对源自一株已记录的GII.6诺如病毒株的主要衣壳蛋白进行全面表征。

Comprehensive characterization of a major capsid protein derived from a documented GII.6 norovirus strain.

作者信息

Zheng Lijun, Wang Wenhui, Liu Jinjin, Huo Yuqi, Qin Chuan, Wang Mingchen, Shen Shuo

机构信息

The Sixth People's Hospital of Zhengzhou, No. 29 Jingguangnan Road, Zhengzhou, 450000, People's Republic of China.

Wuhan Institute of Biological Products, Wuhan, People's Republic of China.

出版信息

Arch Virol. 2017 Dec;162(12):3863-3868. doi: 10.1007/s00705-017-3537-4. Epub 2017 Sep 2.

DOI:10.1007/s00705-017-3537-4

PMID:28866835

Abstract

In this study, we successfully produced VLPs derived from full-length or chimeric VP1 of a documented GII.6 strain. Trypsin digestion of purified VLPs led to total cleavage of VP1, while the integrity of assembled VLPs was not affected. In vitro VLP-histo-blood group antigen (HBGA) binding and binding blockade assays indicated that trypsin digestion enhanced the binding of GII.6 VLPs to salivary HBGAs and that this binding could only be blocked by serum produced against a homologous strain. The data regarding the assembly, morphology and binding patterns of GII.6 NoV VLPs presented here might be useful for further study of GII.6 NoVs.

摘要

在本研究中，我们成功制备了源自一株已记录的GII.6毒株全长或嵌合VP1的病毒样颗粒（VLPs）。对纯化的VLPs进行胰蛋白酶消化导致VP1完全裂解，而组装好的VLPs的完整性未受影响。体外VLP-组织血型抗原（HBGA）结合及结合阻断试验表明，胰蛋白酶消化增强了GII.6 VLPs与唾液HBGAs的结合，且这种结合只能被针对同源毒株产生的血清阻断。此处呈现的关于GII.6诺如病毒VLPs的组装、形态和结合模式的数据可能对GII.6诺如病毒的进一步研究有用。

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对源自一株已记录的GII.6诺如病毒株的主要衣壳蛋白进行全面表征。

Comprehensive characterization of a major capsid protein derived from a documented GII.6 norovirus strain.

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