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首页> 外文期刊>Plant physiology >MASTOPARAN-INDUCED INTRACELLULAR CA2+ FLUXES MAY REGULATE CELL-TO-CELL COMMUNICATION IN PLANTS
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MASTOPARAN-INDUCED INTRACELLULAR CA2+ FLUXES MAY REGULATE CELL-TO-CELL COMMUNICATION IN PLANTS

机译:MASTOPARAN诱导的细胞内CA2 +通量可能调节植物中的细胞间通讯

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摘要

The relationship of Ca2+ and plasmodesmatal closure was examined in staminal hairs of Setcreasea purpurea by microinjecting cells with active mastoparan (Mas-7), inactive mastoparan (Mas-17), active inositol-1,4,5-trisphosphate (IP3), or inactive IP3. Calcium green dextran 10,000 was used to study cellular free Ca2+, and carboxyfluorescein was used to monitor plasmodesmatal closure. When Mas-7 was microinjected into the cytoplasm of cell 1 (the tip cell of a chain of cells), a rapid increase in calcium green dextran-10,000 fluorescence was observed in the cytoplasmic areas on both sides of the plasmodesmata connecting cells 1 and 2 during the same time that the diffusion of carboxyfluorescein through them was blocked. The inhibition of cell-to-cell diffusion was transient, and the closed plasmodesmata reopened within 30 s. The elevated Ca2+ level near plasmodesmata was also transient and returned to base level in about 1.5 min. The transient increase in Ca2+, once initiated in cell 1, repeated with an oscillatory period of 3 min. Elevated Ca2+ and oscillations of Ca2+ were also observed near interconnecting cell walls throughout the chain of cells, indicating that the signal had been transmitted. Previously, we reported that IP3 closed plasmodesmata; now we report that it stimulated Ca2+ and oscillations similar to Mas-7. The effect was specific for similar concentrations of Mas-7 over Mas-17 and active IP3 over inactive IP3. It is important that the Ca2+ channel blocker La3+ eliminated the responses from Mas-7 and IP3, indicating that an influx of Ca2+ was required. These results support the contention that plasmodesmata functioning is regulated via Ca2+ and that IP3 may be an intermediary between the stimulus and Ca2+ elevations. [References: 49]
机译:Ca2 +与紫茎泽兰的毛发之间的关系通过微注射具有活性紫杉醇(Mas-7),无活性紫杉醇(Mas-17),活性肌醇-1,4,5-三三磷酸(IP3)或无效的IP3。钙绿色葡聚糖10,000用于研究细胞中游离的Ca2 +,而羧基荧光素用于监测胞膜关闭。当将Mas-7微注射到细胞1(细胞链的末端细胞)的细胞质中时,在连接细胞1和2的胞膜两侧的细胞质区域中观察到钙绿葡聚糖10,000荧光迅速增加。同时阻止了羧基荧光素通过它们的扩散。细胞间扩散的抑制作用是短暂的,并且封闭的胞膜瘤在30 s内重新开放。胞膜附近的Ca2 +水平升高也是短暂的,并在约1.5分钟内恢复到基本水平。一旦在细胞1中引发,Ca2 +的瞬时增加就会重复3分钟的振荡周期。在整个细胞链的相互连接的细胞壁附近也观察到了Ca2 +升高和Ca2 +振荡,表明信号已被传输。以前,我们报道说IP3封闭了胞质。现在我们报道它刺激了Ca2 +和类似于Mas-7的振荡。对于在Mas-17上相似的Mas-7浓度和在非活性IP3上相似的活性IP3,效果是特定的。 Ca2 +通道阻滞剂La3 +消除了Mas-7和IP3的响应很重要,这表明需要大量Ca2 +的流入。这些结果支持以下观点:线虫功能是通过Ca2 +调节的,而IP3可能是刺激和Ca2 +升高之间的中介。 [参考:49]

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