A modification to heptad repeat 1 of gp41 improves yield and/or quality of soluble pre-fusion HIV-1 envelope glycoprotein trimers.

IF 3.8 2区医学 Q2 VIROLOGY

Journal of Virology Pub Date : 2025-09-23 Epub Date: 2025-08-27 DOI:10.1128/jvi.00913-25

Devidas N Chaturbhuj, Kwinten Sliepen, Albert Cupo, Benjamin Steinberg, Simon Kazimierczyk, Tarek Munawar, Kyle Kramer, Anila Yasmeen, Thales G Andrade, Wen-Hsin Lee, Lara van der Maas, Grace Gibson, Oscar Feliciano, Ivan Del Moral Sanchez, Edith Schermer, Rhianna Bronson, Alison Benner, Madhu Prabhakaran, Rosemarie Mason, P J Klasse, Andrew B Ward, Gabriel Ozorowski, Rogier W Sanders, John P Moore

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引用次数: 0

Abstract

Native-like HIV-1 envelope glycoprotein (Env) trimers, exemplified by the SOSIP design, are widely used as immunogens, analytical antigens, and for structural studies. These vaccine research and development programs require trimers that are based on multiple HIV-1 genotypes. While a wide range of protein engineering strategies can produce SOSIP trimers from most Env gene sequences, there are still examples of trimers that are expressed only at impractically low yields or that are unstable. Accordingly, additional protein modifications aimed at overcoming such limitations need to be evaluated. Here, we describe a new heptad repeat 1 modification of gp41, known as dPG, that helps to further stabilize the gp41 component of prototypic and germline-targeting SOSIP trimers in the pre-fusion state and thereby increases post-purification yields substantially. The dPG modification involves a deletion (d) at the highly conserved 566 position that disrupts the heptad repeat and introduces proline (P) and glycine (G) substitutions at positions 567 and 568, respectively. We show that the dPG strategy reinforces previously described stabilization changes in existing SOSIP trimers and can rescue otherwise problematic trimer constructs. The latter includes trimers used to target or analyze human germline antibodies and others derived from the global HIV-1 neutralization panel. In summary, the dPG modification strategy can increase the yield and/or quality of Env trimers that are otherwise difficult to produce.

Importance: Stabilized, soluble, pre-fusion SOSIP trimers are widely used in HIV-1 Env vaccine research. Protein engineering techniques have identified multiple ways to stabilize SOSIP trimers from a range of genotypes. However, some SOSIP trimers remain difficult to express at adequate yields and/or purity, so there is a need for additional modifications. Here, we identified a sequence change, designated dPG, to the gp41 subunit that increases the yield and/or quality of various otherwise problematic SOSIP trimers without compromising their antigenicity or structure. This new modification may have general value for HIV-1 vaccine research and development.

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对gp41的七磷酸重复1的修饰提高了可溶性预融合HIV-1包膜糖蛋白三聚体的产量和/或质量。

以SOSIP设计为例，原生样HIV-1包膜糖蛋白（Env）三聚体被广泛用作免疫原、分析抗原和结构研究。这些疫苗研究和开发项目需要基于多种HIV-1基因型的三聚体。虽然各种各样的蛋白质工程策略可以从大多数Env基因序列中产生SOSIP三聚体，但仍有三聚体的例子只能以不切实际的低产量表达或不稳定。因此，需要评估旨在克服这些限制的其他蛋白质修饰。在这里，我们描述了gp41的一种新的七tad重复1修饰，称为dPG，有助于进一步稳定原型和种系靶向SOSIP三聚体在融合前状态的gp41成分，从而大大提高纯化后的产量。dPG修饰涉及高度保守的566位的缺失(d)，该缺失破坏了七肽重复，并分别在567位和568位引入脯氨酸(P)和甘氨酸(G)取代。我们发现dPG策略加强了先前描述的现有SOSIP三聚体的稳定化变化，并可以挽救其他有问题的三聚体结构。后者包括用于靶向或分析人类种系抗体和其他来自全球HIV-1中和小组的三聚体。总之，dPG修饰策略可以提高难以生产的Env三聚体的产量和/或质量。重要性：稳定的、可溶的、预融合的SOSIP三聚体广泛用于HIV-1 Env疫苗研究。蛋白质工程技术已经确定了多种方法来稳定来自一系列基因型的SOSIP三聚体。然而，一些SOSIP三聚体仍然难以以足够的产量和/或纯度表达，因此需要进行额外的修饰。在这里，我们发现了gp41亚基的序列变化，称为dPG，可以在不影响其抗原性或结构的情况下提高各种有问题的SOSIP三聚体的产量和/或质量。这种新的修改可能对HIV-1疫苗的研究和开发具有普遍价值。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Journal of Virology 医学-病毒学

CiteScore

10.10

自引率

7.40%

发文量

906

审稿时长

1 months

期刊介绍： Journal of Virology (JVI) explores the nature of the viruses of animals, archaea, bacteria, fungi, plants, and protozoa. We welcome papers on virion structure and assembly, viral genome replication and regulation of gene expression, genetic diversity and evolution, virus-cell interactions, cellular responses to infection, transformation and oncogenesis, gene delivery, viral pathogenesis and immunity, and vaccines and antiviral agents.