Preparation of Polyclonal Antiserum to the Recombinant TiLV-S8 Protein and Its Application in the Detection of Naturally Tilapia Lake Virus (TiLV) Infected Tilapia

Authors

  • Chatchapong Sopa Department of Biology, Faculty of Science, Srinakharinwirot University, Bangkok 10110, Thailand
  • Pradit Wangman Center of Excellence in Animal, Plant and Parasite Biotechnology, Srinakharinwirot University, Bangkok 10110, Thailand
  • Nantawut Ponpukdee Department of Biology, Faculty of Science, Srinakharinwirot University, Bangkok 10110, Thailand
  • Parin Chaivisuthangkura Department of Biology, Faculty of Science, Srinakharinwirot University, Bangkok 10110, Thailand
  • Siwaporn Longyant

Keywords:

Nile tilapia, Tilapia Lake virus-TiLV, Polyclonal antiserum, Immunohistochemistry, Dot blotting

Abstract

Tilapia lake virus (TiLV) is classified as a negative-sense, single-stranded RNA virus in the family Amnoonviridae. It is an enveloped virus with 10 genomic RNA segments, each coding for a protein. TiLV causes disease in tilapia, and outbreaks can lead to significant economic losses for the tilapia aquaculture industry. In this study, the gene encoding the segment 8 protein of TiLV was cloned into the expression vector pET15-b and then transformed into Escherichia coli strain BL21. After induction, the recombinant TiLV-S8 protein (rTiLV-S8), with a molecular mass of 20 kDa, was expressed, purified, and used to immunize mice. The mouse antiserum against rTiLV-S8 protein demonstrated specific immunoreactivity for the viral protein, approximately 19 kDa in TiLV-infected fish tissues, as determined by Western blotting. According to the results of the dot blotting assay, the antiserum was about 80 times less sensitive than one-step RT-PCR in detecting TiLV in homogenates of infected fish samples and showed no cross-reaction with uninfected fish tissues, other common fish viruses, or prevalent bacterial species found in aquatic animals. Furthermore, this polyclonal antiserum could be employed to identify TiLV-infected fish in the field using dot blotting assay, and the results can be confirmed by immunohistochemistry.

Downloads

Download data is not yet available.

Downloads

Published

2023-12-27

How to Cite

Sopa, C. ., Wangman, P. ., Ponpukdee, N. ., Chaivisuthangkura, P. ., & Longyant, S. (2023). Preparation of Polyclonal Antiserum to the Recombinant TiLV-S8 Protein and Its Application in the Detection of Naturally Tilapia Lake Virus (TiLV) Infected Tilapia. Science Essence Journal, 39(2), 79–95. Retrieved from https://ejournals.swu.ac.th/index.php/sej/article/view/15749

Issue

Vol. 39 No. 2 (2023): Sci. Ess. J. Vol. 39 No. 2 (July - December 2023)

Section

Research Article