Development, Optimization and Evaluation of a Sensitive Enzyme-Linked Immunosorbent Assay (ELISA) Prototype for Detection of Chicken-Based IgY Polyclonal Antibodies against Toxins of D. polylepis Venom

Author:

Kpordze Stephen Wilson12ORCID,Kikuvi Gideon Mutie3,Kimotho James Hungo4,Mobegi Victor Atunga5

Affiliation:

1. Department of Molecular Biology and Biotechnology, Pan African University Institute for Basic Sciences, Technology and Innovation (PAUSTI), JKUAT-Juja Campus, Nairobi 62000-00200, Kenya

2. Spanish Laboratory Complex, University for Development Studies, Nyankpala Campus, Tamale TL 1350, Ghana

3. Department of Environmental Health and Disease Control, Jomo Kenyatta University of Agriculture and Technology, JKUAT-Juja Campus, Nairobi 62000-00200, Kenya

4. Kenya Medical Research Institute, Off Raila Odinga Way, Nairobi 54840-00200, Kenya

5. Department of Biochemistry, University of Nairobi, Chiromo Campus, Nairobi 30197-00100, Kenya

Abstract

Life-threatening medical issues can result from snakebite, and hence this is a public health concern. In many tropical and subtropical nations such as Kenya, where a wide variety of poisonous snakes are prevalent, diagnosis of snakebite in health facilities is imperative. Different antivenoms are needed to treat the venom of different snake species. Nonetheless, it might be difficult for medical professionals to identify the exact snake species that envenomated a patient due to the similarities of several snake envenomations’ clinical symptoms. Therefore, the necessity for an assay or technique for identifying venomous species is critical. The current study sought to develop a sensitive ELISA prototype for the detection of D. polylepis venom in Kenya using generated chicken-based IgY polyclonal antibodies. Serum samples containing specific chicken-based IgY antibodies previously raised against D. polylepis venom toxins were used in the assay development. ELISA parameters were optimized, and the developed assay was assessed for applicability. The limit of detection (LoD) of the ELISA for neurotoxic venoms was determined to be 0.01 µg/mL. Successful discrimination between neurotoxic and cytotoxic venoms was achieved by the ensuing inhibition ELISA assay. The developed assay showed the capability of identifying venoms in blood samples (from spiked and venom-challenged blood samples) of BALB/c mice, providing compelling evidence of the strategy’s usefulness. This assay could help physicians diagnose and manage victims of snakebites through the evaluation of clinical samples.

Funder

African Union Commission

Publisher

MDPI AG

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