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DAO 40:137-146 (2000)
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Abstract
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Molecular detection of Marteilia sydneyi, pathogen of Sydney rock oysters
Sarah N. Kleeman1,*, Robert D. Adlard2
1Department of Parasitology, University of Queensland, Brisbane, Queensland 4072, Australia
2Protozoa Section, Queensland Museum, PO Box 3300, South Brisbane, Queensland 4101, Australia
*E-mail: s.kleeman@mailbox.uq.edu.au
ABSTRACT: The life cycle of Marteilia sydneyi, the aetiological agent of QX disease in the Sydney rock oyster Saccostrea commercialis, is not known. We have developed and optimised 2 diagnostic assays, the polymerase chain reaction (PCR) and
in situ hybridisation, for use in investigating the role of possible alternative hosts in the life cycle of this pathogen. PCR primers, designed within the ITS1 rDNA of M. sydneyi, amplified a 195 bp fragment. Sensitivity of the PCR assay
was assessed using DNA extracted from known numbers of sporonts purified from infected oyster digestive gland. DNA equivalent to 0.01 sporonts was detectable following agarose gel electrophoresis. The potential inhibitory effect of the presence of host
DNA on the PCR assay was tested by the addition of oyster genomic DNA during amplification. Concentrations of host DNA in excess of 50 ng per 20 µl reaction reduced the sensitivity of the test. Environmental validation of the PCR assay was demonstrated by
the amplification of M. sydneyi DNA from 50 ng of genomic DNA extracted from QX-infected oysters. A DNA probe was constructed using the M. sydneyi unique primers and was able to detect 10 pg of M. sydneyi PCR amplified DNA in
dot-blot hybridisations. The probe hybridised with presporulating and sporulating M. sydneyi stages in paraffin sections of oyster digestive gland. No non-specific binding was observed. Hybridisation consistency and signal intensity decreased as
sporonts matured. While the high sensitivity and specificity of the PCR test will allow rapid screening of large numbers of potential alternative hosts for the presence of parasite DNA, it does not actually identify infective stages. In situ
hybridisation conducted on paraffin sections will determine the location of the parasite within the host for morphological characterisation.
KEY WORDS: Marteilia sydneyi · PCR primers · DNA probe · In situ hybridisation · Saccostrea commercialis · rDNA gene sequence
Published in DAO Vol.
40, No. 2
(2000) on March 14
ISSN: 0177-5103.
Copyright © Inter-Research, Oldendorf/Luhe, 2000
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