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鲍曼不动杆菌 K20 和 K21 荚膜多糖结构确定了 UDP-葡萄糖脱氢酶 Ugd2、丙酮酸转移酶 Ptr2 和两个糖基转移酶的作用。

Acinetobacter baumannii K20 and K21 capsular polysaccharide structures establish roles for UDP-glucose dehydrogenase Ugd2, pyruvyl transferase Ptr2 and two glycosyltransferases.

机构信息

N. D. Zelinsky Institute of Organic Chemistry, Russian Academy of Sciences, 47 Leninskii prosp., Moscow, Russia.

Higher Chemical College of the Russian Academy of Sciences, D. I. Mendeleev University of Chemical Technology of Russia, 9 Miusskaya pl., Moscow, Russia.

出版信息

Glycobiology. 2018 Nov 1;28(11):876-884. doi: 10.1093/glycob/cwy074.

DOI:10.1093/glycob/cwy074
PMID:30107435
Abstract

Infections caused by Acinetobacter baumannii isolates from the major global clones, GC1 and GC2, are difficult to treat with antibiotics, and phage therapy, which requires extensive knowledge of the variation in the surface polysaccharides, is an option under consideration. The gene clusters directing the synthesis of capsular polysaccharide (CPS) in A. baumannii GC1 isolate A388 and GC2 isolate G21 differ by a single glycosyltransferase (gtr) gene. They include genes encoding a novel UDP-glucose dehydrogenase (Ugd2) and a putative pyruvyl transferase (Ptr2). The composition and structures of the linear K20 and K21 tetrasaccharide repeats (K units) of the CPSs isolated from A338 and G21, respectively, were established by sugar analyses and Smith degradation along with 1D and 2D 1H and 13C NMR spectroscopy. The K20 and K21 CPSs are the first known to include GlcpA produced by Ugd2 and d-galactose with an (R)-configured 4,6-pyruvic acid acetal added by Prt2. The first sugar in the tetrasaccharide K units is 2-acetamido-4-amino-2,4,6-trideoxy-d-glucose (d-QuipNAc4N) that carries a 4-N-[(S)-3-hydroxybutanoyl] group in some K units and a 4-N-acetyl group in the others. Accordingly, K unit polymerases WzyK20 and WzyK21 form a β-d-QuipNAc4NR-(1→2)-d-Galp bond. The K20 and K21 units differ only in the configuration of the glycosidic linkages of d-GlcpNAc allowing the unique inverting glycosyltransferases Gtr43 and the retaining glycosyltransferase Gtr45 to be assigned to the formation of the β-d-GlcpNAc-(1→4)-d-GlcpA and α-d-GlcpNAc-(1→4)-d-GlcpA linkages, respectively.

摘要

由主要全球克隆群 GC1 和 GC2 中的鲍曼不动杆菌分离株引起的感染对抗生素治疗具有抗性,而噬菌体治疗(需要广泛了解表面多糖的变化)是正在考虑的一种选择。 基因簇指导 GC1 分离株 A388 和 GC2 分离株 G21 中荚膜多糖(CPS)的合成,其差异仅在于单个糖基转移酶(gtr)基因。 它们包括编码一种新型 UDP-葡萄糖脱氢酶(Ugd2)和一种假定的丙酮酸转移酶(Ptr2)的基因。 通过糖分析和 Smith 降解以及 1D 和 2D 1H 和 13C NMR 光谱,分别从 A338 和 G21 中分离出的 CPS 的线性 K20 和 K21 四糖重复(K 单元)的组成和结构得以确定。 K20 和 K21 CPS 是已知的第一个包含由 Ugd2 产生的 GlcpA 和通过 Prt2 添加的具有(R)构型的 4,6-丙酮酸缩醛的 d-半乳糖。 在四糖 K 单元中的第一个糖是 2-乙酰氨基-4-氨基-2,4,6-三脱氧-d-葡萄糖(d-QuipNAc4N),在一些 K 单元中带有 4-N-[(S)-3-羟基丁酰基]基团,而在其他单元中带有 4-N-乙酰基。 相应地,K 单元聚合酶 WzyK20 和 WzyK21 形成β-d-QuipNAc4NR-(1→2)-d-Galp 键。 K20 和 K21 单元仅在 d-GlcpNAc 的糖苷键的构型上有所不同,这使得独特的反转糖基转移酶 Gtr43 和保留糖基转移酶 Gtr45 能够分别负责β-d-GlcpNAc-(1→4)-d-GlcpA 和α-d-GlcpNAc-(1→4)-d-GlcpA 键的形成。

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