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来自枯草芽孢杆菌的果糖通透酶(IIBLev)IIB亚基的晶体结构。

Crystal structure of the IIB subunit of a fructose permease (IIBLev) from Bacillus subtilis.

作者信息

Schauder S, Nunn R S, Lanz R, Erni B, Schirmer T

机构信息

Department of Structural Biology, University of Basel, Switzerland.

出版信息

J Mol Biol. 1998 Feb 27;276(3):591-602. doi: 10.1006/jmbi.1997.1544.

DOI:10.1006/jmbi.1997.1544
PMID:9551099
Abstract

The bacterial phosphoenolpyruvate-dependent phosphotransferase system (PTS) mediates both the uptake of carbohydrates across the cytoplasmic membrane and their phosphorylation. During this process, a phosphoryl group is transferred from phosphoenolpyruvate via the general PTS proteins enzyme I, HPr and the sugar-specific components IIA, IIB to the transported sugar. The crystal structure of the IIB subunit of a fructose transporter from Bacillus subtilis (IIBLev) was solved by MIRAS to a resolution of 2.9 A. IIBLev comprises 163 amino acid residues that are folded into an open, mainly parallel beta-sheet with helices packed on either face. The phosphorylation site (His15) is located on the first loop (1/A) at one of the topological switch-points of the fold. Despite different global folds, IIBLev and HPr have very similar active-site loop conformations with the active-site histidine residues located close to the N terminus of the first helix. This resemblance may be of functional importance, since both proteins exchange a phosphoryl group with the same IIA subunit. The structural basis of phosphoryl transfer from HPr to IIAMan to IIBMan was investigated by modeling of the respective transition state complexes using the known HPr and IIAMan structures and a homology model of IIBMan that was derived from the IIBLev structure. All three proteins contain a helix that appears to be suitable for stabilization of the phospho-histidine by dipole and H-bonding interactions. Smooth phosphoryl transfer from one N-cap position to the other appears feasible with a minimized transition state energy due to simultaneous interactions with the donor and the acceptor helix.

摘要

细菌磷酸烯醇丙酮酸依赖性磷酸转移酶系统(PTS)介导碳水化合物跨细胞质膜的摄取及其磷酸化过程。在此过程中,磷酸基团从磷酸烯醇丙酮酸经通用PTS蛋白酶I、HPr以及糖特异性组分IIA、IIB转移至被转运的糖上。通过分子置换法(MIRAS)解析了枯草芽孢杆菌果糖转运体IIB亚基(IIBLev)的晶体结构,分辨率为2.9埃。IIBLev由163个氨基酸残基组成,折叠成一个开放的、主要为平行的β折叠片层,螺旋堆积在两侧。磷酸化位点(His15)位于折叠结构拓扑转换点之一的第一个环(1/A)上。尽管整体折叠结构不同,但IIBLev和HPr具有非常相似的活性位点环构象,活性位点组氨酸残基位于第一个螺旋的N端附近。这种相似性可能具有功能重要性,因为这两种蛋白都与同一个IIA亚基交换磷酸基团。利用已知的HPr和IIAMan结构以及从IIBLev结构推导得到的IIBMan同源模型,对从HPr到IIAMan再到IIBMan的磷酰基转移的结构基础进行了相应过渡态复合物的建模研究。所有这三种蛋白都包含一个螺旋,该螺旋似乎适合通过偶极和氢键相互作用来稳定磷酰化组氨酸。由于与供体螺旋和受体螺旋同时相互作用,磷酰基从一个N帽位置平滑转移到另一个位置似乎是可行的,且过渡态能量最小。

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