Weber D J, Gittis A G, Mullen G P, Abeygunawardana C, Lattman E E, Mildvan A S
Department of Biological Chemistry, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205.
Proteins. 1992 Aug;13(4):275-87. doi: 10.1002/prot.340130402.
The conformation of the staphylococcal nuclease-bound metal-dTdA complex, previously determined by NMR methods [Weber, D.J., Mullen, G.P., Mildvan, A.S. (1991) Biochemistry 30:7425-7437] was docked into the X-ray structure of the enzyme-Ca(2+)-3',5'-pdTp complex [Loll, P.J., Lattman, E.E. (1989) Proteins: Struct., Funct., Genet. 5:183-201] by superimposing the metal ions, taking into account intermolecular nuclear Overhauser effects from assigned aromatic proton resonances of Tyr-85, Tyr-113, and Tyr-115 to proton resonances of the leaving dA moiety of dTdA, and energy minimization to relieve small overlaps. The proton resonances of the Phe, Tyr, and Trp residues of the enzyme in the ternary enzyme-La(3+)-dTdA complex were sequence specifically assigned by 2D phase-sensitive NOESY, with and without deuteration of the aromatic protons of the Tyr residues, and by 2D heteronuclear multiple quantum correlation (HMQC) spectroscopy and 3D NOESY-HMQC spectroscopy with 15N labeling. While resonances of most Phe, Tyr and Trp residues were unshifted by the substrate dTdA from those found in the enzyme-La(3+)-3',5'-pdTp complex and the enzyme-Ca(2+)-3',5'-pdTp complex, proton resonances of Tyr-85, Tyr-113, Tyr-115, and Phe-34 were shifted by 0.08 to 0.33 ppm and the 15N resonance of Tyr-113 was shifted by 2.1 ppm by the presence of substrate. The optimized position of enzyme-bound dTdA shows the 5'-dA leaving group to partially overlap the inhibitor, 3',5'-pdTp (in the X-ray structure). The 3'-TMP moiety of dTdA points toward the solvent in a channel defined by Ile-18, Asp-19, Thr-22, Lys-45, and His-46. The phosphate of dTdA is coordinated by the metal, and an adjacent inner sphere water ligand is positioned to donate a hydrogen bond to the general base Glu-43 and to attack the phosphorus with inversion. Arg-35 and Arg-87 donate monodentate hydrogen bonds to different phosphate oxygens of dTdA, with Arg-87 positioned to protonate the leaving 5'-oxygen of dA, thus clarifying the mechanism of hydrolysis. Model building of an additional 5'-dGMP onto the 3'-oxygen of dA placed this third nucleotide onto a surface cleft near residues Glu-80, Asp-83, Lys-84, and Tyr-115 with its 3'-OH group accessible to the solvent, thus defining the size of the substrate binding site as accommodating a trinucleotide.
先前通过核磁共振方法[Weber, D.J., Mullen, G.P., Mildvan, A.S. (1991) Biochemistry 30:7425 - 7437]确定的葡萄球菌核酸酶结合金属 - dTdA复合物的构象,通过叠加金属离子,考虑来自Tyr - 85、Tyr - 113和Tyr - 115指定芳香族质子共振到dTdA离去dA部分质子共振的分子间核Overhauser效应,并进行能量最小化以消除小的重叠,被对接至酶 - Ca(2+) - 3',5'-pdTp复合物的X射线结构[Loll, P.J., Lattman, E.E. (1989) Proteins: Struct., Funct., Genet. 5:183 - 201]中。通过二维相敏NOESY,在有和没有Tyr残基芳香族质子氘代的情况下,以及通过二维异核多量子相关(HMQC)光谱和15N标记的三维NOESY - HMQC光谱,对三元酶 - La(3+) - dTdA复合物中酶的Phe、Tyr和Trp残基的质子共振进行了序列特异性归属。虽然大多数Phe、Tyr和Trp残基的共振与在酶 - La(3+) - 3',5'-pdTp复合物和酶 - Ca(2+) - 3',5'-pdTp复合物中发现的相比,未因底物dTdA而发生位移,但Tyr - 85、Tyr - 113、Tyr - 115和Phe - 34的质子共振因底物的存在而位移了0.08至0.33 ppm,且Tyr - 113的15N共振位移了2.1 ppm。酶结合dTdA的优化位置显示5'-dA离去基团与抑制剂3',5'-pdTp(在X射线结构中)部分重叠。dTdA的3'-TMP部分在由Ile - 18、Asp - 19、Thr - 22、Lys - 45和His - 46定义的通道中指向溶剂。dTdA的磷酸基团由金属配位,并且一个相邻的内球水配体被定位成向通用碱Glu - 43提供氢键并以反转方式攻击磷。Arg - 35和Arg - 87向dTdA的不同磷酸氧原子提供单齿氢键,Arg - 87被定位成使dA的离去5'-氧质子化,从而阐明了水解机制。在dA的3'-氧上额外构建一个5'-dGMP的模型构建将这个第三个核苷酸放置在靠近Glu - 80、Asp - 83、Lys - 84和Tyr - 115残基的表面裂隙上,其3'-OH基团可接触溶剂,从而将底物结合位点的大小定义为可容纳一个三核苷酸。
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