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Upregulated expression of the cDNA fragment possibly related to the virulence of Acanthamoeba culbertsoni
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Original Article

Upregulated expression of the cDNA fragment possibly related to the virulence of Acanthamoeba culbertsoni

The Korean Journal of Parasitology 1999;37(4):257-263.
Published online: December 31, 1999

Department of Parasitology and Institute of Tropical Medicine, Yonsei Univesity College of Medicine, Seoul 120-752, Korea.

Corresponding author (para@yumc.yonsei.ac.kr)
• Received: July 26, 1999   • Accepted: November 5, 1999

Copyright © 1999 by The Korean Society for Parasitology

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  • Taurine, a Component of the Tear Film, Exacerbates the Pathogenic Mechanisms of Acanthamoeba castellanii in the Ex Vivo Amoebic Keratitis Model
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    Pathogens.2023; 12(8): 1049.     CrossRef
  • Acanthamoebaspp. as Agents of Disease in Humans
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    Clinical Microbiology Reviews.2003; 16(2): 273.     CrossRef

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Upregulated expression of the cDNA fragment possibly related to the virulence of Acanthamoeba culbertsoni
Korean J Parasitol. 1999;37(4):257-263.   Published online December 31, 1999
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Upregulated expression of the cDNA fragment possibly related to the virulence of Acanthamoeba culbertsoni
Korean J Parasitol. 1999;37(4):257-263.   Published online December 31, 1999
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Upregulated expression of the cDNA fragment possibly related to the virulence of Acanthamoeba culbertsoni
Image Image Image Image Image
Fig. 1 An example of 5% polyacrylamide gel electrophoresis with DDRT-PCR products. PCR was performed with combinations of an arbitrary primer 283 and oligo-dT11-G, A, and C primers, respectively. Dots denote unique PCR amplicons for the brain-passaged amoeba. G, A and C indicate oligo-dT primers used for PCR, the 3' terminal nucleotide of which was G, A and C, respectively. P, brain-passaged amoeba; N, non-brain-passaged amoeba; M, DNA size marker of 100 bp ladder.
Fig. 2 Identification of DDRT-PCR amplicons of differentially-expressed genes (arrow heads) by Southern slot-blot analysis using the pooled DDRT-PCR products as probes. PCR re-amplified products of the selected 96 unique amplicons for the brain-passaged amoeba were immobilized in duplicate sets onto nylon membranes and hybridized with the pooled original DDRT-PCR products from the brain-passaged amoeba (A) or from the non-brain-passaged amoeba (B).
Fig. 3 Nucleotide sequence and conceptual translation product of the clone A289C. The numbering refers to the nucleotide sequence and amino acid sequence.
Fig. 4 Alignment of A289C with AmsG from Erwinia amylovora (EMBL accession No. Q46628) and cspD from S. agalactial (EMBL accession No. Q04664). Identical amino acids in two sequences are symbolized by bars. Conservative substitutions are marked by dots.
Fig. 5 Upregulated expression of the A289C gene verified by Northern slot-blot analysis. 1, total RNA of brain-passaged Acanthamoeba culbertsoni; 2, negative control; 3, total RNA of non-passaged A. culbertsoni.
Upregulated expression of the cDNA fragment possibly related to the virulence of Acanthamoeba culbertsoni
Primer dT-G dT-A dT-C Total
235 5 5 NDa) 10
252 3 ND ND 3
269 ND ND 4 4
280 ND ND 6 6
283 12 6 5 23
284 ND ND 3 3
285 5 5 ND 10
287 ND 6 ND 6
289 ND ND 6 6
290 ND ND 5 5
296 ND 3 9 12
299 2 3 3 8
Primer combinations Size (bp)
dT-A : 235 310
dT-A : 235 420
dT-A : 287 170
dT-A : 296 220
dT-A : 296 300
dT-A : 299 460
dT-C : 289 300
dT-C : 289 440
dT-C : 289 460
dT-C : 289 550
dT-C : 289 750
dT-C : 299 650
Table 1. Number of unique DDRT-PCR products observed only in brain-passaged Acanthamoeba culbertsoni

Not done; DDRT-PCR was not done with this primer because of the lack of informative PCR products observed in the preliminary experiment.

Table 2. DDRT-PCR products hybridized only with the probe synthesized from the pooled DDRT-PCR products of brain-passaged Acanthamoeba culbertsoni