Life Science Group, Scientific Research Division, National Synchrotron Radiation Research Center, Hsinchu 30076, Taiwan.
J Biol Chem. 2010 Oct 8;285(41):31603-15. doi: 10.1074/jbc.M110.149310. Epub 2010 Aug 4.
Chitinases hydrolyze chitin, an insoluble linear polymer of N-acetyl-d-glucosamine (NAG)(n), into nutrient sources. Bacillus cereus NCTU2 chitinase (ChiNCTU2) predominantly produces chitobioses and belongs to glycoside hydrolase family 18. The crystal structure of wild-type ChiNCTU2 comprises only a catalytic domain, unlike other chitinases that are equipped with additional chitin binding and insertion domains to bind substrates into the active site. Lacking chitin binding and chitin insertion domains, ChiNCTU2 utilizes two dynamic loops (Gly-67-Thr-69 and Ile-106-Val-112) to interact with (NAG)(n), generating novel substrate binding and distortion for catalysis. Gln-109 is crucial for direct binding with substrates, leading to conformational changes of two loops with a maximum shift of ∼4.6 Å along the binding cleft. The structures of E145Q, E145Q/Y227F, and E145G/Y227F mutants complexed with (NAG)(n) reveal (NAG)(2), (NAG)(2), and (NAG)(4) in the active site, respectively, implying various stages of reaction: before hydrolysis, E145G/Y227F with (NAG)(4); in an intermediate state, E145Q/Y227F with a boat-form NAG at the -1 subsite, -1-(NAG); after hydrolysis, E145Q with a chair form -1-(NAG). Several residues were confirmed to play catalytic roles: Glu-145 in cleavage of the glycosidic bond between -1-(NAG) and +1-(NAG); Tyr-227 in the conformational change of -1-(NAG); Asp-143 and Gln-225 in stabilizing the conformation of -1-(NAG). Additionally, Glu-190 acts in the process of product release, and Tyr-193 coordinates with water for catalysis. Residues Asp-143, E145Q, Glu-190, and Tyr-193 exhibit multiple conformations for functions. The inhibitors zinc ions and cyclo-(l-His-l-Pro) are located at various positions and confirm the catalytic-site topology. Together with kinetics analyses of related mutants, the structures of ChiNCTU2 and its mutant complexes with (NAG)(n) provide new insights into its substrate binding and the mechanistic action.
几丁质酶水解几丁质,几丁质是不溶性的 N-乙酰-d-葡萄糖胺(NAG)(n)的线性聚合物,将其转化为营养源。蜡样芽胞杆菌 NCTU2 几丁质酶(ChiNCTU2)主要产生壳二糖,属于糖苷水解酶家族 18。野生型 ChiNCTU2 的晶体结构仅包含一个催化结构域,与其他配备额外几丁质结合和插入结构域以将底物结合到活性位点的几丁质酶不同。由于缺乏几丁质结合和几丁质插入结构域,ChiNCTU2 利用两个动态环(Gly-67-Thr-69 和 Ile-106-Val-112)与(NAG)(n)相互作用,产生新的底物结合和扭曲以进行催化。Gln-109 对于与底物的直接结合至关重要,导致两个环的构象发生变化,沿结合裂隙最大移动约 4.6 Å。E145Q、E145Q/Y227F 和 E145G/Y227F 突变体与(NAG)(n)的复合物结构分别揭示了活性位点中的(NAG)(2)、(NAG)(2)和(NAG)(4),这表明了不同的反应阶段:水解前,E145G/Y227F 与(NAG)(4);在中间状态下,E145Q/Y227F 与 -1 亚位点处的船形 NAG 结合,-1-(NAG);水解后,E145Q 与椅式 -1-(NAG)结合。几个残基被证实具有催化作用:Glu-145 在 -1-(NAG)和 +1-(NAG)之间糖苷键的断裂中起作用;Tyr-227 在 -1-(NAG)构象变化中的作用;Asp-143 和 Gln-225 在稳定 -1-(NAG)的构象中的作用。此外,Glu-190 在产物释放过程中起作用,Tyr-193 与水配位进行催化。残基 Asp-143、E145Q、Glu-190 和 Tyr-193 表现出多种功能构象。抑制剂锌离子和环-(l-His-l-Pro)位于不同位置,并证实了催化部位的拓扑结构。结合相关突变体的动力学分析,ChiNCTU2 及其与(NAG)(n)的突变体复合物的结构为其底物结合和机制作用提供了新的见解。
