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ABI3调节ABI1的功能,以控制主根伸长区的细胞长度。

ABI3 regulates ABI1 function to control cell length in primary root elongation zone.

作者信息

Datta Saptarshi, Mandal Drishti, Mitra Sicon, Chakraborty Swarnavo, Nag Chaudhuri Ronita

机构信息

Department of Biotechnology, St. Xavier's College, 30, Mother Teresa Sarani, Kolkata, 700016, India.

出版信息

Plant J. 2024 Dec;120(6):2437-2455. doi: 10.1111/tpj.17121. Epub 2024 Nov 4.

Abstract

Post-embryonic primary root growth is effectively an interplay of several hormone signalling pathways. Here, we show that the ABA-responsive transcription factor ABI3 controls primary root growth through the regulation of JA signalling molecule JAZ1 along with ABA-responsive factor ABI1. In the absence of ABI3, the primary root elongation zone is shortened with significantly reduced cell length. Expression analyses and ChIP-based assays indicate that ABI3 negatively regulates JAZ1 expression by occupying its upstream regulatory sequence and enriching repressive histone modification mark H3K27 trimethylation, thereby occluding RNAPII occupancy. Previous studies have shown that JAZ1 interacts with ABI1, the protein phosphatase 2C, that works during ABA signalling. Our results indicate that in the absence of ABI3, when JAZ1 expression levels are high, the ABI1 protein shows increased stability, compared to when JAZ1 is absent, or ABI3 is overexpressed. Consequently, in the abi3-6 mutant, due to the higher stability of ABI1, reduced phosphorylation of plasma membrane H-ATPase (AHA2) occurs. HPTS staining further indicated that abi3-6 root cell apoplasts show reduced protonation, compared to wild-type and ABI3 overexpressing seedlings. Such impeded proton extrusion negatively affects cell length in the primary root elongation zone. ABI3 therefore controls cell elongation in the primary root by affecting the ABI1-dependent protonation of root cell apoplasts. In summary, ABI3 controls the expression of JAZ1 and in turn modulates the function of ABI1 to regulate cell length in the elongation zone during primary root growth.

摘要

胚后初生根的生长实际上是几种激素信号通路相互作用的结果。在此,我们表明脱落酸响应转录因子ABI3通过与脱落酸响应因子ABI1一起调控茉莉酸信号分子JAZ1来控制初生根生长。在没有ABI3的情况下,初生根伸长区缩短,细胞长度显著减小。表达分析和基于染色质免疫沉淀的实验表明,ABI3通过占据JAZ1的上游调控序列并富集抑制性组蛋白修饰标记H3K27三甲基化来负调控JAZ1的表达,从而阻止RNA聚合酶II的占据。先前的研究表明,JAZ1与在脱落酸信号传导过程中起作用的蛋白磷酸酶2C即ABI1相互作用。我们的结果表明,在没有ABI3的情况下,当JAZ1表达水平较高时,与JAZ1不存在或ABI3过表达时相比,ABI1蛋白显示出更高的稳定性。因此,在abi3 - 6突变体中,由于ABI1的稳定性较高,质膜H⁺ - ATP酶(AHA2)的磷酸化减少。HPTS染色进一步表明,与野生型和过表达ABI3的幼苗相比,abi3 - 6根细胞质外体的质子化减少。这种质子外排受阻对初生根伸长区的细胞长度产生负面影响。因此,ABI3通过影响根细胞质外体中依赖于ABI1的质子化来控制初生根中的细胞伸长。总之,ABI3控制JAZ1的表达,进而调节ABI1的功能,以在初生根生长过程中调节伸长区的细胞长度。

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