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通过对拟南芥 Pht1;1 中的酪氨酸 312 进行定点突变,增加了磷酸盐的转运,这可能归因于同型相互作用的破坏。

Increased phosphate transport of Arabidopsis thaliana Pht1;1 by site-directed mutagenesis of tyrosine 312 may be attributed to the disruption of homomeric interactions.

机构信息

Department of Biological Sciences, Louisiana State University, Baton Rouge, LA, 70803, USA.

Agricultural Biotechnology Research Center, Academia Sinica, Taipei, 11529, Taiwan, China.

出版信息

Plant Cell Environ. 2015 Oct;38(10):2012-22. doi: 10.1111/pce.12522. Epub 2015 Apr 17.

DOI:10.1111/pce.12522
PMID:25754174
Abstract

Members of the Pht1 family of plant phosphate (Pi) transporters play vital roles in Pi acquisition from soil and in planta Pi translocation to maintain optimal growth and development. The study of the specificities and biochemical properties of Pht1 transporters will contribute to improving the current understanding of plant phosphorus homeostasis and use-efficiency. In this study, we show through split in vivo interaction methods and in vitro analysis of microsomal root tissues that Arabidopsis thaliana Pht1;1 and Pht1;4 form homomeric and heteromeric complexes. Transient and heterologous expression of the Pht1;1 variants, Pht1;1(Y312D), Pht1;1(Y312A) and Pht1;1(Y312F), was used to analyse the role of a putative Pi binding residue (Tyr 312) in Pht1;1 transporter oligomerization and function. The homomeric interaction among Pht1;1 proteins was disrupted by mutation of Tyr 312 to Asp, but not to Ala or Phe. In addition, the Pht1;1(Y312D) variant conferred enhanced Pi transport when expressed in yeast cells. In contrast, mutation of Tyr 312 to Ala or Phe did not affect Pht1;1 transport kinetics. Our study demonstrates that modifications to the Pht1;1 higher-order structure affects Pi transport, suggesting that oligomerization may serve as a regulatory mechanism for modulating Pi uptake.

摘要

植物磷酸盐(Pi)转运蛋白 Pht1 家族的成员在从土壤中获取 Pi 和在植物体内将 Pi 转运到维持最佳生长和发育中发挥着重要作用。对 Pht1 转运蛋白的特异性和生化特性的研究将有助于提高对植物磷稳态和利用效率的现有理解。在这项研究中,我们通过体内分裂相互作用方法和对微体根组织的体外分析表明,拟南芥 Pht1;1 和 Pht1;4 形成同型和异型复合物。瞬时和异源表达 Pht1;1 变体 Pht1;1(Y312D)、Pht1;1(Y312A)和 Pht1;1(Y312F),用于分析假定的 Pi 结合残基(Tyr 312)在 Pht1;1 转运蛋白寡聚化和功能中的作用。Pht1;1 蛋白之间的同源相互作用被突变 Tyr 312 为 Asp 破坏,但不是 Ala 或 Phe。此外,当在酵母细胞中表达时,Pht1;1(Y312D)变体赋予增强的 Pi 转运。相比之下,突变 Tyr 312 为 Ala 或 Phe 不会影响 Pht1;1 运输动力学。我们的研究表明,Pht1;1 高级结构的修饰会影响 Pi 转运,表明寡聚化可能是调节 Pi 摄取的一种调节机制。

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