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配体诱导的大肠杆菌K-12铁色素-铁受体的构象变化。

Ligand-induced conformational change in the ferrichrome-iron receptor of Escherichia coli K-12.

作者信息

Moeck G S, Tawa P, Xiang H, Ismail A A, Turnbull J L, Coulton J W

机构信息

Department of Microbiology and Immunology, McGill University, Montreal, Canada.

出版信息

Mol Microbiol. 1996 Nov;22(3):459-71. doi: 10.1046/j.1365-2958.1996.00112.x.

DOI:10.1046/j.1365-2958.1996.00112.x
PMID:8939430
Abstract

Ferrichrome-iron is actively transported across the outer membrane of Escherichia coli by the TonB-dependent receptor FhuA. To obtain FhuA in a form suitable for secondary-structure analyses, a hexahistidine tag was inserted into a surface-located site and the recombinant protein was purified by metal chelate chromatography. Functional studies indicated that the presence of the hexahistidine tag did not interfere with FhuA localization or with ligand-binding activity. Ferrichrome protected lysine 67 but not lysine 5 of purified recombinant FhuA from trypsinolysis. Results from trypsin digestion were interpreted as a conformational change in FhuA which had occurred upon ferrichrome binding, thereby preventing access of trypsin to lysine 67. Circular dichroism and Fourier transform infrared spectroscopy revealed a predominance of beta-sheet structure for the purified protein. In the presence of ferrichrome, FhuA exhibited a secondary structure and a thermostability which were similar to FhuA without ligand. The addition of ferrichrome to purified FhuA reduced the ability of certain anti-FhuA monoclonal antibodies to bind to the receptor. All antibodies which could in this manner discriminate between FhuA and FhuA bound to ferrichrome had their determinants within a loop which is toward the N-terminus and which is exposed to the periplasm. These data indicate that the binding of ferrichrome induces a structural change that is propogated across the outer membrane and results in an altered conformation of a periplasmically exposed loop of FhuA. It is proposed that by such an alteration of FhuA conformation, TonB is triggered to energize the active transport of the bound ligand across the outer membrane.

摘要

高铁载体铁通过依赖TonB的受体FhuA被主动转运穿过大肠杆菌的外膜。为了获得适合二级结构分析的FhuA形式,在一个位于表面的位点插入了一个六组氨酸标签,并通过金属螯合层析纯化重组蛋白。功能研究表明,六组氨酸标签的存在不干扰FhuA的定位或配体结合活性。高铁载体保护纯化的重组FhuA的赖氨酸67不被胰蛋白酶消化,但不保护赖氨酸5。胰蛋白酶消化的结果被解释为FhuA在结合高铁载体后发生了构象变化,从而阻止胰蛋白酶接近赖氨酸67。圆二色性和傅里叶变换红外光谱显示纯化蛋白以β-折叠结构为主。在高铁载体存在的情况下,FhuA表现出与无配体的FhuA相似的二级结构和热稳定性。向纯化的FhuA中添加高铁载体降低了某些抗FhuA单克隆抗体与受体结合的能力。所有能够以这种方式区分FhuA和结合高铁载体的FhuA的抗体,其决定簇都在一个朝向N端且暴露于周质的环内。这些数据表明,高铁载体的结合诱导结构变化,该变化在外膜上传播,导致FhuA周质暴露环的构象改变。有人提出,通过FhuA构象的这种改变,TonB被触发以激发结合配体跨外膜的主动转运。

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