Development of a multiplex Q-PCR to detect Trichoderma harzianum Rifai strain T22 in plant roots

被引:8
|
作者
Horn, Ivo R. [1 ]
van Rijn, Menno [1 ,3 ]
Zwetsloot, Tom J. J. [1 ]
Basmagi, Said [1 ]
Dirks-Mulder, Anita [1 ]
van Leeuwen, Willem B. [1 ]
Ravensberg, Willem J. [3 ]
Gravendeel, Barbara [1 ,2 ,4 ]
机构
[1] Univ Appl Sci Leiden, Zernikedreef 11, NL-2333 CK Leiden, Netherlands
[2] Nat Biodivers Ctr, Darwinweg 2, NL-2333 Cr Leiden, Netherlands
[3] Koppert Biol Syst, Veilingweg 14, NL-2651 BE Berkel, Netherlands
[4] Leiden Univ, Inst Biol Leiden, Sylviusweg 72, NL-2333 BE Leiden, Netherlands
关键词
Q-PCR; aox1; Biological control agent; Hydrolysis probes; Plant roots; BIOLOGICAL-CONTROL AGENT; REAL-TIME PCR; GROWTH; FUNGI; SOIL; INOCULATION; GLIOCLADIUM; SEEDLINGS; BIOMASS;
D O I
10.1016/j.mimet.2015.12.014
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
The fungal species Trichoderma harzianum is widely used as a biological agent in crop protection. To verify the continued presence of this fungus on plant roots manually inoculated with T. harzianum strain T22, a Q-PCR was designed using specific probes for this particular strain. To develop these molecular diagnostic tools, genome mining was first carried out to retrieve putative new regions by which different strains of T. harzianum could be distinguished. Subsequently, Sanger sequencing of the L-aminoacid oxidase gene (aox1) in T. harzianum was applied to determine the mutations differing between various strains isolated from the Trichoderma collection of Koppert Biological Systems. Based on the sequence information obtained, a set of hydrolysis probes was subsequently developed which discriminated T. harzianum T22 strains varying in only a single nucleotide. Probes designed for two strains uniquely recognized the respective strains in Q-PCR with a detection limit of 12,5 ng DNA. Titration assays in which T. harzianum DNA from distinct strains was varied further underscored the specificity of the probes. Lastly, fungal DNA extracted from roots of greenhouse cultured tomato plants was analyzed using the probe-based assay. DNA from T. harzianum strain T22 could readily be identified on roots of greenhouse reared tomato plants inoculated with varying concentrations up to one week after treatment with a detection limit of 3e6 colony forming units of T. harzianum T22. We conclude that the Q-PCR method is a reliable and robust method for assessing the presence and quantity of T. harzianum strain T22 in manually inoculated plant material. Our method provides scope for the development of DNA based strain specific identification of additional strains of Trichoderma and other fungal biological control agents. (C) 2015 Elsevier B.V. All rights reserved.
引用
收藏
页码:44 / 49
页数:6
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