Journal
BIOCONTROL
Volume 52, Issue 4, Pages 491-505Publisher
SPRINGER
DOI: 10.1007/s10526-006-9038-0
Keywords
Australia; Dermolepida albohirtum; Metarhizium anisopliae; Queensland; sequential sampling; sugarcane; white grubs
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Three sugarcane fields in Bundaberg and four fields in each of the Burdekin, Tully and Innisfail (Queensland, Australia) were sampled for spores of Metarhizium anisopliae (Metchnikoff) (Deuteromycotina: Hyphomycetes). This entomopathogenic fungus is the active ingredient in the biocide BioCane (TM) stop, which was developed for the management of the greyback canegrub Dermolepida albohirtum (Waterhosue) (Coleoptera: Scarabaeidae) and other scarabs in cane fields. Fields sampled were of different crop ages and all had a history of BioCane (TM) stop treatment in Plant Cane in past years. Soil samples were taken in each field from four depths (0-10,10-20, 20-30 and 30-40 cm below soil level) with the use of an auger. Spore levels were highest at the depths of 10-20 and 20-30 cm. Spore levels differed between locations with Innisfail and Tully recording the highest spore counts. Spores were also found in the inter-row space in plots sampled in Tully. Sampling statistics were determined for M. anisopliae spores at the four soil depths with 0.1 and 0.25 precision levels. Three sampling methods were compared (use of marker beads; use of 100 mm auger and 150 mm auger). Samples that relied on marker beads resulted in higher spore counts, however, an auger can still be used since BioCane (TM) stop does not normally contain coloured markers. Results obtained demonstrate the ability of the pathogen to translocate in soil profile and across rows, most likely due to grub movements and other soil fauna. Sampling for M. anisopliae spores provides good monitoring of their levels in soil. The implications of this on grub management decisions are discussed.
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