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异源表达的植物水通道蛋白SoPIP2;1的5A结构

The 5A structure of heterologously expressed plant aquaporin SoPIP2;1.

作者信息

Kukulski W, Schenk A D, Johanson U, Braun T, de Groot B L, Fotiadis D, Kjellbom P, Engel A

机构信息

Maurice E. Müller Institute for Microscopy, Biozentrum, University of Basel, CH-4056 Basel, Switzerland.

出版信息

J Mol Biol. 2005 Jul 22;350(4):611-6. doi: 10.1016/j.jmb.2005.05.001.

Abstract

SoPIP2;1 is one of the major integral proteins in spinach leaf plasma membranes. In the Xenopus oocyte expression system its water channel activity is regulated by phosphorylation at the C terminus and in the first cytosolic loop. To assess its structure, SoPIP2;1 was heterologously expressed in Pichia pastoris as a His-tagged protein and in the non-tagged form. Both forms were reconstituted into 2D crystals in the presence of lipids. Tubular crystals and double-layered crystalline sheets of non-tagged SoPIP2;1 were observed and analyzed by cryo-electron microscopy. Crystalline sheets were highly ordered and diffracted electrons to a resolution of 2.96A. High-resolution projection maps of tilted specimens provided a 3D structure at 5A resolution. Superposition of the SoPIP2;1 potential map with the atomic model of AQP1 demonstrates the generally well conserved overall structure of water channels. Differences concerning the extracellular loop A explain the particular crystal contacts between oppositely oriented membrane sheets of SoPIP2;1 2D crystals, and may have a function in rapid volume changes observed in stomatal guard cells or mesophyll protoplasts. This crystal packing arrangement provides access to the phosphorylated C terminus as well as the loop B phosphorylation site for studies of channel gating.

摘要

SoPIP2;1是菠菜叶质膜中的主要内在蛋白之一。在非洲爪蟾卵母细胞表达系统中,其水通道活性受C末端和第一个胞质环磷酸化的调节。为了评估其结构,SoPIP2;1在毕赤酵母中作为His标签蛋白和无标签形式进行异源表达。两种形式在脂质存在下都被重构为二维晶体。通过冷冻电子显微镜观察并分析了无标签SoPIP2;1的管状晶体和双层晶体片。晶体片高度有序,电子衍射分辨率达到2.96埃。倾斜标本的高分辨率投影图提供了5埃分辨率的三维结构。SoPIP2;1电位图与AQP1原子模型的叠加表明水通道的总体结构通常保存良好。细胞外环A的差异解释了SoPIP2;1二维晶体中相反取向的膜片之间特殊的晶体接触,并且可能在气孔保卫细胞或叶肉原生质体中观察到的快速体积变化中起作用。这种晶体堆积排列为研究通道门控提供了进入磷酸化C末端以及环B磷酸化位点的途径。

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