Brayer G D, McPherson A
J Mol Biol. 1983 Sep 15;169(2):565-96. doi: 10.1016/s0022-2836(83)80065-5.
The three-dimensional structure of the gene 5 DNA binding protein (G5BP) from bacteriophage fd has been determined from a combination of multiple isomorphous replacement techniques, partial refinements and deleted fragment difference Fourier syntheses. The structure was refined using restrained parameter least-squares and difference Fourier methods to a final residual of R = 0.217 for the 3528 statistically significant reflections present to 2.3 A resolution. In addition to the 682 atoms of the protein, 12 solvent molecules were included. We describe here the dispositions and orientations of the amino acid side-chains and their interactions as visualized in the G5BP structure. The G5BP monomer of 87 peptide units is almost entirely in the beta-conformation, organized as a three-stranded sheet, a two-stranded beta-ribbon and a broad connecting loop. There is no alpha-helix present in the molecule. Two G5BP monomers are tightly interlocked about an intermolecular dyad axis to form a compact dimer unit of about 55 A X 45 A X 36 A. The dimer is characterized by two symmetry-related antiparallel clefts that traverse the monomer surfaces essentially perpendicular to the dyad axis. From the three-stranded antiparallel beta-sheet, formed from the first two-thirds of the sequence, extend three tyrosine residues (26, 34, 41), a lysine (46) and two arginine residues (16, 21) that, as indicated by other physical and chemical experiments, are directly involved in DNA binding. Other residues likely to share binding responsibility are arginine 80 extending from the beta-ribbon and phenylalanine 73 from the tip of this loop, but as provided, however, by the opposite monomer within each G5BP dimer pair. Thus, both symmetry-related DNA binding sites have a composite nature and include contributions from both elements of the dimer. The gene 5 dimer is clearly the active binding species, and the two monomers within the dyad-related pair are so structurally contiguous that one cannot be certain whether the isolated monomer would maintain its observed crystal structure. This linkage is manifested primarily as a skeletal core of hydrophobic residues that extends from the center of each monomer continuously through an intermolecular beta-barrel that joins the pair. Protruding from the major area of density of each monomer is an elongated wing of tenuous structure comprising residues 15 through 32, which is, we believe, intimately involved in DNA binding. This wing appears to be dynamic and mobile, even in the crystal and, therefore, is likely to undergo conformational change in the presence of the ligand.
通过多种同晶置换技术、部分精修和缺失片段差分傅里叶合成相结合的方法,确定了噬菌体fd基因5 DNA结合蛋白(G5BP)的三维结构。使用约束参数最小二乘法和差分傅里叶方法对结构进行精修,对于2.3 Å分辨率下的3528个具有统计学意义的反射,最终残余因子R = 0.217。除了蛋白质的682个原子外,还包含12个溶剂分子。我们在此描述G5BP结构中氨基酸侧链的排布和取向及其相互作用。由87个肽单元组成的G5BP单体几乎完全处于β构象,由一个三链片层、一个双链β带和一个宽连接环组成。分子中不存在α螺旋。两个G5BP单体围绕分子间二重轴紧密联锁,形成一个约55 Å×45 Å×36 Å的紧密二聚体单元。该二聚体的特征是有两个与对称相关的反平行裂缝,它们基本上垂直于二重轴穿过单体表面。由序列前三分之二形成的三链反平行β片层延伸出三个酪氨酸残基(26、34、41)、一个赖氨酸(46)和两个精氨酸残基(16、21),其他物理和化学实验表明这些残基直接参与DNA结合。其他可能分担结合作用的残基是从β带延伸出的精氨酸80和该环末端的苯丙氨酸73,但它们由每个G5BP二聚体对中的相对单体提供。因此,两个与对称相关的DNA结合位点都具有复合性质,并且包括二聚体两个元件的贡献。基因5二聚体显然是活性结合物种,二重相关对中的两个单体在结构上如此紧密相连,以至于无法确定分离的单体是否会保持其观察到的晶体结构。这种连接主要表现为疏水残基的骨架核心,它从每个单体的中心连续延伸穿过连接这一对单体的分子间β桶。从每个单体的主要密度区域突出的是一个由残基15至32组成的细长的、结构脆弱的侧翼,我们认为它与DNA结合密切相关。这个侧翼似乎是动态的且可移动的,即使在晶体中也是如此,因此在配体存在时可能会发生构象变化。
