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通过定点诱变和核磁共振对核糖核酸酶Barnase活性位点中磷酸盐结合的表征

Characterization of phosphate binding in the active site of barnase by site-directed mutagenesis and NMR.

作者信息

Meiering E M, Bycroft M, Fersht A R

机构信息

Cambridge IRC for Protein Engineering, University Chemical Laboratory, U.K.

出版信息

Biochemistry. 1991 Nov 26;30(47):11348-56. doi: 10.1021/bi00111a022.

Abstract

Phosphate is a competitive inhibitor of transesterification of GpC by the ribonuclease barnase. Barnase is significantly stabilized in the presence of phosphate against urea denaturation. The data are consistent with the existence of a single phosphate binding site in barnase with a dissociation constant, Kd, of 1.3 mM. The 2D 1H NMR spectrum of wild-type barnase with bound phosphate is assigned. Changes in chemical shifts and NOEs for wild type with bound phosphate compared with free wild type indicate that phosphate binds in the active site and that only small conformational changes occur on binding. Site-directed mutagenesis of the active site residues His-102, Lys-27, and Arg-87 to Ala increases the magnitude of Kd for phosphate by more than 20-fold. The 2D 1H NMR spectra of the mutants His-102----Ala, Lys-27----Ala, and Arg-87----Ala are assigned. Comparison with the spectra of wild-type barnase reveals that His-102----Ala and Lys-27----Ala have essentially the same structure as weild type, while some structural changes occur in Arg-87----Ala. It appears that phosphate binding by barnase is effected mainly by positively charge residues including His-102, Lys-27, and Arg-87. This may have applications for the design of phosphate binding sites in other proteins.

摘要

磷酸盐是核糖核酸酶巴那斯(barnase)催化GpC进行酯交换反应的竞争性抑制剂。在磷酸盐存在的情况下,巴那斯在尿素变性作用下能得到显著稳定。这些数据与巴那斯中存在一个单一的磷酸盐结合位点相一致,其解离常数Kd为1.3 mM。已对结合有磷酸盐的野生型巴那斯的二维¹H NMR谱进行了归属。与游离野生型相比,结合有磷酸盐的野生型的化学位移和核Overhauser效应(NOE)的变化表明磷酸盐结合在活性位点,且结合时仅发生了微小的构象变化。将活性位点残基组氨酸-102(His-102)、赖氨酸-27(Lys-27)和精氨酸-87(Arg-87)定点突变为丙氨酸后,磷酸盐的Kd值增大了20多倍。已对突变体His-102→Ala、Lys-27→Ala和Arg-87→Ala的二维¹H NMR谱进行了归属。与野生型巴那斯的谱图比较表明,His-102→Ala和Lys-27→Ala与野生型具有基本相同的结构,而Arg-87→Ala则发生了一些结构变化。看来巴那斯对磷酸盐的结合主要受包括His-102、Lys-27和Arg-87在内的带正电荷残基的影响。这可能在其他蛋白质中磷酸盐结合位点的设计中有应用价值。

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