Antiviral activity of rChIFN-α against vesicular stomatitis virus and Newcastle disease virus: A novel recombinant chicken interferon-α showed high antiviral activity

The sequences of 27 chicken interferon-alpha (ChIFN-α) genes were obtained from GenBank. The gene sequences were compared and homology between them was determined by using a bio-software. On the basis of these results, a new rChIFN-α peptide sequence with 194 amino acids was assembled. Thereafter, o...

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Bibliographic Details
Published in:Research in veterinary science 2011-12, Vol.91 (3), p.e73-e79
Main Authors: Hou, Fengxiang, Liu, Ke, Shen, Ting, Zhou, Bin, Cao, Ruibin, Li, Peide, Chen, Puyan
Format: Article
Language:English
Subjects:
Amino Acid Sequence
amino acid sequences
amino acids
Animals
Antiviral Agents - pharmacology
antiviral properties
antiviral proteins
Cells, Cultured
Chick Embryo
Chicken interferon
Chickens
engineering
Fibroblasts
Gene Expression
genes
genetic vectors
interferon-alpha
Interferon-alpha - chemistry
Interferon-alpha - genetics
Interferon-alpha - metabolism
Interferon-alpha - pharmacology
molecular cloning
Molecular Sequence Data
Newcastle disease virus
Newcastle disease virus - drug effects
nucleotide sequences
Pichia - metabolism
Pichia pastoris
plasmids
Recombinant Proteins - pharmacology
sequence homology
Vesicular stomatitis virus
Vesiculovirus
Vesiculovirus - drug effects
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Summary:The sequences of 27 chicken interferon-alpha (ChIFN-α) genes were obtained from GenBank. The gene sequences were compared and homology between them was determined by using a bio-software. On the basis of these results, a new rChIFN-α peptide sequence with 194 amino acids was assembled. Thereafter, on the basis of the new amino acid sequences and by using the most frequently occurring codes of Pichia pastoris, and a 582 bp gene sequence was formed. In order to amplify this non-templated gene, 16 primers were designed, and their gene sequences were synthesized, and amplified. This amplified gene sequence was cloned into the expression vector pPICZα-A to construct a recombination plasmid named pPICZ-rChIFN-α. Then, the recombination plasmid was induced to express the rChIFN-α protein. The results demonstrated that the recombinant plasmid pPICZ-rChIFN-α was successfully expressed in P. pastoris. Furthermore, rChIFN-α had a considerable antiviral activity against both Newcastle disease virus (NDV) and vesicular stomatitis virus (VSV). Therefore, this method of gene engineering could give direction to research on the key amino acids in the interferon or analogous proteins and enable the construction of proteins with high antiviral activity, which can be used both for research and industrial purposes.
ISSN:0034-5288
1532-2661
DOI:10.1016/j.rvsc.2010.11.015