Wehenkel Annemarie, Bellinzoni Marco, Schaeffer Francis, Villarino Andrea, Alzari Pedro M
Unité de Biochimie Structurale and CNRS-URA 2185, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, France.
J Mol Biol. 2007 Dec 7;374(4):890-8. doi: 10.1016/j.jmb.2007.09.076. Epub 2007 Oct 2.
Phospho-Ser/Thr protein phosphatases (PPs) are dinuclear metalloenzymes classed into two large families, PPP and PPM, on the basis of sequence similarity and metal ion dependence. The archetype of the PPM family is the alpha isoform of human PP2C (PP2Calpha), which folds into an alpha/beta domain similar to those of PPP enzymes. The recent structural studies of three bacterial PPM phosphatases, Mycobacterium tuberculosis MtPstP, Mycobacterium smegmatis MspP, and Streptococcus agalactiae STP, confirmed the conservation of the overall fold and dinuclear metal center in the family, but surprisingly revealed the presence of a third conserved metal-binding site in the active site. To gain insight into the roles of the three-metal center in bacterial enzymes, we report structural and metal-binding studies of MtPstP and MspP. The structure of MtPstP in a new trigonal crystal form revealed a fully active enzyme with the canonical dinuclear metal center but without the third metal ion bound to the catalytic site. The absence of metal correlates with a partially unstructured flap segment, indicating that the third manganese ion contributes to reposition the flap, but is dispensable for catalysis. Studies of metal binding to MspP using isothermal titration calorimetry revealed that the three Mn(2+)-binding sites display distinct affinities, with dissociation constants in the nano- and micromolar range for the two catalytic metal ions and a significantly lower affinity for the third metal-binding site. In agreement, the structure of inactive MspP at acidic pH was determined at atomic resolution and shown to lack the third metal ion in the active site. Structural comparisons of all bacterial phosphatases revealed positional variations in the third metal-binding site that are correlated with the presence of bound substrate and the conformation of the flap segment, supporting a role of this metal ion in assisting enzyme-substrate interactions.
磷酸化丝氨酸/苏氨酸蛋白磷酸酶(PPs)是双核金属酶,根据序列相似性和金属离子依赖性可分为两个大家族,即PPP和PPM。PPM家族的原型是人类PP2C的α亚型(PP2Cα),其折叠成与PPP酶类似的α/β结构域。最近对三种细菌PPM磷酸酶,即结核分枝杆菌MtPstP、耻垢分枝杆菌MspP和无乳链球菌STP的结构研究,证实了该家族中整体折叠和双核金属中心的保守性,但令人惊讶地发现活性位点存在第三个保守的金属结合位点。为了深入了解三金属中心在细菌酶中的作用,我们报告了MtPstP和MspP的结构及金属结合研究。新的三角晶型的MtPstP结构显示其为具有典型双核金属中心的完全活性酶,但催化位点未结合第三个金属离子。金属的缺失与部分无结构的侧翼片段相关,表明第三个锰离子有助于侧翼的重新定位,但对催化作用并非必需。使用等温滴定量热法对MspP的金属结合研究表明,三个Mn(2+)结合位点表现出不同的亲和力,两个催化金属离子的解离常数在纳摩尔和微摩尔范围内,而对第三个金属结合位点的亲和力明显较低。与此一致,在酸性pH下无活性的MspP的结构在原子分辨率下确定,显示活性位点缺乏第三个金属离子。所有细菌磷酸酶的结构比较揭示了第三个金属结合位点的位置变化,这些变化与结合底物的存在和侧翼片段的构象相关,支持了该金属离子在辅助酶-底物相互作用中的作用。
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