Scapin G, Reddy S G, Blanchard J S
Department of Biochemistry, Albert Einstein College of Medicine, Bronx, New York 10461, USA.
Biochemistry. 1996 Oct 22;35(42):13540-51. doi: 10.1021/bi961628i.
Diaminopimelate dehydrogenase catalyzes the NADPH-dependent reduction of ammonia and L-2-amino-6-ketopimelate to form meso-diaminopimelate, the direct precursor of L-lysine in the bacterial lysine biosynthetic pathway. Since mammals lack this metabolic pathway inhibitors of enzymes in this pathway may be useful as antibiotics or herbicides. Diaminopimelate dehydrogenase catalyzes the only oxidative deamination of an amino acid of D configuration and must additionally distinguish between two chiral amino acid centers on the same symmetric substrate. The Corynebacterium glutamicum enzyme has been cloned, expressed in Escherichia coli, and purified to homogeneity using standard biochemical procedures [Reddy, S. G., Scapin, G., & Blanchard, J. S. (1996) Proteins: Structure, Funct. Genet. 25, 514-516]. The three-dimensional structure of the binary complex of diaminopimelate dehydrogenase with NADP+ has been solved using multiple isomorphous replacement procedures and noncrystallographic symmetry averaging. The resulting model has been refined against 2.2 A diffraction data to a conventional crystallographic R-factor of 17.0%. Diaminopimelate dehydrogenase is a homodimer of structurally not identical subunits. Each subunit is composed of three domains. The N-terminal domain contains a modified dinucleotide binding domain, or Rossman fold (six central beta-strands in a 213456 topology surrounded by five alpha-helices). The second domain contains two alpha-helices and three beta-strands. This domain is referred to as the dimerization domain, since it is involved in forming the monomer--monomer interface of the dimer. The third or C-terminal domain is composed of six beta-strands and five alpha-helices. The relative position of the N- and C-terminal domain in the two monomers is different, defining an open and a closed conformation that may represent the enzyme's binding and active state, respectively. In both monomers the nucleotide is bound in an extended conformation across the C-terminal portion of the beta-sheet of the Rossman fold, with its C4 facing the C-terminal domain. In the closed conformer two molecules of acetate have been refined in this region, and we postulate that they define the DAP binding site. The structure of diaminopimelate dehydrogenase shows interesting similarities to the structure of glutamate dehydrogenase [Baker, P. J., Britton, K. L., Rice, D. W., Rob, A., & Stillmann, T.J. (1992a) J. Mol. Biol. 228, 662-671] and leucine dehydrogenase [Baker, P.J., Turnbull, A.P., Sedelnikova, S.E., Stillman, T. J., & Rice, D. W. (1995) Structure 3, 693-705] and also resembles the structure of dihydrodipicolinate reductase [Scapin, G., Blanchard, J. S., & Sacchettini, J. C. (1995) Biochemistry 34, 3502-3512], the enzyme immediately preceding it in the diaminopimelic acid/lysine biosynthetic pathway.
二氨基庚二酸脱氢酶催化NADPH依赖的氨和L-2-氨基-6-酮基庚二酸还原反应,生成内消旋二氨基庚二酸,它是细菌赖氨酸生物合成途径中L-赖氨酸的直接前体。由于哺乳动物缺乏这种代谢途径,该途径中酶的抑制剂可能可用作抗生素或除草剂。二氨基庚二酸脱氢酶催化唯一的D构型氨基酸的氧化脱氨基反应,并且必须另外区分同一对称底物上的两个手性氨基酸中心。谷氨酸棒杆菌的这种酶已被克隆,在大肠杆菌中表达,并使用标准生化程序纯化至同质[雷迪,S.G.,斯卡平,G.,& 布兰查德,J.S.(1996年)《蛋白质:结构、功能、遗传学》25,514 - 516]。二氨基庚二酸脱氢酶与NADP⁺二元复合物的三维结构已通过多重同晶置换程序和非晶体学对称性平均法解析。所得模型已根据2.2埃的衍射数据进行精修,传统晶体学R因子为17.0%。二氨基庚二酸脱氢酶是由结构不相同的亚基组成的同型二聚体。每个亚基由三个结构域组成。N端结构域包含一个修饰的二核苷酸结合结构域,即罗斯曼折叠(六个中心β链呈213456拓扑结构,被五个α螺旋包围)。第二个结构域包含两个α螺旋和三个β链。该结构域被称为二聚化结构域,因为它参与形成二聚体的单体 - 单体界面。第三个或C端结构域由六个β链和五个α螺旋组成。两个单体中N端和C端结构域的相对位置不同,定义了一种开放构象和一种封闭构象,它们可能分别代表酶的结合状态和活性状态。在两个单体中,核苷酸以延伸构象结合在罗斯曼折叠β片层的C端部分,其C4面向C端结构域。在封闭构象中,该区域已精修出两个乙酸分子,我们推测它们定义了DAP结合位点。二氨基庚二酸脱氢酶的结构与谷氨酸脱氢酶[贝克,P.J.,布里顿,K.L.,赖斯,D.W.,罗布 A.,& 斯蒂尔曼,T.J.(199
