Maurer Till, Meier Sebastian, Kachel Norman, Munte Claudia Elisabeth, Hasenbein Sonja, Koch Brigitte, Hengstenberg Wolfgang, Kalbitzer Hans Robert
Institut für Biophysik und Physikalische Biochemie, Universität Regensburg, Regensburg, Germany.
J Bacteriol. 2004 Sep;186(17):5906-18. doi: 10.1128/JB.186.17.5906-5918.2004.
A high-resolution structure of the histidine-containing phosphocarrier protein (HPr) from Staphylococcus aureus was obtained by heteronuclear multidimensional nuclear magnetic resonance (NMR) spectroscopy on the basis of 1,766 structural restraints. Twenty-three hydrogen bonds in HPr could be directly detected by polarization transfer from the amide nitrogen to the carbonyl carbon involved in the hydrogen bond. Differential line broadening was used to characterize the interaction of HPr with the HPr kinase/phosphorylase (HPrK/P) of Staphylococcus xylosus, which is responsible for phosphorylation-dephosphorylation of the hydroxyl group of the regulatory serine residue at position 46. The dissociation constant Kd was determined to be 0.10 +/- 0.02 mM at 303 K from the NMR data, assuming independent binding. The data are consistent with a stoichiometry of 1 HPr molecule per HPrK/P monomer in solution. Using transversal relaxation optimized spectroscopy-heteronuclear single quantum correlation, we mapped the interaction site of the two proteins in the 330-kDa complex. As expected, it covers the region around Ser46 and the small helix b following this residue. In addition, HPrK/P also binds to the second phosphorylation site of HPr at position 15. This interaction may be essential for the recognition of the phosphorylation state of His15 and the phosphorylation-dependent regulation of the kinase/phosphorylase activity. In accordance with this observation, the recently published X-ray structure of the HPr/HPrK core protein complex from Lactobacillus casei shows interactions with the two phosphorylation sites. However, the NMR data also suggest differences for the full-length protein from S. xylosus: there are no indications for an interaction with the residues preceding the regulatory Ser46 residue (Thr41 to Lys45) in the protein of S. xylosus. In contrast, it seems to interact with the C-terminal helix of HPr in solution, an interaction which is not observed for the complex of HPr with the core of HPrK/P of L. casei in crystals.
基于1766个结构约束条件,通过异核多维核磁共振(NMR)光谱法获得了金黄色葡萄球菌含组氨酸的磷酸载体蛋白(HPr)的高分辨率结构。HPr中的23个氢键可通过从酰胺氮到参与氢键的羰基碳的极化转移直接检测到。利用差分线宽来表征HPr与木糖葡萄球菌的HPr激酶/磷酸化酶(HPrK/P)的相互作用,HPrK/P负责46位调节性丝氨酸残基羟基的磷酸化-去磷酸化。根据NMR数据,在303K下,假设独立结合,解离常数Kd被确定为0.10±0.02 mM。数据与溶液中每个HPrK/P单体1个HPr分子的化学计量比一致。使用横向弛豫优化光谱-异核单量子相关,我们绘制了330 kDa复合物中两种蛋白质的相互作用位点。正如预期的那样,它覆盖了Ser46周围的区域以及该残基之后的小螺旋b。此外,HPrK/P还与HPr第15位的第二个磷酸化位点结合。这种相互作用对于识别His15的磷酸化状态和激酶/磷酸化酶活性的磷酸化依赖性调节可能至关重要。与这一观察结果一致,最近发表的干酪乳杆菌HPr/HPrK核心蛋白复合物的X射线结构显示了与两个磷酸化位点的相互作用。然而,NMR数据也表明木糖葡萄球菌全长蛋白存在差异:没有迹象表明木糖葡萄球菌蛋白中调节性Ser46残基之前的残基(Thr41至Lys45)存在相互作用。相反,它似乎在溶液中与HPr的C末端螺旋相互作用,而在晶体中HPr与干酪乳杆菌HPrK/P核心的复合物中未观察到这种相互作用。
