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Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza

Infection of influenza A virus in mammals induces hyper lung pneumonia, which often causes lethal diseases. FasL is a specific ligand of Fas, which is a type-I transmembrane protein to induce cell death. Previously, it has been reported that the hyper induction of gene expression associated with Fas...

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Autores principales: Fujikura, Daisuke, Chiba, Satoko, Muramatsu, Daisuke, Kazumata, Mika, Nakayama, Yosuke, Kawai, Taro, Akira, Shizuo, Kida, Hiroshi, Miyazaki, Tadaaki
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2013
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3568138/
https://www.ncbi.nlm.nih.gov/pubmed/23408968
http://dx.doi.org/10.1371/journal.pone.0055321
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author Fujikura, Daisuke
Chiba, Satoko
Muramatsu, Daisuke
Kazumata, Mika
Nakayama, Yosuke
Kawai, Taro
Akira, Shizuo
Kida, Hiroshi
Miyazaki, Tadaaki
author_facet Fujikura, Daisuke
Chiba, Satoko
Muramatsu, Daisuke
Kazumata, Mika
Nakayama, Yosuke
Kawai, Taro
Akira, Shizuo
Kida, Hiroshi
Miyazaki, Tadaaki
author_sort Fujikura, Daisuke
collection PubMed
description Infection of influenza A virus in mammals induces hyper lung pneumonia, which often causes lethal diseases. FasL is a specific ligand of Fas, which is a type-I transmembrane protein to induce cell death. Previously, it has been reported that the hyper induction of gene expression associated with Fas signal is observed in lethal influenza A virus infection. More importantly, it was also reported that functional mutation of the FasL gene protects the host against influenza A virus infection. These observations suggest that induction of FasL signal is functionally associated with the severity of influenza. However, regulation of the induction of FasL or Fas by influenza A virus infection is still unknown. Here, we demonstrated that FasL is induced after the viral infection, and inhibition of the Fas/FasL signal by treatment with a recombinant decoy receptor for FasL (Fas-Fc) increases the survival rate of mice after lethal infection of influenza A virus as well as functional mutation of the FasL gene in gld/gld mice. In addition, the induction level of FasL gene expression in the lung was correlated with the severity of influenza. We also showed that a variety of types of cells in the lung express FasL after the viral infection. Furthermore, type-I interferon induced by the viral infection was shown to be critical for induction of FasL protein expression in the lung. These findings suggested that expression of FasL protein induced by type-I IFN on the lung cell surface is critical to determine the severity of influenza.
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spelling pubmed-35681382013-02-13 Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza Fujikura, Daisuke Chiba, Satoko Muramatsu, Daisuke Kazumata, Mika Nakayama, Yosuke Kawai, Taro Akira, Shizuo Kida, Hiroshi Miyazaki, Tadaaki PLoS One Research Article Infection of influenza A virus in mammals induces hyper lung pneumonia, which often causes lethal diseases. FasL is a specific ligand of Fas, which is a type-I transmembrane protein to induce cell death. Previously, it has been reported that the hyper induction of gene expression associated with Fas signal is observed in lethal influenza A virus infection. More importantly, it was also reported that functional mutation of the FasL gene protects the host against influenza A virus infection. These observations suggest that induction of FasL signal is functionally associated with the severity of influenza. However, regulation of the induction of FasL or Fas by influenza A virus infection is still unknown. Here, we demonstrated that FasL is induced after the viral infection, and inhibition of the Fas/FasL signal by treatment with a recombinant decoy receptor for FasL (Fas-Fc) increases the survival rate of mice after lethal infection of influenza A virus as well as functional mutation of the FasL gene in gld/gld mice. In addition, the induction level of FasL gene expression in the lung was correlated with the severity of influenza. We also showed that a variety of types of cells in the lung express FasL after the viral infection. Furthermore, type-I interferon induced by the viral infection was shown to be critical for induction of FasL protein expression in the lung. These findings suggested that expression of FasL protein induced by type-I IFN on the lung cell surface is critical to determine the severity of influenza. Public Library of Science 2013-02-08 /pmc/articles/PMC3568138/ /pubmed/23408968 http://dx.doi.org/10.1371/journal.pone.0055321 Text en © 2013 Fujikura et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Fujikura, Daisuke
Chiba, Satoko
Muramatsu, Daisuke
Kazumata, Mika
Nakayama, Yosuke
Kawai, Taro
Akira, Shizuo
Kida, Hiroshi
Miyazaki, Tadaaki
Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza
title Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza
title_full Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza
title_fullStr Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza
title_full_unstemmed Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza
title_short Type-I Interferon is Critical for FasL Expression on Lung Cells to Determine the Severity of Influenza
title_sort type-i interferon is critical for fasl expression on lung cells to determine the severity of influenza
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3568138/
https://www.ncbi.nlm.nih.gov/pubmed/23408968
http://dx.doi.org/10.1371/journal.pone.0055321
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