首页> 外文OA文献 >Induction of Secondary Dormancy in Chenopodium bonus-henricus L. Seeds by Osmotic and High Temperature Treatments and Its Prevention by Light and Growth Regulators 1
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Induction of Secondary Dormancy in Chenopodium bonus-henricus L. Seeds by Osmotic and High Temperature Treatments and Its Prevention by Light and Growth Regulators 1

机译:渗透和高温处理诱导藜藜种子次生休眠及其光和生长调节剂的预防1

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摘要

Factors controlling the establishment and removal of secondary dormancy in Chenopodium bonus-henricus L. seeds were investigated. Unchilled seeds required light for germination. A moist-chilling treatment at 4 C for 28 to 30 days removed this primary dormancy. Chilled seeds now germinated in the dark. When chilled seeds were held in the dark in −8.6 bars polyethylene glycol 6000 solution at 15 C or in water at 29 C a secondary dormancy was induced which increased progressively with time as determined by subsequent germination. These seeds now failed to germinate under the condition (darkness) which previously allowed their germination. Continuous light or daily brief red light irradiations during prolonged imbibition in polyethylene glycol solution at 15 C or in water at 29 C prevented the establishment of the secondary dormancy and caused an advancement of subsequent germination. Far red irradiations immediately following red irradiation reestablished the secondary dormancy indicating phytochrome participation in “pregerminative” processes. The growth regulator combination, kinetin + ethephon + gibberellin A4+A7 (GA4+7), and to a relatively lesser extent GA4+7, was effective in preventing the establishment of the secondary dormancy and in advancing the germination or emergence time. Following the establishment of the secondary dormancy by osmotic or high temperature treatments the regulator combination was relatively more active than light or GA4+7 in removing the dormancy. Prolonged dark treatment at 29 C seemed to induce changes that were partially independent of light or GA4+7 control. The data presented here indicate that changes during germination preventing dark treatment determine whether the seed will germinate, show an advancement effect, or will become secondarily dormant. These changes appear to be modulated by light and hormones.
机译:研究了控制藜加红种子种子次生休眠的建立和去除的因素。未冷冻的种子需要光才能发芽。在4 C下进行湿冷处理28到30天可以消除这种主要的休眠状态。现在,冷冻种子在黑暗中发芽。当将冷冻种子在15°C下于-8.6 bar的聚乙二醇6000溶液中于黑暗中或在29°C的水中置于黑暗中时,诱导了第二休眠,该休眠随着时间的推移逐渐增加,这取决于随后的萌发。这些种子现在在先前允许其发芽的条件(黑暗)下无法发芽。在15°C的聚乙二醇溶液或29°C的水中长时间吸收期间,连续或每天短暂的红光照射会阻止二次休眠的建立,并导致随后的发芽进程。紧随红色辐照后的远红色辐照重新建立了第二休眠状态,表明植物色素参与了“萌芽”过程。生长调节剂组合,激动素+乙烯利+赤霉素A4 + A7(GA4 + 7),以及相对较小程度的GA4 + 7,可有效防止继发性休眠的建立并延长发芽或出苗时间。在通过渗透或高温处理建立了第二休眠之后,调节剂组合在去除休眠方面比光或GA4 + 7相对更活跃。在29°C下长时间进行黑暗处理似乎会引起部分独立于光照或GA4 + 7对照的变化。此处提供的数据表明,发芽过程中发生的变化防止了黑暗处理,这决定了种子是否将发芽,显示出增效作用或将变得次要休眠。这些变化似乎受到光和激素的调节。

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