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 Australasian Plant Disease Notes
Disease notes, new records and quarantine interception reports are published in Australasian Plant Disease Notes.

 

Article     |     Next >>   Contents Vol 38(2)

A one-tube fluorescent assay for the quarantine detection and identification of Tilletia indica and other grass bunts in wheat

Mui-Keng Tan A B H, Aida Ghalayini A B, Indu Sharma C, Jianping Yi D, Roger Shivas B E, Michael Priest B F, Dominie Wright B G

A Elizabeth Macarthur Agricultural Institute (EMAI), NSW Department of Primary Industries, PMB 8, Camden, NSW 2570, Australia.
B CRC for National Plant Biosecurity, 2/4 Phipps Close, Deakin, ACT 2600, Australia.
C Department of Plant Breeding, Genetics and Biotechnology, Punjab Agricultural University, Ludhiana 141004, Punjab, India.
D Shanghai Entry-Exit Inspection and Quarantine Bureau, 1208 Minsheng Road, Pudong New Area, Shanghai 200135, China.
E Plant Pathology Herbarium, Department of Primary Industries and Fisheries, Indooroopilly, Qld 4068, Australia.
F Orange Agricultural Institute, NSW Department of Primary Industries, Orange, NSW 2800, Australia.
G Department of Agriculture and Food, Locked Bag 4, Bentley Delivery Centre, WA 6983, Australia.
H Corresponding author. Email: mui-keng.tan@dpi.nsw.gov.au
 
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Abstract

A molecular assay with enhanced specificity and sensitivity has been developed to assist in the surveillance of Karnal bunt, a quarantineable disease with a significant impact on international trade. The protocol involves the release of DNA from spores, PCR amplification to enrich Tilletia-specific templates from released DNA and a five-plex, real-time PCR assay to detect, identify and distinguish T. indica and other Tilletia species (T. walkeri, T. ehrhartae, T. horrida and a group comprising T. caries, T. laevis, T. contraversa, T. bromi and T. fusca) in wheat grains. This fluorescent molecular tool has a detection sensitivity of one spore and thus bypasses the germination step, which in the current protocol is required for confirmation when only a few spores have been found in grain samples. The assay contains five dual-labelled, species-specific probes and associated species-specific primer pairs in a PCR mix in one tube. The different amplification products are detected simultaneously by five different fluorescence spectra. This specific and sensitive assay with reduced labour and reagent requirements makes it an effective and economically sustainable tool to be used in a Karnal bunt surveillance program. This protocol will also be valuable for the identification of some contaminant Tilletia sp. in wheat grains.

   
    


 
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