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基于进化和 X 射线晶体学的表面活性剂蛋白 D 诱变增强了体内对甲型流感病毒的防御。

Mutagenesis of surfactant protein D informed by evolution and x-ray crystallography enhances defenses against influenza A virus in vivo.

机构信息

Department of Pathology and Immunology, Washington University School of Medicine, St. Louis, Missouri 63110, USA.

出版信息

J Biol Chem. 2011 Nov 25;286(47):40681-92. doi: 10.1074/jbc.M111.300673. Epub 2011 Sep 30.

DOI:10.1074/jbc.M111.300673
PMID:21965658
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3220461/
Abstract

The recognition of influenza A virus (IAV) by surfactant protein D (SP-D) is mediated by interactions between the SP-D carbohydrate recognition domains (CRD) and glycans displayed on envelope glycoproteins. Although native human SP-D shows potent antiviral and aggregating activity, trimeric recombinant neck+CRDs (NCRDs) show little or no capacity to influence IAV infection. A mutant trimeric NCRD, D325A/R343V, showed marked hemagglutination inhibition and viral neutralization, with viral aggregation and aggregation-dependent viral uptake by neutrophils. D325A/R343V exhibited glucose-sensitive binding to Phil82 hemagglutinin trimer (HA) by surface plasmon resonance. By contrast, there was very low binding to the HA trimer from another virus (PR8) that lacks glycans on the HA head. Mass spectrometry demonstrated the presence of high mannose glycans on the Phil82 HA at positions known to contribute to IAV binding. Molecular modeling predicted an enhanced capacity for bridging interactions between HA glycans and D325A/R343V. Finally, the trimeric D325A/R343V NCRD decreased morbidity and increased viral clearance in a murine model of IAV infection using a reassortant A/WSN/33 virus with a more heavily glycosylated HA. The combined data support a model in which altered binding by a truncated mutant SP-D to IAV HA glycans facilitates viral aggregation, leading to significant viral neutralization in vitro and in vivo. These studies demonstrate the potential utility of homology modeling and protein structure analysis for engineering effective collectin antivirals as in vivo therapeutics.

摘要

肺泡表面活性物质蛋白 D(SP-D)通过 SP-D 糖识别域(CRD)与包膜糖蛋白上展示的糖基相互作用来识别甲型流感病毒(IAV)。尽管天然人 SP-D 表现出强大的抗病毒和聚集活性,但三聚体重组颈+CRD(NCRD)几乎没有或没有能力影响 IAV 感染。一种突变的三聚体 NCRD,D325A/R343V,表现出明显的血凝抑制和病毒中和作用,具有病毒聚集作用,并通过中性粒细胞依赖聚集的病毒摄取作用。D325A/R343V 通过表面等离子体共振显示出对 Phil82 血凝素三聚体(HA)的葡萄糖敏感结合。相比之下,对缺乏 HA 头部糖基的另一种病毒(PR8)的 HA 三聚体的结合非常低。质谱法证明了 Phil82 HA 上的高甘露糖糖基的存在,这些位置已知有助于 IAV 结合。分子建模预测了 D325A/R343V 与 HA 糖基之间桥接相互作用的增强能力。最后,三聚体 D325A/R343V NCRD 减少了使用带有更重糖基化 HA 的重配 A/WSN/33 病毒的 IAV 感染的小鼠模型中的发病率并增加了病毒清除率。综合数据支持了这样一种模型,即截短突变 SP-D 对 IAV HA 糖基的改变结合促进了病毒聚集,从而导致体外和体内的显著病毒中和。这些研究表明,同源建模和蛋白质结构分析在工程有效集落素抗病毒剂作为体内治疗剂方面具有潜在的应用价值。

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