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Publication no. D-2000-0218-01R
Detection of Acidovorax avenae subsp. citrulli in
Watermelon Seed Using Immunomagnetic Separation and the Polymerase Chain
Reaction. R. R. Walcott and R. D. Gitaitis, University of Georgia, Coastal
Plain Experiment Station, Tifton 31793. Plant Dis. 84:470-474. Accepted for
publication 5 January 2000. Copyright 2000 The American Phytopathological
Society.
An immunomagnetic separation and polymerase chain reaction (IMS-PCR)-based
assay was developed for detecting Acidovorax avenae subsp. citrulli
in watermelon seed. IMS yielded a 10-fold increase in recovery of A.
avenae subsp. citrulli over direct spread-plating on King’s Medium
B; however, the presence of seed debris reduced IMS efficiency. Synthetic
oligonucleotide primers were designed based on the 16S rRNA gene of a known A.
avenae subsp. citrulli strain and tested for specific DNA
amplification by PCR. The primers amplified DNA from all A. avenae subsp.
citrulli strains tested but also yielded amplicons with several closely
related bacteria. IMS-PCR resulted in a 100-fold increase in A. avenae subsp.
citrulli detection sensitivity over direct PCR and was unaffected by PCR
inhibitors in watermelon seed. The threshold of A. avenae subsp.
citrulli detection for IMS-PCR was 10 CFU/ml in watermelon seed
wash, and seedlots with 0.1% infestation were consistently detected.
IMS-PCR represents an efficient and sensitive approach to detecting A. avenae
subsp. citrulli in watermelon seedlots. Additional keywords: Citrulus
lanatus, watermelon fruit blotch.
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