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大肠杆菌 sn-甘油-3-磷酸 ATP 结合盒转运蛋白(UgpB-AEC2)的底物特异性和生化特性的决定因素。

Determinants of substrate specificity and biochemical properties of the sn-glycerol-3-phosphate ATP binding cassette transporter (UgpB-AEC2 ) of Escherichia coli.

机构信息

Division of Microbial Physiology, Humboldt-Universität zu Berlin, Unter den Linden 6, D-10099, Berlin, Germany.

出版信息

Mol Microbiol. 2012 Nov;86(4):908-20. doi: 10.1111/mmi.12025. Epub 2012 Sep 27.

DOI:10.1111/mmi.12025
PMID:23013274
Abstract

Under phosphate starvation conditions, Escherichia coli can utilize sn-glycerol-3-phosphate (G3P) and G3P diesters as phosphate source when transported by an ATP binding cassette importer composed of the periplasmic binding protein, UgpB, the transmembrane subunits, UgpA and UgpE, and a homodimer of the nucleotide binding subunit, UgpC. The current knowledge on the Ugp transporter is solely based on genetic evidence and transport assays using intact cells. Thus, we set out to characterize its properties at the level of purified protein components. UgpB was demonstrated to bind G3P and glycerophosphocholine with dissociation constants of 0.68 ± 0.02 μM and 5.1 ± 0.3 μM, respectively, while glycerol-2-phosphate (G2P) is not a substrate. The crystal structure of UgpB in complex with G3P was solved at 1.8 Å resolution and revealed the interaction with two tryptophan residues as key to the preferential binding of linear G3P in contrast to the branched G2P. Mutational analysis validated the crucial role of Trp-169 for G3P binding. The purified UgpAEC2 complex displayed UgpB/G3P-stimulated ATPase activity in proteoliposomes that was neither inhibited by phosphate nor by the signal transducing protein PhoU or the phosphodiesterase UgpQ. Furthermore, a hybrid transporter composed of MalFG-UgpC could be functionally reconstituted while a UgpAE-MalK complex was unstable.

摘要

在磷酸盐饥饿条件下,大肠杆菌可以利用 sn-甘油-3-磷酸(G3P)和 G3P 二酯作为磷酸源,此时它们通过由周质结合蛋白 UgpB、跨膜亚基 UgpA 和 UgpE 以及核苷酸结合亚基 UgpC 组成的 ATP 结合盒进口器进行运输。目前关于 Ugp 转运体的知识仅基于遗传证据和使用完整细胞进行的转运测定。因此,我们着手在纯化的蛋白成分水平上表征其特性。证明 UgpB 与 G3P 和甘油磷酸胆碱的结合解离常数分别为 0.68±0.02μM 和 5.1±0.3μM,而甘油-2-磷酸(G2P)不是底物。UgpB 与 G3P 复合物的晶体结构在 1.8Å分辨率下得到解决,揭示了与两个色氨酸残基的相互作用是优先结合线性 G3P 而不是支链 G2P 的关键。突变分析验证了色氨酸 169 对 G3P 结合的关键作用。在脂质体中,纯化的 UgpAEC2 复合物显示出 UgpB/G3P 刺激的 ATP 酶活性,既不受磷酸盐抑制,也不受信号转导蛋白 PhoU 或磷酸二酯酶 UgpQ 抑制。此外,MalFG-UgpC 组成的杂种转运体可以功能性重建,而 UgpAE-MalK 复合物不稳定。

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