Dynamic regulation of guard cell anion channels by cytosolic free Ca2+concentration and protein phosphorylation

被引:109
作者
Chen, Zhong-Hua [1 ]
Hills, Adrian [1 ]
Lim, Choon K. [1 ]
Blatt, Michael R. [1 ]
机构
[1] Fac Biomed & Life Sci, Plant Sci Res Grp, Lab Plant Physiol & Biophys, Glasgow G12 8QQ, Lanark, Scotland
基金
英国生物技术与生命科学研究理事会;
关键词
Ca2+-dependent anion channel; cytosolic-free Ca2+concentration; Ca2+-dependent channel gating; stomatal movement; plasma membrane; Vicia faba L; ABSCISIC-ACID; PLASMA-MEMBRANE; STOMATAL CLOSURE; SIGNAL-TRANSDUCTION; FREE CALCIUM; K+ CHANNELS; HYDROGEN-PEROXIDE; INWARD-RECTIFIER; CA2+ CHANNELS; NITRIC-OXIDE;
D O I
10.1111/j.1365-313X.2009.04108.x
中图分类号
Q94 [植物学];
学科分类号
071001 ;
摘要
P>In guard cells, activation of anion channels (I-anion) is an early event leading to stomatal closure. Activation of I-anion has been associated with abscisic acid (ABA) and its elevation of the cytosolic free Ca2+ concentration ([Ca2+](i)). However, the dynamics of the action of [Ca2+](i) on I-anion has never been established, despite its importance for understanding the mechanics of stomatal adaptation to stress. We have quantified the [Ca2+](i) dynamics of I-anion in Vicia faba guard cells, measuring channel current under a voltage clamp while manipulating and recording [Ca2+](i) using Fura-2 fluorescence imaging. We found that I-anion rises with [Ca2+](i) only at concentrations substantially above the mean resting value of 125 +/- 13 nm, yielding an apparent K-d of 720 +/- 65 nm and a Hill coefficient consistent with the binding of three to four Ca2+ ions to activate the channels. Approximately 30% of guard cells exhibited a baseline of I-anion activity, but without a dependence of the current on [Ca2+](i). The protein phosphatase antagonist okadaic acid increased this current baseline over twofold. Additionally, okadaic acid altered the [Ca2+](i) sensitivity of I-anion, displacing the apparent K-d for [Ca2+](i) to 573 +/- 38 nm. These findings support previous evidence for different modes of regulation for I-anion, only one of which depends on [Ca2+](i), and they underscore an independence of [Ca2+](i) from protein (de-)phosphorylation in controlling I-anion. Most importantly, our results demonstrate a significant displacement of I-anion sensitivity to higher [Ca2+](i) compared with that of the guard cell K+ channels, implying a capacity for variable dynamics between net osmotic solute uptake and loss.
引用
收藏
页码:816 / 825
页数:10
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