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大肠杆菌L-阿拉伯糖结合蛋白的质子核磁共振光谱和配体结合动力学

Proton nuclear magnetic resonance spectroscopy and ligand binding dynamics of the Escherichia coli L-arabinose binding protein.

作者信息

Clark A F, Gerken T A, Hogg R W

出版信息

Biochemistry. 1982 Apr 27;21(9):2227-33. doi: 10.1021/bi00538a035.

DOI:10.1021/bi00538a035
PMID:7046797
Abstract

The L-arabinose binding protein (ABP) from Escherichia coli was studied by proton nuclear magnetic resonance spectroscopy (1H NMR). Distinct spectral changes occur when ABP binds its natural ligand, L-arabinose, which involve resonances in the aromatic ring current shifted methyl, bulk methyl, methylene, aromatic, and amide proton regions of the spectra. Several amide resonances can be "protected" from deuterium exchange if L-arabinose is bound to ABP prior to deuterium oxide dialysis. On the basis of the pH dependence of their chemical shifts, two low-field resonances have been tentatively assigned to C2 protons of two of the three histidines present in ABP. These histidyl residues have pK values of 8.0 and 8.6 which support their involvement in ionic interactions observed earlier in the crystallographic analysis. One histidyl residue shows a small chemical shift change upon the addition of arabinose. When ABP binds D-galactose, changes in the spectra occur which are different than those observed when L-arabinose is bound. Binding of L-arabinose and D-galactose to the binding protein (ABP) was considered by equilibrium binding and fluorescence emission spectroscopy. ABP binds L-arabinose and D-galactose with high affinities (Kd's at 6 degrees C of 1.3 x 10(-7) and 1.9 x 10(-7) M, respectively), and both enthalpy and entropy contribute to the ABP-ligand association. When excited at 285 nm, ABP has a fluorescence emission maximum of 340 nm which is quenched and blue shifted (to 337 nm) upon binding L-arabinose. ABP binding D-galactose produced a similar emission shift but no fluorescence quenching.

摘要

利用质子核磁共振波谱法(1H NMR)对大肠杆菌的L-阿拉伯糖结合蛋白(ABP)进行了研究。当ABP与其天然配体L-阿拉伯糖结合时,会发生明显的光谱变化,这涉及到光谱中芳香环电流位移甲基、大量甲基、亚甲基、芳香族和酰胺质子区域的共振。如果在重水透析之前L-阿拉伯糖已与ABP结合,则几个酰胺共振可免受氘交换的影响。根据其化学位移的pH依赖性,已初步将两个低场共振归属于ABP中三个组氨酸中两个组氨酸的C2质子。这些组氨酸残基的pK值分别为8.0和8.6,这支持了它们参与早期晶体学分析中观察到的离子相互作用。一个组氨酸残基在添加阿拉伯糖后显示出较小的化学位移变化。当ABP结合D-半乳糖时,会发生与结合L-阿拉伯糖时观察到的不同的光谱变化。通过平衡结合和荧光发射光谱法研究了L-阿拉伯糖和D-半乳糖与结合蛋白(ABP)的结合。ABP以高亲和力结合L-阿拉伯糖和D-半乳糖(6℃时的Kd分别为1.3×10-7和1.9×10-7 M),焓和熵都对ABP-配体缔合有贡献。当在285 nm激发时,ABP的荧光发射最大值为340 nm,在结合L-阿拉伯糖时会发生猝灭并蓝移(至337 nm)。ABP结合D-半乳糖产生了类似的发射位移,但没有荧光猝灭。

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