利用不规则根瘤进行体外茎枝测定

IF 1 Q3 BIOLOGY
Takaya Tominaga, Hironori Kaminaka
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引用次数: 0

摘要

大多数陆生植物都与共生的 Glomeromycotina 真菌(通常称为丛枝菌根(AM)真菌)相关联。在磷酸盐贫乏的条件下,AM 真菌通过向宿主分配矿质养分来增加植物的生物量;因此,宿主根系会积极分泌各种特殊代谢物,并协调共生伙伴。以前曾利用一种体外检测系统发现了由绞股蓝内酯(SLs)(一类植物激素)诱导的菌丝分枝活动。在这种生物测定中,通常使用的是巨孢菌属(Gigasporaeae)的AM真菌,因为它们具有线性的芽胞伸长,而且简单的分枝模式便于显微镜观察。然而,许多研究人员也使用颖壳菌科真菌作为寄主植物的共生伴侣,如Rhizophagus种,尽管它们通常表现出复杂的菌体分枝模式。在此,我们介绍了一种制作和量化流行的模式 AM 真菌不规则根瘤菌(Rhizophagus irregularis)的芽胞分枝的方法。在该系统中,R. irregularis 孢子夹在凝胶之间,相关化学物质从凝胶表面扩散到发芽的孢子。通过这种方法,可以再现合成 SL 对不规则形葡萄孢芽孢分枝的积极影响。因此,该方法可用于量化合成化学物质或植物来源的特殊代谢物对不规则红球菌的生理影响。主要特点 - 利用不规则根瘤菌的发芽孢子,开发出一种体外顶芽分枝测定方法。- 该体外检测系统基于 Kameoka 等人开发的方法 [1],但经过修改使其更适用于亲水性化合物。- 针对 R. irregularis 进行了优化,以计算菌丝分枝。- 该生物测定至少需要 12 天才能完成。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
In Vitro Hyphal Branching Assay Using Rhizophagus irregularis.

Most terrestrial plants are associated with symbiotic Glomeromycotina fungi, commonly known as arbuscular mycorrhizal (AM) fungi. AM fungi increase plant biomass in phosphate-depleted conditions by allocating mineral nutrients to the host; therefore, host roots actively exude various specialized metabolites and orchestrate symbiotic partners. The hyphal branching activity induced by strigolactones (SLs), a category of plant hormones, was previously discovered using an in vitro assay system. For this bioassay, AM fungi of the Gigaspora genus (Gigasporaeae) are commonly used due to their linear hyphal elongation and because the simple branching pattern is convenient for microscopic observation. However, many researchers have also used Glomeraceae fungi, such as Rhizophagus species, as the symbiotic partner of host plants, although they often exhibit a complex hyphal branching pattern. Here, we describe a method to produce and quantify the hyphal branches of the popular model AM fungus Rhizophagus irregularis. In this system, R. irregularis spores are sandwiched between gels, and chemicals of interest are diffused from the surface of the gel to the germinating spores. This method enables the positive effect of a synthetic SL on R. irregularis hyphal branching to be reproduced. This method could thus be useful to quantify the physiological effects of synthesized chemicals or plant-derived specialized metabolites on R. irregularis. Key features • Development of an in vitro hyphal branching assay using germinating spores of Rhizophagus irregularis. • This in vitro assay system builds upon a method developed by Kameoka et al. [1] but modified to make it more applicable to hydrophilic compounds. • Optimized for R. irregularis to count the hyphal branches. • This bioassay requires at least 12 days to be done.

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