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Original Article

Immunodiagnosis of clonorchiasis using a recombinant antigen

The Korean Journal of Parasitology 1998;36(3):183-190.
Published online: September 30, 1998

Department of Parasitology, Yonsei University College of Medicine, Seoul 120-752, Korea.

Corresponding author (tsyong212@yumc.yonsei.ac.kr)
• Received: May 23, 1998   • Accepted: July 22, 1998

Copyright © 1998 by The Korean Society for Parasitology

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Citations

Citations to this article as recorded by  Crossref logo
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    Pathogens and Global Health.2013; 107(5): 253.     CrossRef
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Immunodiagnosis of clonorchiasis using a recombinant antigen
Korean J Parasitol. 1998;36(3):183-190.   Published online September 30, 1998
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Immunodiagnosis of clonorchiasis using a recombinant antigen
Korean J Parasitol. 1998;36(3):183-190.   Published online September 30, 1998
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Immunodiagnosis of clonorchiasis using a recombinant antigen
Image Image Image Image Image
Fig. 1 IgG-immunoblot analysis of pBCs31 fusion protein. The pBCs31 induced in E. coli XLl-Blue MRF' shows 28 kDa band reactive to an C. sinensis infected rabbit serum, (a) Negative control of E. coli lysate containing pBK-CMV vector only, (b) E. coli lysate containing induced pBCs31. At about 14 kDa, background reacting bands against a E. coli protein were noticed in both (a) and (b).
Fig. 2 The size of C. sinensis cDNA insert contained in pBCs31 was 0.8 kb (closed arrowhead) on 0.8% agarose electrophoresis following double digestable with EcoR I and Xho I. Open arrowhead shows the vector.
Fig. 3 The nucleotide sequence of pBCs31 insert and deduced amino acid sequence showed that one open reading frame encoding an antigenic protein bearing repetitive epitopes. The indicated reading frame is in phase with the β-galactosidase gene of pBK-CMV vector, and G in the parenthesis at the beginning is from the adaptor sequence for cloning.
Fig. 4 Total RNAs of adult C. sinensis and P. westermani (5 µg each) were blotted, and hybridized with 32P-labelled cloned gene (i.e., C. sinensis cDNA contained in pBCs31). Clonorchis sinensis RNA showed a positive reaction, while P. westermani RNA showed no reaction.
Fig. 5 Immunoblot analysis of an affinity purified recombinant protein. The recombinant fused protein to β-galactosidase shows a band reacting to the C. sinensis infected sera.
Immunodiagnosis of clonorchiasis using a recombinant antigen
Source of human sera No. of cases assayed No. of cases to pBCs31 No. of cases anti-C. sinensis adult worm antigen positive
clonorchiasis 20 11 14
paragonimiasis 10 0 2
cysticercosis 10 0 0
sparganosis 6 0 0
Table 1. Reactivity of pBCs31 recombinant protein to sera from cases with various parasitic infections or negative control by ELISA