Bae Hanhong, Kim Moon S, Sicher Richard C, Bae Hyeun-Jong, Bailey Bryan A
U.S. Department of Agriculture/Agricultural Research Service, Beltsville Agricultural Research Center, Beltsville, Maryland 20705, USA.
Plant Physiol. 2006 Jul;141(3):1056-67. doi: 10.1104/pp.106.076869. Epub 2006 May 12.
Treatment of Arabidopsis (Arabidopsis thaliana) with a necrosis- and ethylene-inducing peptide (Nep1) from Fusarium oxysporum inhibited both root and cotyledon growth and triggered cell death, thereby generating necrotic spots. Nep1-like proteins are produced by divergent microbes, many of which are plant pathogens. Nep1 in the plant was localized to the cell wall and cytosol based on immunolocalization results. The ratio of chlorophyll a fluorescence (F685 nm/F730 nm) significantly decreased after 75-min treatment with Nep1 in comparison to the control. This suggested that a short-term compensation of photosynthesis occurred in response to localized damage to cells. The concentrations of most water-soluble metabolites analyzed were reduced in Arabidopsis seedlings after 6 h of Nep1 treatment, indicating that the integrity of cellular membranes had failed. Microarray results showed that short-term treatment with Nep1 altered expression of numerous genes encoding proteins putatively localized to organelles, especially the chloroplast and mitochondria. Short-term treatment with Nep1 induced multiple classes of genes involved in reactive oxygen species production, signal transduction, ethylene biosynthesis, membrane modification, apoptosis, and stress. Quantitative PCR was used to confirm the induction of genes localized in the chloroplast, mitochondria, and plasma membrane, and genes responsive to calcium/calmodulin complexes, ethylene, jasmonate, ethylene biosynthesis, WRKY, and cell death. The majority of Nep1-induced genes has been associated with general stress responses but has not been critically linked to resistance to plant disease. These results are consistent with Nep1 facilitating cell death as a component of diseases caused by necrotrophic plant pathogens.
用尖孢镰刀菌的坏死和乙烯诱导肽(Nep1)处理拟南芥(Arabidopsis thaliana)会抑制根和子叶的生长,并引发细胞死亡,从而产生坏死斑。Nep1样蛋白由多种微生物产生,其中许多是植物病原体。基于免疫定位结果,植物中的Nep1定位于细胞壁和细胞质。与对照相比,用Nep1处理75分钟后,叶绿素a荧光比值(F685 nm/F730 nm)显著降低。这表明光合作用发生了短期补偿以应对细胞的局部损伤。Nep1处理6小时后,拟南芥幼苗中分析的大多数水溶性代谢物浓度降低,表明细胞膜的完整性已遭到破坏。微阵列结果显示,用Nep1短期处理会改变许多编码假定定位于细胞器(尤其是叶绿体和线粒体)的蛋白质的基因的表达。用Nep1短期处理会诱导参与活性氧产生、信号转导、乙烯生物合成、膜修饰、凋亡和胁迫的多类基因。定量PCR用于确认定位于叶绿体、线粒体和质膜的基因以及对钙/钙调蛋白复合物、乙烯、茉莉酸、乙烯生物合成、WRKY和细胞死亡有响应的基因的诱导。大多数Nep1诱导的基因与一般胁迫反应有关,但与植物病害抗性没有关键联系。这些结果与Nep1促进细胞死亡作为坏死性植物病原体引起的疾病的一个组成部分是一致的。