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体内 FRET-FLIM 揭示了环境胁迫下 ER 中 ABA 水平的特异性增加。

In vivo FRET-FLIM reveals ER-specific increases in the ABA level upon environmental stresses.

机构信息

Key Laboratory of Molecular Design for Plant Cell Factory of Guangdong Higher Education Institutes, Department of Biology, School of Life Science, Southern University of Science and Technology, Shenzhen 518055, China.

Jiangsu Key Laboratory of Crop Genetics and Physiology/Co-Innovation Center for Modern Production Technology of Grain Crops, Key Laboratory of Plant Functional Genomics of the Ministry of Education, Yangzhou University, Yangzhou 225009, China.

出版信息

Plant Physiol. 2021 Jul 6;186(3):1545-1561. doi: 10.1093/plphys/kiab165.

Abstract

Plant hormone abscisic acid (ABA) is essential for regulating plant growth and various stress responses. ABA-mediated signaling depends on local ABA levels rather than the overall cellular ABA concentration. While cellular concentration of ABA can be detected using Förster resonance energy transfer (FRET)-based ABA probes, direct imaging of subcellular ABA levels remains unsolved. Here, we modified the previously reported ABAleon2.1 and generated a new ABA sensor, named ABAleon2.1_Tao3. Via transient expression in tobacco (Nicotiana tabacum) protoplasts, we targeted ABAleon2.1_Tao3s to the endoplasmic reticulum (ER) membrane with the ABA sensing unit facing the cytosol and the ER, respectively, through a nanobody-epitope-mediated protein interaction. Combining FRET with fluorescence lifetime imaging microscopy, ABA-triggered-specific increases in the fluorescence lifetime of the donor mTurquoise in the ABAleon2.1_Tao3 were detected in both transient assays and stably transformed Arabidopsis plants. In tobacco protoplasts, ER membrane-targeted ABAleon2.1_Tao3s showed a generally higher basal level of ABA in the ER than that in the cytosol and ER-specific alterations in the level of ABA upon environmental cues. In ABAleon2.1_Tao3-transformed Arabidopsis roots, mannitol triggered increases in cytosolic ABA in the division zone and increases in ER ABA in the elongation and maturation zone within 1 h after treatment, both of which were abolished in the bg1-2 mutant, suggesting the requirement for BG1 in osmotic stress-triggered early ABA induction in Arabidopsis roots. These data demonstrate that ABAleon2.1_Tao3s can be used to monitor ABA levels in the cytosol and the ER, providing key information on stress-induced changes in the level of ABA in different subcellular compartments.

摘要

植物激素脱落酸(ABA)是调节植物生长和各种应激反应所必需的。ABA 介导的信号取决于局部 ABA 水平,而不是细胞内 ABA 的总体浓度。虽然可以使用Förster 共振能量转移(FRET)基于 ABA 探针检测细胞内 ABA 浓度,但亚细胞 ABA 水平的直接成像仍然是一个未解决的问题。在这里,我们对之前报道的 ABAleon2.1 进行了修改,并生成了一个新的 ABA 传感器,命名为 ABAleon2.1_Tao3。通过在烟草(Nicotiana tabacum)原生质体中的瞬时表达,我们通过纳米体-表位介导的蛋白质相互作用,将 ABAleon2.1_Tao3 的 ABA 感应单元分别靶向内质网膜的细胞质和内质网,从而将其靶向内质网膜。通过将 FRET 与荧光寿命成像显微镜相结合,我们在瞬时测定和稳定转化的拟南芥植物中均检测到 ABAleon2.1_Tao3 中供体 mTurquoise 的荧光寿命在 ABA 触发后特异性增加。在烟草原生质体中,靶向内质网的 ABAleon2.1_Tao3 在 ER 中表现出通常比细胞质更高的基础 ABA 水平,并且在环境线索作用下 ER 中 ABA 的水平发生了特定的改变。在 ABAleon2.1_Tao3 转化的拟南芥根中,甘露醇处理 1 小时后,分裂区细胞质中 ABA 增加,伸长和成熟区内质网中 ABA 增加,而在 bg1-2 突变体中这两种情况均被消除,表明 BG1 在拟南芥根中渗透胁迫触发早期 ABA 诱导中是必需的。这些数据表明,ABaelon2.1_Tao3 可用于监测细胞质和内质网中 ABA 的水平,为不同亚细胞区室中 ABA 水平的应激诱导变化提供关键信息。

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