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来自荧光假单胞菌外膜的磷酸盐选择性孔蛋白

Phosphate-selective porins from the outer membranes of fluorescent Pseudomonas sp.

作者信息

Poole K, Parr T R, Hancock R E

出版信息

Can J Microbiol. 1987 Jan;33(1):63-9. doi: 10.1139/m87-011.

DOI:10.1139/m87-011
PMID:2436733
Abstract

Phosphate starvation induced oligomeric proteins from the outer membranes of Pseudomonas fluorescens, Pseudomonas putida, Pseudomonas aureofaciens, and Pseudomonas chlororaphis were purified to homogeneity. The incorporation of the purified proteins into planar lipid bilayer membranes resulted in stepwise increases in membrane conductance. Single channel conductance experiments demonstrated that these proteins were all capable of forming small channels, similar to the Pseudomonas aeruginosa phospsate porin protein P, with average single channel conductances in 1 M KCl of between 233 and 252 pS. Single channel conductance measurements made in salts of varying cation or anion size indicated that the channels were uniformly anion selective. The measurement of single channel conductance as a function of KCl concentration revealed that all channels saturated at higher salt concentrations, consistent with the presence of an anion-binding site in the channel. Apparent Kd values for Cl- binding were calculated and shown to vary only twofold (180-297 mM) among all channels, including protein P channels. Phosphate competitively inhibited chloride conductance through these channels with apparent I50 values of between 0.59 and 2.5 mM phosphate at 40 mM Cl- and between 9.7 and 27 mM phosphate at 1 m Cl-. These data were consistent with the presence of a phosphate-binding site in the channels of these phosphate-regulated proteins. Furthermore, they indicated that these channels exhibit at least a 20- to 80-fold higher affinity for phosphate than for chloride.

摘要

对荧光假单胞菌、恶臭假单胞菌、金色假单胞菌和绿针假单胞菌外膜中由磷酸盐饥饿诱导产生的寡聚蛋白进行了纯化,使其达到均一状态。将纯化后的蛋白整合到平面脂质双分子层膜中,导致膜电导逐步增加。单通道电导实验表明,这些蛋白均能够形成小通道,类似于铜绿假单胞菌磷酸盐孔蛋白P,在1 M KCl中平均单通道电导在233至252 pS之间。在不同阳离子或阴离子大小的盐中进行的单通道电导测量表明,这些通道对阴离子具有一致的选择性。单通道电导作为KCl浓度函数的测量结果表明,所有通道在较高盐浓度下均达到饱和,这与通道中存在阴离子结合位点一致。计算了Cl-结合的表观Kd值,结果表明在所有通道(包括蛋白P通道)中,其变化仅为两倍(180 - 297 mM)。磷酸盐竞争性抑制通过这些通道的氯化物电导,在40 mM Cl-时,表观I50值在0.59至2.5 mM磷酸盐之间,在1 M Cl-时,表观I50值在9.7至27 mM磷酸盐之间。这些数据与这些磷酸盐调节蛋白的通道中存在磷酸盐结合位点一致。此外,这些数据表明,这些通道对磷酸盐的亲和力比对氯化物至少高20至80倍。

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