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Arabidopsis INOSITOL TRANSPORTER2 Mediates H+ Symport of Different Inositol Epimers and Derivatives across the Plasma Membrane

机译:拟南芥INOSITOL TRANSPORTER2介导跨血浆膜的不同肌醇差向异构体和衍生物的H +迁移

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摘要

Of the four genes of the Arabidopsis (Arabidopsis thaliana) INOSITOL TRANSPORTER family (AtINT family) so far only AtINT4 has been described. Here we present the characterization of AtINT2 and AtINT3. cDNA sequencing revealed that the AtINT3 gene is incorrectly spliced and encodes a truncated protein of only 182 amino acids with four transmembrane helices. In contrast, AtINT2 codes for a functional transporter. AtINT2 localization in the plasma membrane was demonstrated by transient expression of an AtINT2-GREEN FLUORESCENT PROTEIN fusion in Arabidopsis and tobacco (Nicotiana tabacum) epidermis cells and in Arabidopsis protoplasts. Its functional and kinetic properties were determined by expression in yeast (Saccharomyces cerevisiae) cells and Xenopus laevis oocytes. Expression of AtINT2 in a Δitr1 (inositol uptake)/Δino1 (inositol biosynthesis) double mutant of bakers' yeast complemented the deficiency of this mutant to grow on low concentrations of myoinositol. In oocytes, AtINT2 mediated the symport of H+ and several inositol epimers, such as myoinositol, scylloinositol, d-chiroinositol, and mucoinositol. The preference for individual epimers differed from that found for AtINT4. Moreover, AtINT2 has a lower affinity for myoinositol (Km = 0.7–1.0 mm) than AtINT4 (Km = 0.24 mm), and the Km is slightly voltage dependent, which was not observed for AtINT4. Organ and tissue specificity of AtINT2 expression was analyzed in AtINT2 promoter/reporter gene plants and showed weak expression in the anther tapetum, the vasculature, and the leaf mesophyll. A T-DNA insertion line (Atint2.1) and an Atint2.1/Atint4.2 double mutant were analyzed under different growth conditions. The physiological roles of AtINT2 are discussed.
机译:迄今为止,在拟南芥(Arabidopsis thaliana)INOSITOL TRANSPORTER家族(AtINT家族)的四个基因中,仅描述了AtINT4。在这里,我们介绍AtINT2和AtINT3的特征。 cDNA测序表明,AtINT3基因的剪接错误,编码的截短蛋白只有182个氨基酸,带有四个跨膜螺旋。相反,AtINT2为功能性转运蛋白编码。 AtINT2在质膜中的定位是通过在拟南芥和烟草(烟草)表皮细胞以及拟南芥原生质体中瞬时表达AtINT2-GREEN荧光蛋白融合蛋白来证明的。通过在酵母(Saccharomyces cerevisiae)细胞和非洲爪蟾(Xenopus laevis)卵母细胞中表达来确定其功能和动力学特性。面包酵母的Δitr1(肌醇摄取)/Δino1(肌醇生物合成)双重突变体中AtINT2的表达弥补了该突变体在低浓度肌醇中生长的缺陷。在卵母细胞中,AtINT2介导H + 与几种肌醇差向异构体(例如肌醇,鞘氨醇,d-手性肌醇和粘液肌醇)的同位体。单个差向异构体的偏好不同于AtINT4。此外,AtINT2对肌醇的亲和力(Km = 0.7–1.0 mm)比AtINT4(Km = 0.24 mm)低, K m电压依赖性很小,而AtINT4则没有。在 AtINT2 启动子/报告基因植物中分析了 AtINT2 表达的器官和组织特异性,并显示在花药绒毡层,脉管系统和叶肉中弱表达。在不同的生长条件下分析了一个T-DNA插入线(Atint2.1)和一个 Atint2.1 / Atint4.2 双突变体。讨论了AtINT2的生理作用。

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