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水通道蛋白0在2.2埃分辨率下的通道结构。

The channel architecture of aquaporin 0 at a 2.2-A resolution.

作者信息

Harries William E C, Akhavan David, Miercke Larry J W, Khademi Shahram, Stroud Robert M

机构信息

Macromolecular Structure Group, Department of Biochemistry and Biophysics, University of California, S-412C Genentech Hall, 600 16th Street, San Francisco, CA 94143-2240, USA.

出版信息

Proc Natl Acad Sci U S A. 2004 Sep 28;101(39):14045-50. doi: 10.1073/pnas.0405274101. Epub 2004 Sep 17.

Abstract

We determined the x-ray structure of bovine aquaporin 0 (AQP0) to a resolution of 2.2 A. The structure of this eukaryotic, integral membrane protein suggests that the selectivity of AQP0 for water transport is based on the identity and location of signature amino acid residues that are hallmarks of the water-selective arm of the AQP family of proteins. Furthermore, the channel lumen is narrowed only by two, quasi-2-fold related tyrosine side chains that might account for reduced water conductance relative to other AQPs. The channel is functionally open to the passage of water because there are eight discreet water molecules within the channel. Comparison of this structure with the recent electron-diffraction structure of the junctional form of sheep AQP0 at pH 6.0 that was interpreted as closed shows no global change in the structure of AQP0 and only small changes in side-chain positions. We observed no structural change to the channel or the molecule as a whole at pH 10, which could be interpreted as the postulated pH-gating mechanism of AQP0-mediated water transport at pH >6.5. Contrary to the electron-diffraction structure, the comparison shows no evidence of channel gating induced by association of the extracellular domains of AQP0 at pH 6.0. Our structure aids the analysis of the interaction of the extracellular domains and the possibility of a cell-cell adhesion role for AQP0. In addition, our structure illustrates the basis for formation of certain types of cataracts that are the result of mutations.

摘要

我们确定了牛水通道蛋白0(AQP0)的X射线结构,分辨率为2.2埃。这种真核整合膜蛋白的结构表明,AQP0对水运输的选择性基于特征性氨基酸残基的身份和位置,这些残基是AQP蛋白家族水选择性臂的标志。此外,通道腔仅被两个近似二倍体相关的酪氨酸侧链变窄,这可能解释了相对于其他水通道蛋白水导率降低的原因。通道在功能上对水的通过是开放的,因为通道内有八个离散的水分子。将此结构与最近在pH 6.0时绵羊AQP0连接形式的电子衍射结构(被解释为关闭)进行比较,结果表明AQP0的结构没有全局变化,只有侧链位置有小的变化。我们在pH 10时未观察到通道或整个分子的结构变化,这可以解释为AQP0介导的水运输在pH>6.5时假定的pH门控机制。与电子衍射结构相反,比较结果显示没有证据表明在pH 6.0时AQP0细胞外结构域的缔合会诱导通道门控。我们的结构有助于分析细胞外结构域的相互作用以及AQP0在细胞间粘附作用的可能性。此外,我们的结构阐明了某些类型白内障形成的基础,这些白内障是由突变导致的。

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