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线虫中的 UDP-半乳糖吡喃糖变位酶。

UDP-galactopyranose mutase in nematodes.

机构信息

Department of Biochemistry, University of Wisconsin-Madison, United States.

出版信息

Biochemistry. 2013 Jun 25;52(25):4391-8. doi: 10.1021/bi400264d. Epub 2013 Jun 11.

Abstract

Nematodes represent a diverse phylum of both free living and parasitic species. While the species Caenorhabditis elegans is a valuable model organism, parasitic nematodes or helminths pose a serious threat to human health. Indeed, helminths cause many neglected tropical diseases that afflict humans. Nematode glycoconjugates have been implicated in evasive immunomodulation, a hallmark of nematode infections. One monosaccharide residue present in the glycoconjugates of several human pathogens is galactofuranose (Galf). This five-membered ring isomer of galactose has not been detected in mammals, making Galf metabolic enzymes attractive therapeutic targets. The only known pathway for biosynthetic incorporation of Galf into glycoconjugates depends upon generation of the glycosyl donor UDP-Galf by the flavoenzyme uridine 5'-diphosphate (UDP) galactopyranose mutase (UGM or Glf). A putative UGM encoding gene (glf-1) was recently identified in C. elegans. We sought to assess the catalytic activity of the corresponding gene product (CeUGM). CeUGM catalyzes the isomerization of UDP-Galf and UDP-galactopyranose (UDP-Galp). In the presence of enzyme, substrate, and a hydride source, a galactose-N5-FAD adduct was isolated, suggesting the CeUGM flavin adenine dinucleotide (FAD) cofactor serves as a nucleophile in covalent catalysis. Homology modeling and protein variants indicate that CeUGM possesses an active site similar to that of prokaryotic enzymes, despite the low sequence identity (∼15%) between eukaryotic and prokaryotic UGM proteins. Even with the primary sequence differences, heterocyclic UGM inhibitors developed against prokaryotic proteins also inhibit CeUGM activity. We postulate that inhibitors of CeUGM can serve as chemical probes of Galf in nematodes and as anthelmintic leads. The available data suggest that CeUGM facilitates the biosynthetic incorporation of Galf into nematode glycoconjugates through generation of the glycosyl donor UDP-Galf.

摘要

线虫是自由生活和寄生物种的多样化门。虽然秀丽隐杆线虫是一种有价值的模式生物,但寄生线虫或蠕虫对人类健康构成严重威胁。事实上,蠕虫会导致许多影响人类的被忽视的热带病。线虫糖缀合物已被牵连到逃避免疫调节中,这是线虫感染的一个标志。在几种人类病原体的糖缀合物中存在一个单糖残基是半乳糖呋喃糖(Galf)。这种半乳糖的五员环异构体在哺乳动物中未被检测到,使得 Galf 代谢酶成为有吸引力的治疗靶点。将 Galf 生物合成掺入糖缀合物的唯一已知途径依赖于黄素酶尿苷 5'-二磷酸(UDP)半乳糖吡喃糖基转移酶(UGM 或 Glf)生成糖基供体 UDP-Galf。最近在秀丽隐杆线虫中鉴定出一个假定的 UGM 编码基因(glf-1)。我们试图评估相应基因产物(CeUGM)的催化活性。CeUGM 催化 UDP-Galf 和 UDP-半乳糖(UDP-Galp)的异构化。在酶、底物和氢供体存在的情况下,分离出半乳糖-N5-FAD 加合物,表明 CeUGM 黄素腺嘌呤二核苷酸(FAD)辅因子在共价催化中充当亲核试剂。同源建模和蛋白质变体表明,尽管真核生物和原核生物 UGM 蛋白之间的序列同一性(约 15%)较低,但 CeUGM 具有类似于原核酶的活性位点。即使存在主要序列差异,针对原核蛋白开发的杂环 UGM 抑制剂也抑制 CeUGM 活性。我们假设 CeUGM 的抑制剂可以作为线虫中 Galf 的化学探针,并作为驱虫先导化合物。现有数据表明,CeUGM 通过生成糖基供体 UDP-Galf 促进 Galf 掺入线虫糖缀合物的生物合成。

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