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氧化应激下气孔行为和保卫细胞胞质游离钙的变化

Changes in Stomatal Behavior and Guard Cell Cytosolic Free Calcium in Response to Oxidative Stress.

作者信息

McAinsh M. R., Clayton H., Mansfield T. A., Hetherington A. M.

机构信息

Institute of Environmental and Biological Sciences, Division of Biological Sciences, Lancaster University, Lancaster, United Kingdom LA1 4YQ.

出版信息

Plant Physiol. 1996 Aug;111(4):1031-1042. doi: 10.1104/pp.111.4.1031.

Abstract

We have investigated the cellular basis for the effects of oxidative stress on stomatal behavior using stomatal bioassay and ratio photometric techniques. Two oxidative treatments were employed in this study: (a) methyl viologen, which generates superoxide radicals, and (b) H2O2. Both methyl viologen and H2O2 inhibited stomatal opening and promoted stomatal closure. At concentrations [less than or equal to]10-5 M, the effects of methyl viologen and H2O2 on stomatal behavior were reversible and were abolished by 2 mM EGTA or 10 [mu]M verapamil. In addition, at 10-5 M, i.e. the maximum concentration at which the effects of the treatments were prevented by EGTA or verapamil, methyl viologen and H2O2 caused an increase in guard cell cytosolic free Ca2+ ([Ca2+]i), which was abolished in the presence of EGTA. Therefore, at low concentrations of methyl viologen and H2O2, removal of extracellular Ca2+ prevented both the oxidative stress-induced changes in stomatal aperture and the associated increases in [Ca2+]i. This suggests that in this concentration range the effects of the treatments are Ca2+-dependent and are mediated by changes in [Ca2+]i. In contrast, at concentrations of methyl viologan and H2O2 > 10-5 M, EGTA and verapamil had no effect. However, in this concentration range the effects of the treatments were irreversible and correlated with a marked reduction in membrane integrity and guard cell viability. This suggests that at high concentrations the effects of methyl viologen and H2O2 may be due to changes in membrane integrity. The implications of oxidative stress-induced increases in [Ca2+]i and the possible disruption of guard-cell Ca2+ homeostasis are discussed in relation to the processes of Ca2+-based signal transduction in stomatal guard cells and the control of stomatal aperture.

摘要

我们使用气孔生物测定法和比率光度技术研究了氧化应激对气孔行为影响的细胞基础。本研究采用了两种氧化处理方法:(a)甲基紫精,可产生超氧自由基;(b)过氧化氢。甲基紫精和过氧化氢均抑制气孔开放并促进气孔关闭。在浓度≤10⁻⁵ M时,甲基紫精和过氧化氢对气孔行为的影响是可逆的,并且被2 mM乙二醇双乙醚二胺四乙酸(EGTA)或10 μM维拉帕米消除。此外,在10⁻⁵ M时,即EGTA或维拉帕米阻止处理效果的最大浓度,甲基紫精和过氧化氢导致保卫细胞胞质游离钙离子([Ca²⁺]i)增加,在EGTA存在时这种增加被消除。因此,在低浓度的甲基紫精和过氧化氢下,去除细胞外钙离子可防止氧化应激诱导的气孔孔径变化以及相关的[Ca²⁺]i增加。这表明在该浓度范围内,处理效果依赖于钙离子且由[Ca²⁺]i的变化介导。相反,在甲基紫精和过氧化氢浓度>10⁻⁵ M时,EGTA和维拉帕米没有作用。然而,在该浓度范围内,处理效果是不可逆的,并且与膜完整性和保卫细胞活力的显著降低相关。这表明在高浓度时,甲基紫精和过氧化氢的作用可能是由于膜完整性的变化。结合气孔保卫细胞中基于钙离子的信号转导过程和气孔孔径的控制,讨论了氧化应激诱导的[Ca²⁺]i增加以及保卫细胞钙离子稳态可能被破坏的影响。

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