Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein

The tumor necrosis factor (TNF) superfamily is composed by several proteins with similar structure and functions. One of the main representatives of this family is TNF-alpha (TNFα), a proinflammatory cytokine which is produced by different immune cells and presents a wide variety of activities. Usin...

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Published in:Molecular Immunology
Main Authors: Ordás, M. C., Costa, M. M., Roca, F. J., López-Castejón, G., Mulero, V., Meseguer, J., Figueras, A., Novoa, B.
Format: Article in Journal/Newspaper
Language:English
Published: 2007
Subjects:
TNF
Online Access:https://research.manchester.ac.uk/en/publications/4fa405c2-b373-489d-9ad7-c4cda8aeed15
https://doi.org/10.1016/j.molimm.2006.02.028
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spelling ftumanchesterpub:oai:pure.atira.dk:publications/4fa405c2-b373-489d-9ad7-c4cda8aeed15 2023-11-12T04:27:40+01:00 Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein Ordás, M. C. Costa, M. M. Roca, F. J. López-Castejón, G. Mulero, V. Meseguer, J. Figueras, A. Novoa, B. 2007-01 https://research.manchester.ac.uk/en/publications/4fa405c2-b373-489d-9ad7-c4cda8aeed15 https://doi.org/10.1016/j.molimm.2006.02.028 eng eng info:eu-repo/semantics/closedAccess Ordás , M C , Costa , M M , Roca , F J , López-Castejón , G , Mulero , V , Meseguer , J , Figueras , A & Novoa , B 2007 , ' Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein ' , Molecular immunology , vol. 44 , no. 4 , pp. 389-400 . https://doi.org/10.1016/j.molimm.2006.02.028 Gene expression Inflamation Recombinant protein Sea bream TNF Tumor necrosis factor Turbot VHSV Vibrio pelagius Virus article 2007 ftumanchesterpub https://doi.org/10.1016/j.molimm.2006.02.028 2023-10-30T09:11:54Z The tumor necrosis factor (TNF) superfamily is composed by several proteins with similar structure and functions. One of the main representatives of this family is TNF-alpha (TNFα), a proinflammatory cytokine which is produced by different immune cells and presents a wide variety of activities. Using the RACE technique, we have cloned and sequenced the turbot TNF cDNA. The analysis of its sequence showed several conserved motifs characteristic of members of the TNFα family. A phylogenetic tree constructed with different TNFs of fish and mammals grouped our sequence within the fish TNFα cluster. Therefore, the turbot TNF here studied was identified as TNFα. The complete TNFα gene was obtained by gene walking, and, similarly to the other known fish TNFα genes, presented three introns and four exons. A PCR was designed to study the turbot TNFα expression in vivo using as stimulus the bacteria Vibrio pelagius strain Hq222 and virus VHSV. The expression of the cytokine happened early after injection, and it was dependent on the pathogen injected and organ analyzed. Virus induced a higher TNFα expression, but this response was shorter in time than that induced by bacteria. In addition, TNFα expression was in general higher in kidney than in liver, as expected since the former is the haematopoietic organ of fish. The turbot recombinant TNFα (rTNFα) was obtained by IPTG induction of bacteria transformed with the pET15b-TNFα construct, and it was purified in native conditions. The recombinant protein was approximately 20 kDa in size, and its biological activity was assessed in vitro. No effect of the rTNFα neither alone nor in combination with LPS was observed on the chemiluminescence activity of turbot macrophages at any time tested. However, NO production was enhanced by the recombinant protein alone or with LPS 72 h after the addition of the treatments. Finally, turbot rTNFα was able to recruit and activate inflammatory cells when injected in gilthead seabream, although to a lesser extent than gilthead seabream rTNFα. ... Article in Journal/Newspaper Turbot The University of Manchester: Research Explorer Molecular Immunology 44 4 389 400
institution Open Polar
collection The University of Manchester: Research Explorer
op_collection_id ftumanchesterpub
language English
topic Gene expression
Inflamation
Recombinant protein
Sea bream
TNF
Tumor necrosis factor
Turbot
VHSV
Vibrio pelagius
Virus
spellingShingle Gene expression
Inflamation
Recombinant protein
Sea bream
TNF
Tumor necrosis factor
Turbot
VHSV
Vibrio pelagius
Virus
Ordás, M. C.
