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来自拟杆菌属细菌的GH99糖苷水解酶的内切-α-1,2-甘露聚糖酶活性的结构与动力学剖析

Structural and kinetic dissection of the endo-α-1,2-mannanase activity of bacterial GH99 glycoside hydrolases from Bacteroides spp.

作者信息

Hakki Zalihe, Thompson Andrew J, Bellmaine Stephanie, Speciale Gaetano, Davies Gideon J, Williams Spencer J

机构信息

School of Chemistry and Bio21 Molecular Science and Biotechnology Institute, University of Melbourne, Parkville, Victoria 3010 (Australia).

出版信息

Chemistry. 2015 Jan 26;21(5):1966-77. doi: 10.1002/chem.201405539. Epub 2014 Dec 8.

DOI:10.1002/chem.201405539
PMID:25487964
Abstract

Glycoside hydrolase family 99 (GH99) was created to categorize sequence-related glycosidases possessing endo-α-mannosidase activity: the cleavage of mannosidic linkages within eukaryotic N-glycan precursors (Glc1-3 Man9 GlcNAc2 ), releasing mono-, di- and triglucosylated-mannose (Glc1-3 -1,3-Man). GH99 family members have recently been implicated in the ability of Bacteroides spp., present within the gut microbiota, to metabolize fungal cell wall α-mannans, releasing α-1,3-mannobiose by hydrolysing αMan-1,3-αMan→1,2-αMan-1,2-αMan sequences within branches off the main α-1,6-mannan backbone. We report the development of a series of substrates and inhibitors, which we use to kinetically and structurally characterise this novel endo-α-1,2-mannanase activity of bacterial GH99 enzymes from Bacteroides thetaiotaomicron and xylanisolvens. These data reveal an approximate 5 kJ mol(-1) preference for mannose-configured substrates in the -2 subsite (relative to glucose), which inspired the development of a new inhibitor, α-mannopyranosyl-1,3-isofagomine (ManIFG), the most potent (bacterial) GH99 inhibitor reported to date. X-ray structures of ManIFG or a substrate in complex with wild-type or inactive mutants, respectively, of B. xylanisolvens GH99 reveal the structural basis for binding to D-mannose- rather than D-glucose-configured substrates.

摘要

糖苷水解酶家族99(GH99)用于对具有内切α-甘露糖苷酶活性的序列相关糖苷酶进行分类:即真核生物N-聚糖前体(Glc1-3 Man9 GlcNAc2)中甘露糖苷键的裂解,释放单糖、二糖和三糖基化的甘露糖(Glc1-3 -1,3-Man)。最近发现,肠道微生物群中的拟杆菌属具有代谢真菌细胞壁α-甘露聚糖的能力,通过水解主α-1,6-甘露聚糖主链分支中的αMan-1,3-αMan→1,2-αMan-1,2-αMan序列释放α-1,3-甘露二糖。我们报道了一系列底物和抑制剂的开发,用于对来自多形拟杆菌和木聚糖分离拟杆菌的细菌GH99酶的这种新型内切α-1,2-甘露聚糖酶活性进行动力学和结构表征。这些数据揭示了在-2亚位点(相对于葡萄糖)中对甘露糖构型底物的约5 kJ mol(-1)偏好,这促使开发了一种新的抑制剂,α-甘露吡喃糖基-1,3-异法戈明(ManIFG),这是迄今为止报道的最有效的(细菌)GH99抑制剂。木聚糖分离拟杆菌GH99的野生型或无活性突变体分别与ManIFG或底物形成的X射线结构揭示了与D-甘露糖而非D-葡萄糖构型底物结合的结构基础。

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