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水通道蛋白-1在平面脂质双分子层中的水和离子渗透。结构决定因素和化学计量的主要差异。

Water and ion permeation of aquaporin-1 in planar lipid bilayers. Major differences in structural determinants and stoichiometry.

作者信息

Saparov S M, Kozono D, Rothe U, Agre P, Pohl P

机构信息

Nachwuchsgruppe Biophysik, Forschungsinstitut für Molekulare Pharmakologie, Robert-Rössle-Strasse 10, 13125 Berlin, Germany.

出版信息

J Biol Chem. 2001 Aug 24;276(34):31515-20. doi: 10.1074/jbc.M104267200. Epub 2001 Jun 15.

DOI:10.1074/jbc.M104267200
PMID:11410596
Abstract

The aquaporin-1 (AQP1) water channel protein is known to facilitate the rapid movement of water across cell membranes, but a proposed secondary role as an ion channel is still unsettled. Here we describe a method to simultaneously measure water permeability and ion conductance of purified human AQP1 after reconstitution into planar lipid bilayers. Water permeability was determined by measuring Na(+) concentrations adjacent to the membrane. Comparisons with the known single channel water permeability of AQP1 indicate that the planar lipid bilayers contain from 10(6) to 10(7) water channels. Addition of cGMP induced ion conductance in planar bilayers containing AQP1, whereas cAMP was without effect. The number of water channels exceeded the number of active ion channels by approximately 1 million-fold, yet p-chloromethylbenzenesulfonate inhibited the water permeability but not ion conductance. Identical ion channel parameters were achieved with AQP1 purified from human red blood cells or AQP1 heterologously expressed in Saccharomyces cerevisae and affinity purified with either N- or C-terminal poly-histidine tags. Rp-8-Br-cGMP inhibited all of the observed conductance levels of the cation selective channel (2, 6, and 10 pS in 100 mm Na(+) or K(+)). Deletion of the putative cGMP binding motif at the C terminus by introduction of a stop codon at position 237 yielded a truncated AQP1 protein that was still permeated by water but not by ions. Our studies demonstrate a method for simultaneously measuring water permeability and ion conductance of AQP1 reconstituted into planar lipid bilayers. The ion conductance occurs (i) through a pathway distinct from the aqueous pathway, (ii) when stimulated directly by cGMP, and (iii) in only an exceedingly small fraction of AQP1 molecules.

摘要

水通道蛋白-1(AQP1)水通道蛋白已知可促进水在细胞膜上的快速移动,但作为离子通道的潜在次要作用仍未确定。在这里,我们描述了一种在重组到平面脂质双分子层后同时测量纯化的人AQP1的水渗透性和离子电导率的方法。通过测量膜附近的Na(+)浓度来确定水渗透性。与已知的AQP1单通道水渗透性比较表明,平面脂质双分子层包含10(6)至10(7)个水通道。添加cGMP可在含有AQP1的平面双分子层中诱导离子电导率,而cAMP则无作用。水通道的数量比活性离子通道的数量大约多100万倍,但对氯甲基苯磺酸盐抑制水渗透性但不抑制离子电导率。用从人红细胞纯化的AQP1或在酿酒酵母中异源表达并用N端或C端多组氨酸标签亲和纯化的AQP1获得相同的离子通道参数。Rp-8-Br-cGMP抑制阳离子选择性通道的所有观察到的电导率水平(在100 mM Na(+)或K(+)中为2、6和10 pS)。通过在第237位引入终止密码子删除C端假定的cGMP结合基序,产生了一种截短的AQP1蛋白,该蛋白仍可被水渗透但不能被离子渗透。我们的研究证明了一种同时测量重组到平面脂质双分子层中的AQP1的水渗透性和离子电导率的方法。离子电导率发生在(i)通过与水通道不同的途径,(ii)直接由cGMP刺激时,以及(iii)仅在极少数AQP1分子中。

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