Sowadski J M, Handschumacher M D, Murthy H M, Foster B A, Wyckoff H W
J Mol Biol. 1985 Nov 20;186(2):417-33. doi: 10.1016/0022-2836(85)90115-9.
The structure of alkaline phosphatase from Escherichia coli has been determined to 2.8 A resolution. The multiple isomorphous replacement electron density map of the dimer at 3.4 A was substantially improved by molecular symmetry averaging and solvent flattening. From these maps, polypeptide chains of the dimer were built using the published amino acid sequence. Stereochemically restrained least-squares refinement of this model against native data, starting with 3.4 A data and extending in steps to 2.8 A resolution, proceeded to a final overall crystallographic R factor of 0.256. Alkaline phosphatase-phosphomonoester hydrolase (EC 3.1.3.1) is a metalloenzyme that forms an isologous dimer with two reactive centers 32 A apart. The topology of the polypeptide fold of the subunit is of the alpha/beta class of proteins. Despite the similarities in the overall alpha/beta fold with other proteins, alkaline phosphatase does not have a characteristic binding cleft formed at the carboxyl end of the parallel sheet, but rather an active pocket that contains a cluster of three functional metal sites located off the plane of the central ten-stranded sheet. This active pocket is located near the carboxyl ends of four strands and the amino end of the antiparallel strand, between the plane of the sheet and two helices on the same side. Alkaline phosphatase is a non-specific phosphomonoesterase that hydrolyzes small phosphomonoesters as well as the phosphate termini of DNA. The accessibility calculations based on the refined co-ordinates of the enzyme show that the active pocket barely accommodates inorganic phosphate. Thus, the alcoholic or phenolic portion of the substrate would have to be exposed on the surface of the enzyme. Two metal sites, M1 and M2, 3.9 A apart, are occupied by zinc. The third site, M3, 5 A from site M2 and 7 A from site M1, is occupied by magnesium or, in the absence of magnesium, by zinc. As with other zinc-containing enzymes, histidine residues are ligands to zinc site M1 (three) and to zinc site M2 (one). Ligand assignment and metal preference indicate that the crystallographically found metal sites M1, M2 and M3 correspond to the spectroscopically deduced metal sites A, B and C, respectively. Arsenate, a product analog and enzyme inhibitor, binds between Ser102 and zinc sites M1 and M2. The position of the guanidinium group of Arg 166 is within hydrogen-bonding distance from the arsenate site.(ABSTRACT TRUNCATED AT 400 WORDS)
已将大肠杆菌碱性磷酸酶的结构解析到2.8埃的分辨率。通过分子对称性平均和溶剂扁平化,二聚体在3.4埃时的多同晶置换电子密度图得到了显著改善。根据已发表的氨基酸序列,利用这些图谱构建了二聚体的多肽链。以3.4埃的数据开始,逐步扩展到2.8埃分辨率,对该模型进行立体化学约束最小二乘精修,最终整体晶体学R因子达到0.256。碱性磷酸酶 - 磷酸单酯水解酶(EC 3.1.3.1)是一种金属酶,形成一个同源二聚体,两个活性中心相距32埃。亚基的多肽折叠拓扑结构属于α/β类蛋白质。尽管与其他蛋白质在整体α/β折叠上有相似之处,但碱性磷酸酶在平行片层的羧基末端没有形成特征性的结合裂隙,而是有一个活性口袋,其中包含位于中央十条链片层平面之外的三个功能性金属位点簇。这个活性口袋位于四条链的羧基末端和反平行链的氨基末端附近,在片层平面和同一侧的两个螺旋之间。碱性磷酸酶是一种非特异性磷酸单酯酶,能水解小的磷酸单酯以及DNA的磷酸末端。基于酶的精修坐标进行的可及性计算表明,活性口袋几乎无法容纳无机磷酸。因此,底物的醇或酚部分必须暴露在酶的表面。两个相距3.9埃的金属位点M1和M2被锌占据。第三个位点M3,距离位点M2 5埃,距离位点M1 7埃,被镁占据,或者在没有镁的情况下被锌占据。与其他含锌酶一样,组氨酸残基是锌位点M1(三个)和锌位点M2(一个)的配体。配体归属和金属偏好表明,晶体学上发现的金属位点M1、M2和M3分别对应于光谱推断的金属位点A、B和C。砷酸盐是一种产物类似物和酶抑制剂,结合在Ser102与锌位点M1和M2之间。Arg 166的胍基位置与砷酸盐位点的距离在氢键作用范围内。(摘要截断于400字)
