Visualization of the Npro protein in living cells using biarsenically labeling tetracysteine-tagged classical swine fever virus

•We generated CSFV mutants bearing the tetracysteine tag in the Npro protein.•Biarsenical labeling resulted in fluorescent Npro protein in CSFV-infected cells.•Labeled Npro was localized in the cytoplasm at 27 hpi and in the nucleus at 48 hpi.•Real-time Npro nuclear import and export from 36.5 to 37...

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Published in:Virus research 2014-08, Vol.189, p.67-74
Main Authors: Li, Yongfeng, Shen, Liang, Li, Chao, Huang, Junhua, Zhao, Bibo, Sun, Yuan, Li, Su, Luo, Yuzi, Qiu, Hua-Ji
Format: Article
Language:English
Subjects:
Animals
Cell Line
Cell Nucleus - chemistry
Classical swine fever virus
Classical swine fever virus - enzymology
Cytoplasm - chemistry
Endopeptidases - analysis
Npro protein
Optical Imaging - methods
Real-time fluorescence imaging
Swine
Tetracysteine tag
Viral Proteins - analysis
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cited_by cdi_FETCH-LOGICAL-c2469-a4c3cf5e08e135b34191c3061339e932b28f226272a1517b43f940fa51450433
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container_end_page 74
container_issue
container_start_page 67
container_title Virus research
container_volume 189
creator Li, Yongfeng
Shen, Liang
Li, Chao
Huang, Junhua
Zhao, Bibo
Sun, Yuan
Li, Su
Luo, Yuzi
Qiu, Hua-Ji
description •We generated CSFV mutants bearing the tetracysteine tag in the Npro protein.•Biarsenical labeling resulted in fluorescent Npro protein in CSFV-infected cells.•Labeled Npro was localized in the cytoplasm at 27 hpi and in the nucleus at 48 hpi.•Real-time Npro nuclear import and export from 36.5 to 37 hpi was visualized.•Npro protein transported into the nucleus by passive diffusion. Real-time fluorescence imaging of viral proteins in living cells is a valuable means to study virus–host interactions, and tetracysteine (TC)-biarsenical technology has been used in several viruses but not in classical swine fever virus (CSFV). Here, we generated CSFV mutants vSMTC385 or vSMTC412 bearing the small TC tag (CCPGCC) in the N-terminal region of the Npro protein. The mutants showed growth characteristics indistinguishable from that of the wild-type virus, and retained similar Npro subcellular localization to that of the parent virus. Furthermore, labeling with membrane-permeable biarsenical dye resulted in the fluorescent Npro protein in the context of virus infection. Finally, we showed that Npro was localized in the cytoplasm of CSFV-infected cells at 27h post-infection (hpi) and present in the nucleus at 48 hpi, and the nuclear import and export was clearly observed from 36.5 to 37 hpi. Interestingly, our results demonstrated that Npro transported across the nuclear pores by passive diffusion, which might be prevented by exogenous interferon regulatory factor 3 interacting with Npro. Taken together, biarsenical labeling allows real-time visualization of the nucleus import and export of the fluorescent Npro protein in CSFV-infected living cells.
doi_str_mv 10.1016/j.virusres.2014.04.018
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Real-time fluorescence imaging of viral proteins in living cells is a valuable means to study virus–host interactions, and tetracysteine (TC)-biarsenical technology has been used in several viruses but not in classical swine fever virus (CSFV). Here, we generated CSFV mutants vSMTC385 or vSMTC412 bearing the small TC tag (CCPGCC) in the N-terminal region of the Npro protein. The mutants showed growth characteristics indistinguishable from that of the wild-type virus, and retained similar Npro subcellular localization to that of the parent virus. Furthermore, labeling with membrane-permeable biarsenical dye resulted in the fluorescent Npro protein in the context of virus infection. Finally, we showed that Npro was localized in the cytoplasm of CSFV-infected cells at 27h post-infection (hpi) and present in the nucleus at 48 hpi, and the nuclear import and export was clearly observed from 36.5 to 37 hpi. Interestingly, our results demonstrated that Npro transported across the nuclear pores by passive diffusion, which might be prevented by exogenous interferon regulatory factor 3 interacting with Npro. Taken together, biarsenical labeling allows real-time visualization of the nucleus import and export of the fluorescent Npro protein in CSFV-infected living cells.</description><identifier>ISSN: 0168-1702</identifier><identifier>EISSN: 1872-7492</identifier><identifier>DOI: 10.1016/j.virusres.2014.04.018</identifier><identifier>PMID: 24815879</identifier><language>eng</language><publisher>Netherlands: Elsevier B.V</publisher><subject>Animals ; Cell Line ; Cell Nucleus - chemistry ; Classical swine fever virus ; Classical swine fever virus - enzymology ; Cytoplasm - chemistry ; Endopeptidases - analysis ; Npro protein ; Optical Imaging - methods ; Real-time fluorescence imaging ; Swine ; Tetracysteine tag ; Viral Proteins - analysis</subject><ispartof>Virus research, 2014-08, Vol.189, p.67-74</ispartof><rights>2014 Elsevier B.V.</rights><rights>Copyright © 2014 Elsevier B.V. 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Real-time fluorescence imaging of viral proteins in living cells is a valuable means to study virus–host interactions, and tetracysteine (TC)-biarsenical technology has been used in several viruses but not in classical swine fever virus (CSFV). Here, we generated CSFV mutants vSMTC385 or vSMTC412 bearing the small TC tag (CCPGCC) in the N-terminal region of the Npro protein. The mutants showed growth characteristics indistinguishable from that of the wild-type virus, and retained similar Npro subcellular localization to that of the parent virus. Furthermore, labeling with membrane-permeable biarsenical dye resulted in the fluorescent Npro protein in the context of virus infection. Finally, we showed that Npro was localized in the cytoplasm of CSFV-infected cells at 27h post-infection (hpi) and present in the nucleus at 48 hpi, and the nuclear import and export was clearly observed from 36.5 to 37 hpi. Interestingly, our results demonstrated that Npro transported across the nuclear pores by passive diffusion, which might be prevented by exogenous interferon regulatory factor 3 interacting with Npro. 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Real-time fluorescence imaging of viral proteins in living cells is a valuable means to study virus–host interactions, and tetracysteine (TC)-biarsenical technology has been used in several viruses but not in classical swine fever virus (CSFV). Here, we generated CSFV mutants vSMTC385 or vSMTC412 bearing the small TC tag (CCPGCC) in the N-terminal region of the Npro protein. The mutants showed growth characteristics indistinguishable from that of the wild-type virus, and retained similar Npro subcellular localization to that of the parent virus. Furthermore, labeling with membrane-permeable biarsenical dye resulted in the fluorescent Npro protein in the context of virus infection. Finally, we showed that Npro was localized in the cytoplasm of CSFV-infected cells at 27h post-infection (hpi) and present in the nucleus at 48 hpi, and the nuclear import and export was clearly observed from 36.5 to 37 hpi. 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subjects Animals
Cell Line
Cell Nucleus - chemistry
Classical swine fever virus
Classical swine fever virus - enzymology
Cytoplasm - chemistry
Endopeptidases - analysis
Npro protein
Optical Imaging - methods
Real-time fluorescence imaging
Swine
Tetracysteine tag
Viral Proteins - analysis
title Visualization of the Npro protein in living cells using biarsenically labeling tetracysteine-tagged classical swine fever virus
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