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与麦芽糖转运复合体激活相关的构象变化的证明

Demonstration of conformational changes associated with activation of the maltose transport complex.

作者信息

Mannering D E, Sharma S, Davidson A L

机构信息

Department of Molecular Virology and Microbiology, Baylor College of Medicine, Houston, Texas 77030, USA.

出版信息

J Biol Chem. 2001 Apr 13;276(15):12362-8. doi: 10.1074/jbc.M011686200. Epub 2001 Jan 9.

DOI:10.1074/jbc.M011686200
PMID:11150310
Abstract

In Escherichia coli, interaction of a periplasmic maltose-binding protein with a membrane-associated ATP-binding cassette transporter stimulates ATP hydrolysis, resulting in translocation of maltose into the cell. The maltose transporter contains two transmembrane subunits, MalF and MalG, and two copies of a nucleotide-hydrolyzing subunit, MalK. Mutant transport complexes that function in the absence of binding protein are thought to be stabilized in an ATPase-active conformation. To probe the conformation of the nucleotide-binding site and to gain an understanding of the nature of the conformational changes that lead to activation, cysteine 40 within the Walker A motif of the MalK subunit was modified by the fluorophore 2-(4'-maleimidoanilino)naphthalene-6-sulfonic acid. Fluorescence differences indicated that residues involved in nucleotide binding were less accessible to aqueous solvent in the binding protein independent transporter than in the wild-type transporter. Similar differences in fluorescence were seen when a vanadate-trapped transition state conformation was compared with the ground state in the wild-type transporter. Our results and recent crystal structures are consistent with a model in which activation of ATPase activity is associated with conformational changes that bring the two MalK subunits closer together, completing the nucleotide-binding sites and burying ATP in the interface.

摘要

在大肠杆菌中,周质麦芽糖结合蛋白与膜相关的ATP结合盒转运体相互作用会刺激ATP水解,从而导致麦芽糖转运到细胞内。麦芽糖转运体包含两个跨膜亚基MalF和MalG,以及两个核苷酸水解亚基MalK的拷贝。在没有结合蛋白的情况下仍能发挥功能的突变转运复合物被认为稳定在ATP酶活性构象中。为了探究核苷酸结合位点的构象,并了解导致激活的构象变化的本质,通过荧光团2-(4'-马来酰亚胺苯胺基)萘-6-磺酸对MalK亚基的沃克A基序内的半胱氨酸40进行了修饰。荧光差异表明,与野生型转运体相比,在无结合蛋白的转运体中,参与核苷酸结合的残基对水性溶剂的可及性较低。当将钒酸盐捕获的过渡态构象与野生型转运体的基态进行比较时,也观察到了类似的荧光差异。我们的结果和最近的晶体结构与一个模型一致,在该模型中,ATP酶活性的激活与构象变化相关,这种构象变化使两个MalK亚基靠得更近,形成完整的核苷酸结合位点并将ATP埋在界面中。

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