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Computational design of virus-like protein assemblies on carbon nanotube surfaces.基于碳纳米管表面的病毒样蛋白组装体的计算设计。
Science. 2011 May 27;332(6033):1071-6. doi: 10.1126/science.1198841.
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Cryo-electron microscopy reconstructions of two types of wild rabbit hemorrhagic disease viruses characterized the structural features of Lagovirus.两种野生兔出血症病毒的冷冻电子显微镜重建描绘了 Lagovirus 的结构特征。
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The T=1 capsid protein of Penicillium chrysogenum virus is formed by a repeated helix-rich core indicative of gene duplication.产黄青霉病毒的 T=1 衣壳蛋白由富含重复螺旋的核心组成,表明存在基因复制。
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Conformational changes in the capsid of a calicivirus upon interaction with its functional receptor.衣壳构象在杯状病毒与其功能性受体相互作用时的变化。
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High-resolution cryo-electron microscopy structures of murine norovirus 1 and rabbit hemorrhagic disease virus reveal marked flexibility in the receptor binding domains.高分辨率冷冻电子显微镜结构的鼠诺如病毒 1 和兔出血症病毒揭示受体结合域的显著灵活性。
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High-resolution x-ray structure and functional analysis of the murine norovirus 1 capsid protein protruding domain.高分辨率 X 射线结构和功能分析鼠诺如病毒 1 衣壳蛋白突出结构域。
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Tomato bushy stunt virus at 2.9 A resolution.番茄丛矮病毒,分辨率为2.9埃。
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Structure of the hepatitis E virus-like particle suggests mechanisms for virus assembly and receptor binding.戊型肝炎病毒样颗粒的结构揭示了病毒组装和受体结合的机制。
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兔出血症病毒 T=3 衣壳蛋白 N 端分子开关处的表位插入导致更大的 T=4 衣壳。

Epitope insertion at the N-terminal molecular switch of the rabbit hemorrhagic disease virus T = 3 capsid protein leads to larger T = 4 capsids.

机构信息

Department of Structure of Macromolecules, Centro Nacional de Biotecnología/CSIC, Cantoblanco, Madrid, Spain.

出版信息

J Virol. 2012 Jun;86(12):6470-80. doi: 10.1128/JVI.07050-11. Epub 2012 Apr 4.

DOI:10.1128/JVI.07050-11
PMID:22491457
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3393579/
Abstract

Viruses need only one or a few structural capsid proteins to build an infectious particle. This is possible through the extensive use of symmetry and the conformational polymorphism of the structural proteins. Using virus-like particles (VLP) from rabbit hemorrhagic disease virus (RHDV) as a model, we addressed the basis of calicivirus capsid assembly and their application in vaccine design. The RHDV capsid is based on a T=3 lattice containing 180 identical subunits (VP1). We determined the structure of RHDV VLP to 8.0-Å resolution by three-dimensional cryoelectron microscopy; in addition, we used San Miguel sea lion virus (SMSV) and feline calicivirus (FCV) capsid subunit structures to establish the backbone structure of VP1 by homology modeling and flexible docking analysis. Based on the three-domain VP1 model, several insertion mutants were designed to validate the VP1 pseudoatomic model, and foreign epitopes were placed at the N- or C-terminal end, as well as in an exposed loop on the capsid surface. We selected a set of T and B cell epitopes of various lengths derived from viral and eukaryotic origins. Structural analysis of these chimeric capsids further validates the VP1 model to design new chimeras. Whereas most insertions are well tolerated, VP1 with an FCV capsid protein-neutralizing epitope at the N terminus assembled into mixtures of T=3 and larger T=4 capsids. The calicivirus capsid protein, and perhaps that of many other viruses, thus can encode polymorphism modulators that are not anticipated from the plane sequence, with important implications for understanding virus assembly and evolution.

摘要

病毒仅需一种或几种结构衣壳蛋白即可构建感染性颗粒。这是通过广泛利用对称和结构蛋白的构象多态性来实现的。我们使用兔出血症病毒 (RHDV) 的病毒样颗粒 (VLP) 作为模型,研究了杯状病毒衣壳组装的基础及其在疫苗设计中的应用。RHDV 衣壳基于包含 180 个相同亚基(VP1)的 T=3 晶格。我们通过三维冷冻电子显微镜确定了 RHDV VLP 的结构分辨率为 8.0-Å;此外,我们使用圣米格尔海狮病毒 (SMSV) 和猫杯状病毒 (FCV) 衣壳亚基结构通过同源建模和柔性对接分析建立了 VP1 的骨干结构。基于三域 VP1 模型,设计了几个插入突变体来验证 VP1 拟原子模型,并在衣壳表面的 N 或 C 末端以及暴露环处放置了外源表位。我们选择了一组来自病毒和真核生物来源的不同长度的 T 和 B 细胞表位。这些嵌合衣壳的结构分析进一步验证了 VP1 模型以设计新的嵌合体。虽然大多数插入都能很好地耐受,但在 N 末端具有 FCV 衣壳蛋白中和表位的 VP1 组装成 T=3 和更大的 T=4 衣壳的混合物。杯状病毒衣壳蛋白,也许还有许多其他病毒的衣壳蛋白,因此可以编码多态性调节剂,这些调节剂不能从平面序列中预测,这对理解病毒组装和进化具有重要意义。