pseudoviruses. The high affinity of the yeast glycoprotein Pst1 for 2G12 highlights its potential as a novel antigen to induce 2G12-like antibodies.

摘要

1型人类免疫缺陷病毒(HIV-1)包膜(Env)蛋白含有大量N-连接碳水化合物,这些碳水化合物会屏蔽保守的肽表位,并通过与细胞表面凝集素结合促进树突状细胞的转染。强效且具有广泛中和作用的单克隆抗体2G12可结合Env的gp120亚基上的一组高甘露糖型寡糖,从而在聚糖屏蔽上揭示一个保守且高度暴露的表位。为了找到一种能引发2G12样抗体的有效抗原,我们在一组酿酒酵母糖基化基因敲除菌株中寻找能与2G12结合的内源性酵母蛋白,并发现一种在高糖基化缺陷的Δpmr1菌株中结合较弱的蛋白。在Δpmr1背景中添加Δmnn1缺失可增强2G12与这种被鉴定为Pst1的蛋白的结合,确保高甘露糖聚糖的D1和D3臂上末端α1,2-连接的甘露糖残基暴露。然而,当在Δoch1Δmnn1Δmnn4酵母中以均一的Man(8)GlcNAc(2)结构表达高度N-糖基化的蛋白Pst1时,发现其具有最佳的2G12抗原性。这种形式的Pst1的表面等离子体共振分析显示其对2G12具有高亲和力,这转化为Pst1能有效抑制gp120与2G12和DC-SIGN的相互作用,并阻断2G12介导的HIV-1假病毒中和作用。酵母糖蛋白Pst1对2G12的高亲和力突出了其作为诱导2G12样抗体的新型抗原的潜力。

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