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Expression of major piroplasm protein (p33) of Theileria sergenti (Korean isolate) and its immunogenicity in guinea pigs
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Original Article

Expression of major piroplasm protein (p33) of Theileria sergenti (Korean isolate) and its immunogenicity in guinea pigs

The Korean Journal of Parasitology 1999;37(4):277-283.
Published online: December 31, 1999

National Veterinary Research and Quarantine Service, MAF, Anyang, 340-016, Korea.

Corresponding author (kangsw@mail.nvrqs.go.kr)
• Received: August 6, 1998   • Accepted: November 4, 1999

Copyright © 1999 by The Korean Society for Parasitology

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Citations

Citations to this article as recorded by  Crossref logo
  • Adjuvant effect of bovine heat shock protein 70 on piroplasm surface protein, p33, of Theileria sergenti
    Wooseog Jeong, Chang Hee Kweon, Seung Won Kang, Hyang Sim Lee, Yingtian Xu, Cheng Lu, Shoufa Zhang, Vishvanath Nene
    Biologicals.2009; 37(5): 282.     CrossRef
  • SEROLOGICAL INVESTIGATION OF THEILERIA SERGENTI USING LATEX AGGLUTINATION TEST IN SOUTH KOREA
    Wooseog Jeong, Chang Hee Kweon, Jong Man Kim, Hwan Jang, Sang Gi Paik
    Journal of Parasitology.2005; 91(1): 164.     CrossRef

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Expression of major piroplasm protein (p33) of Theileria sergenti (Korean isolate) and its immunogenicity in guinea pigs
Korean J Parasitol. 1999;37(4):277-283.   Published online December 31, 1999
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Expression of major piroplasm protein (p33) of Theileria sergenti (Korean isolate) and its immunogenicity in guinea pigs
Korean J Parasitol. 1999;37(4):277-283.   Published online December 31, 1999
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Expression of major piroplasm protein (p33) of Theileria sergenti (Korean isolate) and its immunogenicity in guinea pigs
Image Image Image Image Image Image
Fig. 1 Construction of transfer vector for baculovirus expression. A. DNA fragment containing p33 of T. sergenti was ligated with a transfer vector (pBaKPak8) using BamHI and EcoRI site. B. Nucleotide sequences of recombinant transfer vector in pBaKPAK8. First translational codon (ATG) of p33 is indicated with an arrow.
Fig. 2 Identification of a p33 gene of T. sergenti from recombinant AcNPV by PCR. Lane 1, Standard size marker; lane 2, recombinant AcNPV clone 1; lane 3, recombinant AcNPV clone 2; lane 4, control AcNPV; lane 5 and 6, positive standard PCR; lane 7, positive isolate (Sunghwan), respectively.
Fig. 3 Immunofluorescence of Sf 21 cells. A. Control cells. B. cells infected with recombinant baculovirus cloned from 10-6 dilution of transfection supernatant. Cells were reacted with T. sergenti positive bovine serum (1:50. ×660.
Fig. 4 Identification of p33 protein expressed in Sf21 cells infected with recombinant AcNPV by SDS-PAGE (12%). Lane 1, standard size marker; lane 2, Control-Sf 21 cell-lysates; lane 3 and 4, Sf21 cell-lysates infected with recombinant AcNPV cloned from the dilution of 10-5 (lane 3) and 10-6 (land 4) from transfected supernatant, respectively.
Fig. 5 Indirect fluorescence antibody test of T. sergenti-infected RBC with guinea pig serum immunized with Sf21 cell-lysate infected by recombinant baculovirus. ×1,200.
Fig. 6 Immunoblotting analysis of T. sergenti with sera of guinea pig immunized with recombinant baculovirus infected Sf21 cell-lysates. Lane 1, Standard M.W.marker; lane 2, T. sergenti reacted with guinea pig serum raised from wild AcNPV infected Sf21 cell lysates; lane 3, T. sergenti reacted with guinea pig serum raised from p33 expressing recombinant AcNPV infected Sf21 cell lysates.
Expression of major piroplasm protein (p33) of Theileria sergenti (Korean isolate) and its immunogenicity in guinea pigs