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法氏克氏锥虫中GDP-D-阿拉伯吡喃糖的生物合成:D-阿拉伯糖-1-激酶活性的表征及其在GDP-[5-³H]D-阿拉伯吡喃糖合成中的应用。

The biosynthesis of GDP-D-arabinopyranose in Crithidia fasciculata: characterization of a D-arabino-1-kinase activity and its use in the synthesis of GDP-[5-3H]D-arabinopyranose.

作者信息

Schneider P, Nikolaev A, Ferguson M A

机构信息

Department of Biochemistry, University of Dundee, UK.

出版信息

Biochem J. 1995 Oct 1;311 ( Pt 1)(Pt 1):307-15. doi: 10.1042/bj3110307.

Abstract

GDP-D-arabinopyranose (GDP-D-Ara) is the precursor of the uncommon D-arabinopyranose residues present in the glycoconjugates of a few trypanosomatid parasites. Biosynthetic labelling experiments with Crithidia fasciculata showed that GDP-D-Ara could be labelled with [3H]D-Ara, [2-3H]D-Glc and [6-3H]D-Glc, but not with [1-3H]D-Glc, suggesting that D-Ara can be either taken up directly by the parasite or derived from D-Glc through a pathway involving the loss of carbon C-1. In vivo pulse-chase experiments indicated that D-Ara was sequentially incorporated into D-Ara-1-PO4 and GDP-D-Ara prior to transfer to the acceptor glycoconjugate, lipoarabinogalactan. An MgATP-dependent D-arabino-1-kinase activity present in soluble extracts of C. fasciculata was purified away from phosphatase activities by size-exclusion chromatography. The D-arabino-1-kinase had an apparent molecular mass of 600 kDa, a neutral optimum pH, and displayed substrate inhibition at D-Ara concentrations above 100 microM. It had a KmATP of 1.7 mM and a KmAra of 24 microM. Competition studies indicated that the orientation of every single hydroxyl residue was important for D-Ara recognition by the enzyme, but that methyl or hydroxymethyl groups could be tolerated as equatorial substituents on C-5 of D-Ara. The partially purified D-arabino-1-kinase activity was used in the chemico-enzymic synthesis of GDP-[5-3H]D-Ara from [6-3H]D-GlcN.

摘要

GDP-D-阿拉伯吡喃糖(GDP-D-Ara)是少数锥虫寄生虫糖缀合物中存在的罕见D-阿拉伯吡喃糖残基的前体。用纤细短膜虫进行的生物合成标记实验表明,GDP-D-Ara可以用[3H]D-Ara、[2-3H]D-Glc和[6-3H]D-Glc进行标记,但不能用[1-3H]D-Glc进行标记,这表明D-Ara可以被寄生虫直接摄取,或者通过涉及C-1碳损失的途径从D-Glc衍生而来。体内脉冲追踪实验表明,D-Ara在转移到受体糖缀合物脂阿拉伯半乳聚糖之前,先依次掺入D-Ara-1-PO4和GDP-D-Ara中。通过尺寸排阻色谱法从磷酸酶活性中纯化出纤细短膜虫可溶性提取物中存在的MgATP依赖性D-阿拉伯糖-1-激酶活性。D-阿拉伯糖-1-激酶的表观分子量为600 kDa,最适pH为中性,在D-Ara浓度高于100 microM时表现出底物抑制作用。它的KmATP为1.7 mM,KmAra为24 microM。竞争研究表明,每个羟基残基的取向对于酶识别D-Ara很重要,但甲基或羟甲基基团作为D-Ara C-5上的赤道取代基是可以耐受的。部分纯化的D-阿拉伯糖-1-激酶活性用于从[6-3H]D-GlcN化学酶促合成GDP-[5-3H]D-Ara。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d244/1136153/6ab90d63a30d/biochemj00054-0302-a.jpg

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