5CQM
GTB mutant with mercury - E303C
5CQM の概要
エントリーDOI | 10.2210/pdb5cqm/pdb |
関連するPDBエントリー | 5CMF 5CMG 5CMH 5CMI 5CMJ 5CQL 5CQN 5CQO 5CQP |
分子名称 | Histo-blood group ABO system transferase, MERCURY (II) ION (3 entities in total) |
機能のキーワード | human abo(h) blood group system, glycosyltransferase, double turn motif, catalytic domain, transferase |
由来する生物種 | Homo sapiens (Human) |
細胞内の位置 | Golgi apparatus, Golgi stack membrane; Single-pass type II membrane protein: P16442 |
タンパク質・核酸の鎖数 | 1 |
化学式量合計 | 35391.65 |
構造登録者 | |
主引用文献 | Blackler, R.J.,Gagnon, S.M.,Polakowski, R.,Rose, N.L.,Zheng, R.B.,Letts, J.A.,Johal, A.R.,Schuman, B.,Borisova, S.N.,Palcic, M.M.,Evans, S.V. Glycosyltransfer in mutants of putative catalytic residue Glu303 of the human ABO(H) A and B blood group glycosyltransferases GTA and GTB proceeds through a labile active site. Glycobiology, 27:370-380, 2017 Cited by PubMed Abstract: The homologous glycosyltransferases α-1,3-N-acetylgalactosaminyltransferase (GTA) and α-1,3-galactosyltransferase (GTB) carry out the final synthetic step of the closely related human ABO(H) blood group A and B antigens. The catalytic mechanism of these model retaining enzymes remains under debate, where Glu303 has been suggested to act as a putative nucleophile in a double displacement mechanism, a local dipole stabilizing the intermediate in an orthogonal associative mechanism or a general base to stabilize the reactive oxocarbenium ion-like intermediate in an SNi-like mechanism. Kinetic analysis of GTA and GTB point mutants E303C, E303D, E303Q and E303A shows that despite the enzymes having nearly identical sequences, the corresponding mutants of GTA/GTB have up to a 13-fold difference in their residual activities relative to wild type. High-resolution single crystal X-ray diffraction studies reveal, surprisingly, that the mutated Cys, Asp and Gln functional groups are no more than 0.8 Å further from the anomeric carbon of donor substrate compared to wild type. However, complicating the analysis is the observation that Glu303 itself plays a critical role in maintaining the stability of a strained "double-turn" in the active site through several hydrogen bonds, and any mutation other than E303Q leads to significantly higher thermal motion or even disorder in the substrate recognition pockets. Thus, there is a remarkable juxtaposition of the mutants E303C and E303D, which retain significant activity despite disrupted active site architecture, with GTB/E303Q, which maintains active site architecture but exhibits zero activity. These findings indicate that nucleophilicity at position 303 is more catalytically valuable than active site stability and highlight the mechanistic elasticity of these enzymes. PubMed: 27979997DOI: 10.1093/glycob/cww117 主引用文献が同じPDBエントリー |
実験手法 | X-RAY DIFFRACTION (1.65 Å) |
構造検証レポート
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