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Original Article

Molecular cloning and characterization of an antigenic protein with a repeating region from Clonorchis sinensis

The Korean Journal of Parasitology 2001;39(1):57-66.
Published online: March 31, 2001

1Department of Parasitology, Chung-Ang University Faculty of Medicine, Seoul 156-756, Korea.

2Section of Molecular Parasitology, Department of Molecular Cell Biology, Sungkyunkwan University School of Medicine, Suwon 440-746, Korea.

Corresponding author (hongsj@cau.ac.kr))
• Received: February 6, 2001   • Accepted: February 26, 2001

Copyright © 2001 by The Korean Society for Parasitology

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Molecular cloning and characterization of an antigenic protein with a repeating region from Clonorchis sinensis
Korean J Parasitol. 2001;39(1):57-66.   Published online March 31, 2001
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Molecular cloning and characterization of an antigenic protein with a repeating region from Clonorchis sinensis
Korean J Parasitol. 2001;39(1):57-66.   Published online March 31, 2001
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Molecular cloning and characterization of an antigenic protein with a repeating region from Clonorchis sinensis
Image Image Image Image Image Image
Fig. 1 Partial cDNA and its deduced amino acid sequences of a clone, CsRP12, from Clonorchis sinensis. A stretch of bold characters represents a repetitive unit. An asterisk (*) indicates a translational termination codon. Oligonucleotide primers used for DNA sequencing are underlined.
Fig. 2 multiple alignment of Clonorchis sinensis repetitive peptide, CsRP12-1, with surface proteins of animals. Residues identical to CsRP12-1 were shaded. A gap (-) was introduced for maximal alignment. Cs44, C. sinensis antigen 44 (Yong et al., 1998); XP2pre, Xenopus laevis skin secretory protein XP2 precursor (Hauser et al., 1992); CePro, Caenorhabditis elegans proline and glycine rich protein (Wilson et al., 1994); TcSA, Trypanosoma cruzi surface antigen (Buschiazzo et al., 1992); LdA2pre, Leishmania donovani amastigote-specific protein A2 precursor (Charest and Matlashewski, 1994); PfSAg, Plasmodium falciparum surface antigen protein precursor (Brown et al., 1987).
Fig. 3 Purification of recombinant CsRP12-1 and -2 proteins. Recombinant proteins bacterially produced were charged in a denaturation condition onto Ni-NTA column and eluted with a buffer containing 250 mM imidazole. The recombinant proteins purified and deployed in SDS-polyacrylamide gel were detected by Coomassie blue staining (A) and immunoblotting with anti-Xpress antibody (B). Lane 1, induced bacterial lysate; lane 2, flow-through; lane 3, eluate.
Fig. 4 Immunoblots of purified recombinant CsRP12-1 to helminth-infected patients' sera. A. Immunoblot against clonorchiasis patients' sera. B. Other helminth-infected patients' sera. Pw, paragonimiasis; Sp, sparganosis; Cy, cysticercosis; N, normal human sera; C, control by anti-Xpress antibody.
Fig. 5 An immunoblot of recombinant CsRP12-1 protein to Clonorchis sinensis-infected rabbit sera.
Fig. 6 Purification and antigenicity of bacterial recombinant C-terminus peptides of CsRP12. A. Purification of the recombinant proteins by Ni-NTA affinity chromatography. Lane 1, induced lysate; lane 2, pass-through fraction; lanes 3 and 4, buffers B and C, respectively; lanes 5, 6, 7 and 8, eluates with buffers C, D, E and F containing 250 mM imidazole, respectively. B. Immunolots against C. sinensis-infected patient sera. Lanes 1 to 7, clonorchiasis patients sera; lane 8, anti-RGS His antibody.
Molecular cloning and characterization of an antigenic protein with a repeating region from Clonorchis sinensis
CsRP12-1
CsRP12-2
No. of sera Positive sera (%) No. of sera Positive sera (%)
Clonorchiasis 35 35 (100%) 5 0 (0%)
Paragonimiasis 19 4 (21%) 5 0 (0%)
Sparganosis 17 2 (12%) 5 0 (0%)
Cysticercosis 17 3 (18%) 5 0 (0%)
Normal control 2 0 (0%) 2 0 (0%)
Table 1. Seroreactivity of recombinant CsRP12 proteins to various helminth-infected patient sera.