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光调控的拟南芥光敏色素 A 氨基末端片段的核输入和降解。

Light-regulated nuclear import and degradation of Arabidopsis phytochrome-A N-terminal fragments.

机构信息

Institute of Botany, Biology II, University of Freiburg, Schänzlestrasse 1, D-79104 Freiburg, Germany.

出版信息

Plant Cell Physiol. 2011 Feb;52(2):361-72. doi: 10.1093/pcp/pcq194. Epub 2010 Dec 17.

Abstract

The photoreceptor phytochrome-A (phyA) regulates germination and seedling establishment by mediating very low fluence (VLFR) and far-red high irradiance (FR-HIR) responses in Arabidopsis thaliana. In darkness, phyA homodimers exist in the biologically inactive Pr form and are localized in the cytoplasm. Light induces formation of the biologically active Pfr form and subsequent rapid nuclear import. PhyA Pfr, in contrast to the Pr form, is labile and has a half-life of ∼30 min. We produced transgenic plants in a phyA-201 null background that express the PHYA-yellow fluorescent protein (YFP) or the PHYA686-YFP-dimerization domain (DD) and PHYA686-YFP-DD-nuclear localization signal (NLS) or PHYA686-YFP-DD-nuclear exclusion signal (NES) fusion proteins. The PHYA686-YFP fusion proteins contained the N-terminal domain of phyA (686 amino acid residues), a short DD and the YFP. Here we report that (i) PHYA686-YFP-DD fusion protein is imported into the nucleus in a light-dependent fashion; (ii) neither of the PHYA686 fusion proteins is functional in FR-HIR and nuclear VLFR; and (iii) the phyA-dependent, blue light-induced inhibition of hypocotyl growth is mediated by the PHYA686-YFP-DD-NES but not by the PHYA686-YFP-DD-NLS and PHYA686-YFP-DD fusion proteins. We demonstrate that (i) light induces degradation of all PHYA N-terminal-containing fusion proteins and (ii) these N-terminal domain-containing fusion proteins including the constitutively nuclear PHYA686-YFP-DD-NLS and predominantly cytoplasmic PHYA686-YFP-DD-NES degrade at comparable rates but markedly more slowly than PHYA-YFP, whereas (iii) light-induced degradation of the native phyA is faster compared with PHYA-YFP.

摘要

光受体光敏色素 A(phyA)通过介导拟南芥的极低光(VLFR)和远红光高光(FR-HIR)响应来调节萌发和幼苗建立。在黑暗中,phyA 同源二聚体以生物上无活性的 Pr 形式存在,并定位于细胞质中。光照诱导生物活性 Pfr 形式的形成以及随后的快速核导入。与 Pr 形式相反,phyA Pfr 不稳定,半衰期约为 30 分钟。我们在 phyA-201 缺失背景下产生了表达 PHYA-黄色荧光蛋白(YFP)或 PHYA686-YFP 二聚化结构域(DD)和 PHYA686-YFP-DD-核定位信号(NLS)或 PHYA686-YFP-DD-核排除信号(NES)融合蛋白的转基因植物。PHYA686-YFP 融合蛋白包含 phyA 的 N 端结构域(686 个氨基酸残基)、短的 DD 和 YFP。在这里,我们报告(i)PHYA686-YFP-DD 融合蛋白以光依赖性方式被导入核内;(ii)PHYA686 融合蛋白均不能在 FR-HIR 和核 VLFR 中发挥功能;(iii)phyA 依赖性、蓝光诱导的下胚轴生长抑制由 PHYA686-YFP-DD-NES 介导,而不是由 PHYA686-YFP-DD-NLS 和 PHYA686-YFP-DD 融合蛋白介导。我们证明(i)光诱导所有含有 PHYA N 端结构域的融合蛋白降解,(ii)这些包含 N 端结构域的融合蛋白包括组成型核 PHYA686-YFP-DD-NLS 和主要细胞质 PHYA686-YFP-DD-NES,降解速度相似,但明显慢于 PHYA-YFP,而(iii)与 PHYA-YFP 相比,光诱导的天然 phyA 降解更快。

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