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磷酸烯醇丙酮酸依赖性磷酸转移酶系统。对化学修饰的HPr蛋白的1H核磁共振研究。

Phosphoenolpyruvate-dependent phosphotransferase system. 1H NMR studies on chemically modified HPr proteins.

作者信息

Kalbitzer H R, Muss H P, Engelmann R, Kiltz H H, Stüber K, Hengstenberg W

出版信息

Biochemistry. 1985 Aug 13;24(17):4562-9. doi: 10.1021/bi00338a012.

Abstract

The low-pK tyrosyl residue present in the heat-stable proteins (HPr) of all Gram-positive bacteria studied until now has been labeled by tetranitromethane in the HPr of Bacillus subtilis and Streptococcus faecalis. The nitrotyrosyl derivatives obtained are fully active in the complementation assay. The labeled tyrosyl residues could be identified as Tyr-37 in both proteins. Reinvestigation of the low-pK tyrosyl residue in HPr of Staphylococcus aureus resulted in the same assignment. In all three proteins an interaction between nitrotyrosine-37 and the active center His-15 could be observed, leading to an increase in the pK of His-15 and a change of its chemical shift parameters. The 1H NMR lines of the complete aromatic spin system of HPr of B. subtilis could be assigned by the nitration studies. Labeling of Arg-17 in HPr of S. aureus and S. faecalis by 1,2-cyclohexanedione in the presence of borate ions causes an almost complete inhibition of its enzymatic activity. In the NMR spectrum the labeling of the arginyl residue influences the resonance lines of His-15: two new resonance lines for the C-2 protons of equal intensity are observed, a fact that could be explained by two different conformations in slow exchange. The pK value of His-15 was not changed by the labeling, excluding Arg-17 as responsible for the low pK of His-15.

摘要

迄今为止,在所有已研究的革兰氏阳性菌的热稳定蛋白(HPr)中存在的低pK值酪氨酰残基,已在枯草芽孢杆菌和粪肠球菌的HPr中被四硝基甲烷标记。所得到的硝基酪氨酰衍生物在互补分析中具有完全活性。在这两种蛋白质中,标记的酪氨酰残基均可被鉴定为Tyr-37。对金黄色葡萄球菌HPr中低pK值酪氨酰残基的重新研究得到了相同的结果。在所有这三种蛋白质中,均可观察到硝基酪氨酸-37与活性中心His-15之间的相互作用,导致His-15的pK值升高及其化学位移参数发生变化。通过硝化研究可对枯草芽孢杆菌HPr完整芳香族自旋系统的1H NMR谱线进行归属。在硼酸根离子存在的情况下,用1,2-环己二酮对金黄色葡萄球菌和粪肠球菌HPr中的Arg-17进行标记,几乎完全抑制了其酶活性。在NMR谱中,精氨酰残基的标记影响His-15的共振线:观察到两条强度相等的C-2质子的新共振线,这一事实可用两种不同构象的缓慢交换来解释。His-15的pK值并未因标记而改变,排除了Arg-17是His-15低pK值的原因。

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