Costa, M. M.
Roca, F. J.
López-Castejón, G.
Mulero, V.
Meseguer, J.
Figueras, A.
Novoa, B.
Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein
topic_facet Gene expression
Inflamation
Recombinant protein
Sea bream
TNF
Tumor necrosis factor
Turbot
VHSV
Vibrio pelagius
Virus
description The tumor necrosis factor (TNF) superfamily is composed by several proteins with similar structure and functions. One of the main representatives of this family is TNF-alpha (TNFα), a proinflammatory cytokine which is produced by different immune cells and presents a wide variety of activities. Using the RACE technique, we have cloned and sequenced the turbot TNF cDNA. The analysis of its sequence showed several conserved motifs characteristic of members of the TNFα family. A phylogenetic tree constructed with different TNFs of fish and mammals grouped our sequence within the fish TNFα cluster. Therefore, the turbot TNF here studied was identified as TNFα. The complete TNFα gene was obtained by gene walking, and, similarly to the other known fish TNFα genes, presented three introns and four exons. A PCR was designed to study the turbot TNFα expression in vivo using as stimulus the bacteria Vibrio pelagius strain Hq222 and virus VHSV. The expression of the cytokine happened early after injection, and it was dependent on the pathogen injected and organ analyzed. Virus induced a higher TNFα expression, but this response was shorter in time than that induced by bacteria. In addition, TNFα expression was in general higher in kidney than in liver, as expected since the former is the haematopoietic organ of fish. The turbot recombinant TNFα (rTNFα) was obtained by IPTG induction of bacteria transformed with the pET15b-TNFα construct, and it was purified in native conditions. The recombinant protein was approximately 20 kDa in size, and its biological activity was assessed in vitro. No effect of the rTNFα neither alone nor in combination with LPS was observed on the chemiluminescence activity of turbot macrophages at any time tested. However, NO production was enhanced by the recombinant protein alone or with LPS 72 h after the addition of the treatments. Finally, turbot rTNFα was able to recruit and activate inflammatory cells when injected in gilthead seabream, although to a lesser extent than gilthead seabream rTNFα. ...
format Article in Journal/Newspaper
author Ordás, M. C.
Costa, M. M.
Roca, F. J.
López-Castejón, G.
Mulero, V.
Meseguer, J.
Figueras, A.
Novoa, B.
author_facet Ordás, M. C.
Costa, M. M.
Roca, F. J.
López-Castejón, G.
Mulero, V.
Meseguer, J.
Figueras, A.
Novoa, B.
author_sort Ordás, M. C.
title Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein
title_short Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein
title_full Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein
title_fullStr Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein
title_full_unstemmed Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein
title_sort turbot tnfα gene: molecular characterization and biological activity of the recombinant protein
publishDate 2007
url https://research.manchester.ac.uk/en/publications/4fa405c2-b373-489d-9ad7-c4cda8aeed15
https://doi.org/10.1016/j.molimm.2006.02.028
genre Turbot
genre_facet Turbot
op_source Ordás , M C , Costa , M M , Roca , F J , López-Castejón , G , Mulero , V , Meseguer , J , Figueras , A & Novoa , B 2007 , ' Turbot TNFα gene: Molecular characterization and biological activity of the recombinant protein ' , Molecular immunology , vol. 44 , no. 4 , pp. 389-400 . https://doi.org/10.1016/j.molimm.2006.02.028
op_rights info:eu-repo/semantics/closedAccess
op_doi https://doi.org/10.1016/j.molimm.2006.02.028
container_title Molecular Immunology
container_volume 44
container_issue 4
container_start_page 389
op_container_end_page 400
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