ELISA based on a recombinant Paragonimus heterotremus protein for serodiagnosis of human paragonimiasis in Thailand

Kanokkarn Pothong; Chalit Komalamisra; Thareerat Kalambaheti; Dorn Watthanakulpanich; Timothy P Yoshino; Paron Dekumyoy

doi:10.1186/s13071-018-2878-5

ELISA based on a recombinant Paragonimus heterotremus protein for serodiagnosis of human paragonimiasis in Thailand

Parasit Vectors. 2018 May 30;11(1):322. doi: 10.1186/s13071-018-2878-5.

Authors

Kanokkarn Pothong¹, Chalit Komalamisra², Thareerat Kalambaheti³, Dorn Watthanakulpanich¹, Timothy P Yoshino⁴, Paron Dekumyoy⁵

Affiliations

¹ Department of Helminthology, Faculty of Tropical Medicine, Mahidol University, Bangkok, 10400, Thailand.
² Mahidol-Bangkok School of Tropical Medicine, Faculty of Tropical Medicine, Mahidol University, Bangkok, 10400, Thailand.
³ Department of Microbiology and Immunology, Faculty of Tropical Medicine, Mahidol University, Bangkok, 10400, Thailand.
⁴ Department of Pathobiological Sciences, School of Veterinary Medicine, University of Wisconsin, Madison, Wisconsin, 53706, USA.
⁵ Department of Helminthology, Faculty of Tropical Medicine, Mahidol University, Bangkok, 10400, Thailand. paron.dek@mahidol.edu.

Abstract

Background: Paragonimus heterotremus is the main causative agent of paragonimiasis in Thailand. In Western blot diagnostic assays for paragonimiasis, the 35 kDa band present in crude P. heterotremus somatic extracts represents one of the known diagnostic bands. This study aimed to use a P. heterotremus cDNA library to create a recombinant version of this antigen for use in immunodiagnosis of paragonimiasis.

Methods: To accomplish this aim a cDNA expression library was constructed from adult worm mRNA and immuno-screened using antibodies from mice that had been immunized with the 35 kDa antigen. Screening resulted in the identification of an immunoreactive protein encoded by clone CE3, which contained an inserted sequence composed of 1292 base pairs. This clone was selected for use in the construction of a recombinant P. heterotremus protein because of its similarity to proactivator polypeptide. For recombinant protein expression, the CE3 gene sequence was inserted into the plasmid vector pRset and the resulting product had the expected molecular weight of 35 kDa. An IgG-ELISA based on the CE3 recombinant protein was evaluated by using sera from healthy individuals, from patients with paragonimiasis and other parasitic infections. This ELISA was performed by using human sera diluted at 1:2000, an optimized antigen concentration of 1 μg/ml, and anti-human IgG diluted at 1:4000.

Results: The cut-off optical density value was set as the mean + 2 standard deviations (0.54), which resulted in the test having a sensitivity of 88.89% and a specificity of 95.51%. The recombinant antigen could react with antibodies from P. heterotremus, P. pseudoheterotremus and P. westermani infections. Cross-reactivity occurred with a few cases of Blastocystis hominis infection (2/3), Bancroftian filariasis (1/10), opisthorchiasis (3/10), strongyloidiasis (4/10) and neurocysticercosis (1/11).

Conclusions: Given the high test sensitivity and specificity, reflected in the low level of heterologous infection cross-reactivity (11/215 serum samples), observed in the IgG-ELISA, this 35 kDa antigen may be useful for the detection of paragonimiasis.

Keywords: IgG-ELISA; Immunodiagnosis; Paragonimiasis; Paragonimus heterotremus; Recombinant protein; cDNA library.

MeSH terms

Animals
Antibodies, Helminth / blood*
Antigens, Helminth / immunology*
Cross Reactions
Humans
Immunoglobulin G / blood
Paragonimiasis / diagnosis*
Paragonimiasis / parasitology
Paragonimus / immunology*
Recombinant Proteins
Sensitivity and Specificity
Serologic Tests

Substances

Antibodies, Helminth
Antigens, Helminth
Immunoglobulin G
Recombinant Proteins

Grants and funding

PHD/0269/2549/Thailand Research Fund