[The nuclear import of Newcastle disease virus matrix protein depends on KPNB1 and Ran protein].

微生物学报 Pub Date : 2017-01-04
Zhiqiang Duan, Xinqin Ji, Jouqiang Xu, Jiafu Zhao, Haixu Xu, Shunlin Hu, Xiufan Liu
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引用次数: 0

Abstract

Objective: The aim of this study was to identify the transport proteins that mediates the nuclear import of Newcastle disease virus (NDV) matrix (M) protein.

Methods: Chicken KPNA1 to KPNA6 gene and KPNB1 gene were cloned from DF-1 cells and then inserted into eukaryotic expression vectors. The constructed recombinant plasmids with a combination of grouping were transfected into HEK-293T cells to identify the transport proteins interacting with NDV M protein by co-immunoprecipitation (Co-IP) assay. Moreover, fluorescent co-localization assay was used to verify the transport proteins by co-expressing M and Ran protein mutant or M and its interactive protein deletant.

Results: The recombinant proteins could normally express in plasmid-transfected HEK-293T cells. Indirect immunofluorescence detection showed that the recombinant proteins except for Myc-KPNA2 displayed the same nuclear localization as NDV M protein. The results of Co-IP revealed that M protein could interact with KPNA1 and KPNB1. Further fluorescent co-localization indicated that co-expression of M and DN-KPNA1 did not change the nuclear localization of M, whereas co-expression of M and DN-KPNB1 or M and Ran-Q69L disrupted the nuclear localization of M, demonstrating that the nuclear import of M protein was dependent on KPNB1 and Ran protein.

Conclusion: KPNB1 and Ran protein jointly mediated the nuclear import of NDV M protein, showing that KPNB1 protein interacted with NDV M protein to form binary complex and then entered into the nucleus with the assistance of Ran protein.

[新城疫病毒基质蛋白的核输入取决于KPNB1和Ran蛋白]。
目的:本研究旨在鉴定介导新城疫病毒(NDV)基质(M)蛋白核输入的转运蛋白。方法:从DF-1细胞中克隆鸡KPNA1 ~ KPNA6基因和KPNB1基因,并将其插入真核表达载体中。将组合分组构建的重组质粒转染HEK-293T细胞,用共免疫沉淀法(Co-IP)鉴定与NDV M蛋白相互作用的转运蛋白。此外,采用荧光共定位法通过共表达M和Ran蛋白突变体或M及其相互作用的蛋白缺失来验证转运蛋白。结果:重组蛋白能在转染HEK-293T细胞的质粒中正常表达。间接免疫荧光检测显示,除Myc-KPNA2外,重组蛋白与NDV M蛋白具有相同的核定位。Co-IP结果显示M蛋白可与KPNA1和KPNB1相互作用。进一步的荧光共定位表明,M与DN-KPNA1共表达不会改变M的核定位,而M与DN-KPNB1或M与Ran- q69l共表达会破坏M的核定位,说明M蛋白的核输入依赖于KPNB1和Ran蛋白。结论:KPNB1与Ran蛋白共同介导NDV M蛋白的核输入,表明KPNB1蛋白与NDV M蛋白相互作用形成二元复合物,并在Ran蛋白的协助下进入细胞核。
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
自引率
0.00%
发文量
7960
期刊介绍: Acta Microbiologica Sinica(AMS) is a peer-reviewed monthly (one volume per year)international journal,founded in 1953.It covers a wide range of topics in the areas of general and applied microbiology.The journal publishes original papers,reviews in microbiological science,and short communications describing unusual observations. Acta Microbiologica Sinica has been indexed in Index Copernicus (IC),Chemical Abstract (CA),Excerpt Medica Database (EMBASE),AJ of Viniti (Russia),Biological Abstracts (BA),Chinese Science Citation Database (CSCD),China National Knowledge Infrastructure(CNKI),Institute of Scientific and Technical Information of China(ISTIC),Chinese Journal Citation Report(CJCR),Chinese Biological Abstracts,Chinese Pharmaceutical Abstracts,Chinese Medical Abstracts and Chinese Science Abstracts.
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