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High-throughput gene-expression quantification of grapevine defense responses in the field using microfluidic dynamic arrays

机译:使用微流控动态阵列在野外葡萄防御反应的高通量基因表达定量

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Background The fight against grapevine diseases due to biotrophic pathogens usually requires the massive use of chemical fungicides with harmful environmental effects. An alternative strategy could be the use of compounds able to stimulate plant immune responses which significantly limit the development of pathogens in laboratory conditions. However, the efficiency of this strategy in natura is still insufficient to be included in pest management programs. To understand and to improve the mode of action of plant defense stimulators in the field, it is essential to develop reliable tools that describe the resistance status of the plant upon treatment. Results We have developed a pioneering tool (“NeoViGen96” chip) based on a microfluidic dynamic array platform allowing the expression profiling of 85 defense-related grapevine genes in 90 cDNA preparations in a 4?h single run. Two defense inducers, benzothiadiazole (BTH) and fosetyl-aluminum (FOS), have been tested in natura using the “NeoViGen96” chip as well as their efficacy against downy mildew. BTH-induced grapevine resistance is accompanied by the induction of PR protein genes ( PR1 , PR2 and PR3 ), genes coding key enzymes in the phenylpropanoid pathway ( PAL and STS ), a GST gene coding an enzyme involved in the redox status and an ACC gene involved in the ethylene pathway. FOS, a phosphonate known to possess a toxic activity against pathogens and an inducing effect on defense genes provided a better grapevine protection than BTH. Its mode of action was probably strictly due to its fungicide effect at high concentrations because treatment did not induce significant change in the expression level of selected defense-related genes. Conclusions The NeoViGen96” chip assesses the effectiveness of plant defense inducers on grapevine in vineyard with an excellent reproducibility. A single run with this system (4?h and 1,500 €), corresponds to 180 qPCR plates with conventional Q-PCR assays (Stragene system, 270?h and 9,000 €) thus a throughput 60–70 times higher and 6 times cheaper. Grapevine responses after BTH elicitation in the vineyard were similar to those obtained in laboratory conditions, whereas our results suggest that the protective effect of FOS against downy mildew in the vineyard was only due to its fungicide activity since no activity on plant defense genes was observed. This tool provides better understanding of how the grapevine replies to elicitation in its natural environment and how the elicitor potential can be used to reduce chemical fungicide inputs.
机译:背景技术对抗由生物营养性病原体引起的葡萄疾病的斗争通常需要大量使用对环境有害的化学杀菌剂。替代策略可以是使用能够刺激植物免疫反应的化合物,该化合物显着限制实验室条件下病原体的发育。但是,该策略在自然界中的效率仍然不足以纳入害虫管理计划。为了理解并改善本领域中植物防御刺激物的作用方式,必须开发出可靠的工具来描述处理后植物的抗性状况。结果我们开发了一种基于微流体动态阵列平台的开拓性工具(“ NeoViGen96”芯片),可在4?h单次运行中在90个cDNA制剂中表达85个与国防相关的葡萄基因。在自然中使用“ NeoViGen96”芯片测试了两种防御诱导剂苯并噻二唑(BTH)和乙磷铝(FOS)及其对霜霉病的功效。 BTH诱导的葡萄抗性伴随PR蛋白基因(PR1,PR2和PR3),苯丙烷途径(PAL和STS)中编码关键酶的基因,GST基因编码参与氧化还原状态的酶和ACC的诱导基因参与乙烯途径。 FOS是一种已知对病原体具有毒理作用且对防御基因具有诱导作用的膦酸酯,其提供的葡萄保护性优于BTH。它的作用方式可能严格地是由于其在高浓度下的杀菌作用,因为治疗并未诱导所选防御相关基因的表达水平发生明显变化。结论NeoViGen96“芯片具有出色的可重复性,可评估葡萄园中葡萄藤上植物防御诱导剂的有效性。该系统的单次运行(4?h和1,500€)相当于使用常规Q-PCR分析的180个qPCR板(Stragene系统,270?h和9,000€),因此通量提高60-70倍,便宜6倍。葡萄园中BTH诱导后的葡萄藤反应与实验室条件下的相似,但我们的结果表明FOS对葡萄园中霜霉病的保护作用仅归因于其杀菌剂活性,因为未观察到对植物防御基因的活性。该工具可以更好地了解葡萄在自然环境中如何响应诱导作用,以及如何利用激发电位来减少化学杀菌剂的输入。

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