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Anesthetic Effects on Secondary Dormancy and Phytochrome Responses in Setaria faberi Seeds

机译:麻醉对狗尾草种子次生休眠和植物色素反应的影响

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摘要

Seeds of giant foxtail (Setaria faberi Herm.) entered secondary dormancy after pretreatment in H2O at 35°C. Pretreatment in 0.1 m ethanol, or several other substances with anesthetic properties, prevented secondary dormancy induction. Pretreatment in 0.5 m ethanol inhibited germination in darkness, but germination could be stimulated by a red irradiation. Germination was initially insensitive to light. Two separate responses are indicated. The first, affected by a variety of substances and low (0.1 m or less) concentrations of ethanol, is related to anesthetic effects and prevention of secondary dormancy. The second, induction of response to red irradiation, is caused by 0.5 m ethanol and some closely related substances. The anesthetic effect is accomplished within the first 8 hours of imbibition while the phytochrome induction effect required treatment for more than 24 hours. Both responses were lost if the 35°C imbibition began in H2O. Involvement of cell membranes is suggested in the prevention of secondary dormancy by anesthetics.
机译:在35°C的水中预处理后,巨大的狐尾种子(Setaria faberi Herm。)进入次级休眠状态。在0.1 m乙醇或具有麻醉特性的其他几种物质中进行预处理可防止诱导第二次休眠。在0.5 m乙醇中进行预处理可以抑制黑暗中的发芽,但是发芽可以通过红色辐射来刺激。最初,发芽对光不敏感。指出了两个单独的响应。首先,受到多种物质和低浓度(0.1 m或更少)乙醇的影响,与麻醉作用和防止继发性休眠有关。第二,感应红色辐射是由0.5 m乙醇和一些密切相关的物质引起的。麻醉作用在吸收的前8小时内完成,而植物色素的诱导作用则需要治疗24小时以上。如果在H2O中开始35°C的吸收,则两种反应都将丢失。建议通过麻醉使细胞膜参与防止继发性休眠。

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