Abbott D Wade, Macauley Matthew S, Vocadlo David J, Boraston Alisdair B
Department of Biochemistry and Microbiology, University of Victoria, Victoria, British Columbia V8W 3P6, Canada.
J Biol Chem. 2009 Apr 24;284(17):11676-89. doi: 10.1074/jbc.M809663200. Epub 2009 Jan 30.
Endo-beta-d-glucosaminidases from family 85 of glycoside hydrolases (GH85 endohexosaminidases) act to cleave the glycosidic linkage between the two N-acetylglucosamine units that make up the chitobiose core of N-glycans. Endohexosaminidase D (Endo-D), produced by Streptococcus pneumoniae, is believed to contribute to the virulence of this organism by playing a role in the deglycosylation of IgG antibodies. Endohexosaminidases have received significant attention for this reason and, moreover, because they are powerful tools for chemoenzymatic synthesis of proteins having defined glycoforms. Here we describe mechanistic and structural studies of the catalytic domain (SpGH85) of Endo-D that provide compelling support for GH85 enzymes using a catalytic mechanism involving substrate-assisted catalysis. Furthermore, the structure of SpGH85 in complex with the mechanism-based competitive inhibitor NAG-thiazoline (K(d) = 28 microm) provides a coherent rationale for previous mutagenesis studies of Endo-D and other related GH85 enzymes. We also find GH85, GH56, and GH18 enzymes have a similar configuration of catalytic residues. Notably, GH85 enzymes have an asparagine in place of the aspartate residue found in these other families of glycosidases. We propose that this residue, as the imidic acid tautomer, acts analogously to the key catalytic aspartate of GH56 and GH18 enzymes. This topographically conserved arrangement of the asparagine residue and a conserved glutamic acid, coupled with previous kinetic studies, suggests these enzymes may use an unusual proton shuttle to coordinate effective general acid and base catalysis to aid cleavage of the glycosidic bond. These results collectively provide a blueprint that may be used to facilitate protein engineering of these enzymes to improve their function as biocatalysts for synthesizing glycoproteins having defined glycoforms and also may serve as a guide for generating inhibitors of GH85 enzymes.
糖苷水解酶家族85中的内切-β-D-氨基葡萄糖苷酶(GH85内切己糖胺酶)作用于切割构成N-聚糖壳二糖核心的两个N-乙酰葡糖胺单元之间的糖苷键。肺炎链球菌产生的内切己糖胺酶D(Endo-D)被认为通过在IgG抗体的去糖基化中发挥作用而对该生物体的毒力有贡献。由于这个原因,并且此外,因为它们是用于化学酶促合成具有确定糖型的蛋白质的强大工具,内切己糖胺酶受到了极大关注。在这里,我们描述了Endo-D催化结构域(SpGH85)的机制和结构研究,这些研究为GH85酶使用涉及底物辅助催化的催化机制提供了令人信服的支持。此外,SpGH85与基于机制的竞争性抑制剂NAG-噻唑啉(K(d)=28微摩尔)的复合物结构为先前对Endo-D和其他相关GH85酶的诱变研究提供了连贯的理论依据。我们还发现GH85、GH56和GH18酶具有相似的催化残基构型。值得注意的是,GH85酶中的天冬酰胺取代了这些其他糖苷酶家族中发现的天冬氨酸残基。我们提出,这个残基作为亚氨酸互变异构体,其作用类似于GH56和GH18酶的关键催化天冬氨酸。天冬酰胺残基和保守谷氨酸的这种拓扑保守排列,再加上先前的动力学研究,表明这些酶可能使用一种不寻常的质子穿梭来协调有效的广义酸碱催化,以帮助糖苷键的裂解。这些结果共同提供了一个蓝图,可用于促进这些酶的蛋白质工程,以改善它们作为合成具有确定糖型的糖蛋白的生物催化剂的功能,并且还可作为生成GH