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组装带聚糖的多萜醇磷酸酯:嗜盐栖热菌N-糖基化途径中间体的化学酶法合成

Assembling Glycan-Charged Dolichol Phosphates: Chemoenzymatic Synthesis of a Haloferax volcanii N-Glycosylation Pathway Intermediate.

作者信息

Elharar Yifat, Podilapu Ananda Rao, Guan Ziqiang, Kulkarni Suvarn S, Eichler Jerry

机构信息

Department of Life Sciences, Ben Gurion University of the Negev , Beersheva 8410501, Israel.

Department of Chemistry, Indian Institute of Technology Bombay , Powai, Mumbai 400076, India.

出版信息

Bioconjug Chem. 2017 Sep 20;28(9):2461-2470. doi: 10.1021/acs.bioconjchem.7b00436. Epub 2017 Aug 30.

DOI:10.1021/acs.bioconjchem.7b00436
PMID:28809486
Abstract

N-glycosylation, the covalent attachment of glycans to select protein target Asn residues, is a post-translational modification performed by all three domains of life. In the halophilic archaea Haloferax volcanii, in which understanding of this universal protein-processing event is relatively well-advanced, genes encoding the components of the archaeal glycosylation (Agl) pathway responsible for the assembly and attachment of an N-linked pentasaccharide have been identified. As elsewhere, the N-linked glycan is assembled on phosphodolichol carriers before transfer to target Asn residues. However, as little is presently known of the Hfx. volcanii Agl pathway at the protein level, the seemingly unique ability of Archaea to use dolichol phosphate (DolP) as the glycan lipid carrier, rather than dolichol pyrophosphate used by eukaryotes, remains poorly understood. With this in mind, a chemoenzymatic approach was taken to biochemically study AglG, one of the five glycosyltransferases of the pathway. Accordingly, a novel regio- and stereoselective reduction of naturally isolated polyprenol gave facile access to S-dolichol via asymmetric transfer hydrogenation under very mild conditions. This compound was used to generate glucose-charged DolP, a precursor of the N-linked pentasaccharide, as well as DolP-glucose-glucuronic acid and DolP-glucuronic acid. AglG, purified from Hfx. volcanii membranes in hypersaline conditions, like those encountered in situ, was subsequently combined with uridine diphosphate (UDP)-glucuronic acid and DolP-glucose to yield DolP-glucose-glucuronic acid. The in vitro system for the study of AglG activity developed here represents the first such tool for studying halophilic glycosyltransferases and will allow for a detailed understanding of archaeal N-glycosylation.

摘要

N-糖基化是聚糖与特定蛋白质靶标天冬酰胺残基的共价连接,是一种在生命的三个域中都存在的翻译后修饰。在嗜盐古菌沃氏嗜盐栖热菌中,对这种普遍的蛋白质加工过程的理解相对较为深入,负责组装和连接N-连接五糖的古菌糖基化(Agl)途径的组成成分的编码基因已被鉴定出来。与其他地方一样,N-连接聚糖在转移到靶标天冬酰胺残基之前先在磷酸多萜醇载体上组装。然而,目前对于沃氏嗜盐栖热菌Agl途径在蛋白质水平上的了解很少,古菌使用磷酸多萜醇(DolP)作为聚糖脂质载体而非真核生物使用的焦磷酸多萜醇这一看似独特的能力仍未得到充分理解。考虑到这一点,采用了一种化学酶法来对该途径的五种糖基转移酶之一AglG进行生化研究。因此,通过在非常温和的条件下进行不对称转移氢化,对天然分离的聚异戊二烯进行了新颖的区域和立体选择性还原,从而轻松获得了S-多萜醇。该化合物用于生成带葡萄糖的DolP,即N-连接五糖的前体,以及DolP-葡萄糖-葡萄糖醛酸和DolP-葡萄糖醛酸。从原位遇到的高盐条件下的沃氏嗜盐栖热菌膜中纯化得到的AglG,随后与尿苷二磷酸(UDP)-葡萄糖醛酸和DolP-葡萄糖结合,生成DolP-葡萄糖-葡萄糖醛酸。这里开发的用于研究AglG活性的体外系统是研究嗜盐糖基转移酶的首个此类工具,将有助于详细了解古菌的N-糖基化。

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