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NADP⁺和NADPH在两种小球藻病毒的GDP-D-甘露糖4,6-脱水酶活性及结构中的差异作用

Differential role of NADP+ and NADPH in the activity and structure of GDP-D-mannose 4,6-dehydratase from two chlorella viruses.

作者信息

Fruscione Floriana, Sturla Laura, Duncan Garry, Van Etten James L, Valbuzzi Paola, De Flora Antonio, Di Zanni Eleonora, Tonetti Michela

机构信息

Department of Experimental Medicine, University of Genova and Center of Excellence for Biomedical Research, Viale Benedetto XV, 1, 16132, Genova, Italy.

Department of Biology, Nebraska Wesleyan University, Lincoln, Nebraska 68504-2794.

出版信息

J Biol Chem. 2008 Jan 4;283(1):184-193. doi: 10.1074/jbc.M706614200. Epub 2007 Nov 1.

DOI:10.1074/jbc.M706614200
PMID:17974560
Abstract

GDP-D-mannose 4,6-dehydratase (GMD) is a key enzyme involved in the synthesis of 6-deoxyhexoses in prokaryotes and eukaryotes. Paramecium bursaria chlorella virus-1 (PBCV-1) encodes a functional GMD, which is unique among characterized GMDs because it also has a strong stereospecific NADPH-dependent reductase activity leading to GDP-D-rhamnose formation (Tonetti, M., Zanardi, D., Gurnon, J., Fruscione, F., Armirotti, A., Damonte, G., Sturla, L., De Flora, A., and Van Etten, J.L. (2003) J. Biol. Chem. 278, 21559-21565). In the present study we characterized a recombinant GMD encoded by another chlorella virus, Acanthocystis turfacea chlorella virus 1 (ATCV-1), demonstrating that it has the expected dehydratase activity. However, it also displayed significant differences when compared with PBCV-1 GMD. In particular, ATCV-1 GMD lacks the reductase activity present in the PBCV-1 enzyme. Using recombinant PBCV-1 and ATCV-1 GMDs, we determined that the enzymatically active proteins contain tightly bound NADPH and that NADPH is essential for maintaining the oligomerization status as well as for the stabilization and function of both enzymes. Phylogenetic analysis indicates that PBCV-1 GMD is the most evolutionary diverged of the GMDs. We conclude that this high degree of divergence was the result of the selection pressures that led to the acquisition of new reductase activity to synthesize GDP-D-rhamnose while maintaining the dehydratase activity in order to continue to synthesize GDP-L-fucose.

摘要

GDP-D-甘露糖4,6-脱水酶(GMD)是原核生物和真核生物中参与6-脱氧己糖合成的关键酶。草履虫小球藻病毒-1(PBCV-1)编码一种功能性GMD,在已鉴定的GMD中它是独特的,因为它还具有强大的立体特异性NADPH依赖性还原酶活性,可导致GDP-D-鼠李糖的形成(托内蒂,M.,扎纳尔迪,D.,古尔农,J.,弗鲁西奥内,F.,阿尔米罗蒂,A.,达蒙特,G.,斯特拉,L.,德弗洛拉,A.,以及范埃滕,J.L.(2003年)《生物化学杂志》278卷,21559 - 21565页)。在本研究中,我们对另一种小球藻病毒——棘球藻小球藻病毒1(ATCV-1)编码的重组GMD进行了表征,证明它具有预期的脱水酶活性。然而,与PBCV-1 GMD相比,它也表现出显著差异。特别是,ATCV-1 GMD缺乏PBCV-1酶中存在的还原酶活性。使用重组PBCV-1和ATCV-1 GMD,我们确定具有酶活性的蛋白质含有紧密结合的NADPH,并且NADPH对于维持两种酶的寡聚化状态以及稳定性和功能至关重要。系统发育分析表明,PBCV-1 GMD是GMD中进化分歧最大的。我们得出结论,这种高度的分歧是选择压力的结果,这些压力导致在维持脱水酶活性以继续合成GDP-L-岩藻糖的同时,获得了合成GDP-D-鼠李糖的新还原酶活性。

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