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番茄植株感染期间,病原和非病原尖孢镰刀菌菌株的监测。

Monitoring of pathogenic and non-pathogenic Fusarium oxysporum strains during tomato plant infection.

机构信息

Leiden University, Institute of Biology, Sylviusweg 72, 2333 BE Leiden, The Netherlands.

出版信息

Microb Biotechnol. 2011 Jan;4(1):82-8. doi: 10.1111/j.1751-7915.2010.00214.x.

Abstract

Monitoring of pathogenic strains of Fusarium oxysporum (Fox), which cause wilt and rots on agricultural and ornamental plants, is important for predicting disease outbreaks. Since both pathogenic and non-pathogenic strains of Fox are ubiquitous and are able to colonize plant roots, detection of Fox DNA in plant material is not the ultimate proof of an ongoing infection which would cause damage to the plant. We followed the colonization of tomato plants by strains Fox f. sp. radicis-lycopersici ZUM2407 (a tomato foot and root rot pathogen), Fox f. sp. radiciscucumerinum V03-2g (a cucumber root rot pathogen) and Fox Fo47 (a well-known non-pathogenic biocontrol strain). We determined fungal DNA concentrations in tomato plantlets by quantitative PCR (qPCR) with primers complementary to the intergenic spacer region (IGS) of these three Fox strains. Two weeks after inoculation of tomato seedlings with these Fox strains, the DNA concentration of Forl ZUM2407 was five times higher than that of the non-compatible pathogen Forc V03-2g and 10 times higher than that of Fo47. In 3-week-old plantlets the concentration of Forl ZUM2407 DNA was at least 10 times higher than those of the other strains. The fungal DNA concentration, as determined by qPCR, appeared to be in good agreement with data of the score of visible symptoms of tomato foot and root rot obtained 3 weeks after inoculation of tomato with Forl ZUM2407. Our results show that targeting of the multicopy ribosomal operon results in a highly sensitive qPCR reaction for the detection of Fox DNA. Since formae speciales of Fox cannot be distinguished by comparison of ribosomal operons, detection of Fox DNA is not evidence of plant infection by a compatible pathogen. Nevertheless, the observed difference in levels of plant colonization between pathogenic and non-pathogenic strains strongly suggests that a concentration of Fox DNA in plant material above the threshold level of 0.005% is due to proliferation of pathogenic Fox.

摘要

对引起农业和观赏植物枯萎和腐烂的尖孢镰刀菌(Fox)致病菌株进行监测,对于预测疾病爆发非常重要。由于 Fox 的致病和非致病菌株无处不在,并且能够定植在植物根部,因此在植物材料中检测到 Fox DNA 并不能最终证明正在发生感染,而这种感染会对植物造成损害。我们跟踪了番茄植株被 Fox f. sp. radicis-lycopersici ZUM2407(番茄脚腐和根腐病原菌)、Fox f. sp. radiciscucumerinum V03-2g(黄瓜根腐病原菌)和 Fox Fo47(一种著名的非致病生物防治菌株)菌株的定植情况。我们通过定量 PCR(qPCR)用与这三种 Fox 菌株的基因间 spacer 区(IGS)互补的引物来确定番茄幼苗中的真菌 DNA 浓度。在将这些 Fox 菌株接种到番茄幼苗 2 周后,Forl ZUM2407 的 DNA 浓度是不亲和性病原菌 Forc V03-2g 的 5 倍,是 Fo47 的 10 倍。在 3 周龄的幼苗中,Forl ZUM2407 DNA 的浓度至少是其他菌株的 10 倍。通过 qPCR 确定的真菌 DNA 浓度与用 Forl ZUM2407 接种番茄 3 周后获得的番茄脚腐和根腐可见症状评分数据非常吻合。我们的结果表明,靶向多拷贝核糖体操纵子可导致 Fox DNA 的高灵敏度 qPCR 反应。由于 Fox 的特殊形式不能通过比较核糖体操纵子来区分,因此检测到 Fox DNA 并不能证明植物受到了相容病原菌的感染。然而,在致病和非致病菌株之间观察到的植物定植水平差异强烈表明,植物材料中 Fox DNA 的浓度超过 0.005%的阈值水平是由于致病性 Fox 的增殖。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f195/3815798/8416a1b8dfe8/mbt0004-0082-f2.jpg

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