Specific Primer Designing for Quantitative PCR (qPCR) of Entomopathogenic Fungi Isaria fumosorosea from Soil Samples
Syaiful Amri Saragih(1*), Shuhei Takemoto(2), Hiroaki Sato(3), Naoto Kamata(4)
(1) Department of Agrotechnology, Faculty of Agriculture, Universitas Muhammadiyah Sumatera Utara Jalan Kapten Mukhtar Basri No. 3, Medan, North Sumatra 20238 Indonesia
(2) The University of Tokyo Tanashi Forest, The University of Tokyo Forests, Graduate School of Agricultural and Life Sciences, The University of Tokyo, Nishi-Tokyo, Tokyo, Japan 188-0002
(3) Department of Forest Entomology, Forestry and Forest Products Research Institute, Tsukuba, Ibaraki, Japan 305-8687
(4) The University of Tokyo Chiba Forest, The University of Tokyo Forests, Graduate School of Agricultural and Life Sciences, The University of Tokyo, Kamogawa, Chiba, Japan 299-5503
(*) Corresponding Author
Abstract
Entomopathogenic fungi are important component for regulation of pests in ecosystem. Isaria fumosorosea, as one of the entomopathogenic fungi, was reported to successfully controlled the outbreaks of forest defoliators attacked larch (Larix kaempferi) plantation in Furano, Japan and beech (Fagus crenata) forest in Hachimantai, Japan. Instead of semi-cultured method, in this paper, a culture-independent method based on DNA using qPCR was developed for specific detection and quantification of I. fumosorosea directly from soil DNA extract using specific primer. The primer IFU5821F/IFU6061R was designed and found to be the best primer pair for I. fumosorosea. Standard soil DNA was obtained with strong relationship and good fitting with five levels (R2= 0.989, E = 0.58). I. fumosorosea could not be detected from all soil samples which was possibility caused by low density of the fungi. The qPCR was likely a rapid and specific method to detect the fungus from soil.
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DOI: https://doi.org/10.22146/jpti.77867
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