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Cloning and characterization of Giardia intestinalis cyclophilin
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Original Article

Cloning and characterization of Giardia intestinalis cyclophilin

The Korean Journal of Parasitology 2002;40(3):131-138.
Published online: September 30, 2002

Department of Parasitology, College of Medicine, Kyungpook National University, Daegu 700-422, Korea.

Corresponding author (dichung@knu.ac.kr)
• Received: July 15, 2002   • Accepted: August 22, 2002

Copyright © 2002 by The Korean Society for Parasitology

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Citations

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  • Cyclophilins as key players in protozoan parasite infections
    Reza Mansouri, Enrique Granado-Aparicio, Claudia Alcedo, Julio López-Abán, Reza Shafiei, Antonio Muro, Raúl Manzano-Román, Sajad Rashidi
    Parasites & Vectors.2025;[Epub]     CrossRef
  • Insights into Peptidyl-Prolyl cis-trans Isomerases from Clinically Important Protozoans: From Structure to Potential Biotechnological Applications
    Verónica Aranda-Chan, Rosa Elena Cárdenas-Guerra, Alejandro Otero-Pedraza, Esdras Enoc Pacindo-Cabrales, Claudia Ivonne Flores-Pucheta, Octavio Montes-Flores, Rossana Arroyo, Jaime Ortega-López
    Pathogens.2024; 13(8): 644.     CrossRef
  • Molecular aspects of cyclophilins mediating therapeutic actions of their ligands
    Andrzej Galat, Jacqueline Bua
    Cellular and Molecular Life Sciences.2010; 67(20): 3467.     CrossRef
  • Peptidyl-prolyl cis–trans isomerases (immunophilins) and their roles in parasite biochemistry, host–parasite interaction and antiparasitic drug action
    Angus Bell, Paul Monaghan, Antony P. Page
    International Journal for Parasitology.2006; 36(3): 261.     CrossRef
  • A Cyclophilin from Griffithsia japonica Has Thermoprotective Activity and Is Affected by CsA
    Eun Kyung Cho, Yoo Kyung Lee, Choo Bong Hong
    Molecules and Cells.2005; 20(1): 142.     CrossRef

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Cloning and characterization of Giardia intestinalis cyclophilin
Korean J Parasitol. 2002;40(3):131-138.   Published online September 30, 2002
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Cloning and characterization of Giardia intestinalis cyclophilin
Korean J Parasitol. 2002;40(3):131-138.   Published online September 30, 2002
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Cloning and characterization of Giardia intestinalis cyclophilin
Image Image Image Image Image
Fig. 1 Nucleotide sequences and putative amino acid sequences of Gicyp1. Putative transcriptional signal sequence 'tataa' is shown as boxed sequence. The bolded and underline sequences 'agtaaa' indicate polyadenylation consensus sequence. The italic characters of nucleotide sequences were detected by 5' RACE PCR analyses. The gray-boxed characters represent initiation signals in Giardia.
Fig. 2 A comparison of the deduced amino acid sequences of Giardia cyclophilin with other cyclophilins. Bolded amino acid sequences indicate residues involved in the CsA binding. The tryptophan essential for CsA binding is indicated with an asterisk. G.int, G. intestinalis; E.his, Entamoeba histolytica (accession number AF017993); P.fal, Plasmodium falciparum (accession number U33869); B.mal, Brugia malayi (accession number U47811); L.maj, Leshimania major (accession number Y13576). Yeast, accession number X17505; mouse, accession number X52803; human, accession number X52851; rat, accession number M19533.
Fig. 3 Southern hybridization (A) and Northern hybridization (B) of Giardia intestinalis cyclophilin gene. (A) The genomic DNA of G. intestinalis were digested with Pst I (Lane 1), Eco RI (Lane 2), and Hind III (Lane 3).
Fig. 4 SDS-PAGE gel electrophoresis patterns of recombinant GST fusion protein and purified Gicyp protein. Lane 1, crude extract of recipient strain E. coli BL21; 2, crude extract of transformed BL21 expressing Gicyp; 3, purified GST-Gicyp fusion protein; 4, purified Gicyp.
Fig. 5 Giardia Gicyp is an active and cyclosporin A - sensitive PPIase in protease-coupled peptide assay. The time course of cis → trans isomerase of N-Suc-Ala-Ala-Pro-Phe-p-nitroanilide coupled with chymotryptic cleavage was measured by the increase of absorbance at 390 nm using Shimadzu UV-1201 spectrophotometer. The data were collected every 5 s over 3-8 min interval. The isomerization of the peptide substrate (c; negative control) was accelerated in the presence of Gicyp1 at 20 nM (a). This PPIase activity was blocked after incubation of 20 nM Gicyp with 0.5 µM CsA (b).
Cloning and characterization of Giardia intestinalis cyclophilin