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人N-乙酰半乳糖胺激酶的分子结构

The molecular architecture of human N-acetylgalactosamine kinase.

作者信息

Thoden James B, Holden Hazel M

机构信息

Department of Biochemistry, University of Wisconsin, Madison, Wisconsin 53706, USA.

出版信息

J Biol Chem. 2005 Sep 23;280(38):32784-91. doi: 10.1074/jbc.M505730200. Epub 2005 Jul 8.

DOI:10.1074/jbc.M505730200
PMID:16006554
Abstract

Galactokinase plays a key role in normal galactose metabolism by catalyzing the conversion of alpha-d-galactose to galactose 1-phosphate. Within recent years, the three-dimensional structures of human galactokinase and two bacterial forms of the enzyme have been determined. Originally, the gene encoding galactokinase in humans was mapped to chromosome 17. An additional gene, encoding a protein with sequence similarity to galactokinase, was subsequently mapped to chromosome 15. Recent reports have shown that this second gene (GALK2) encodes an enzyme with greater activity against GalNAc than galactose. This enzyme, GalNAc kinase, has been implicated in a salvage pathway for the reutilization of free GalNAc derived from the degradation of complex carbohydrates. Here we report the first structural analysis of a GalNAc kinase. The structure of the human enzyme was solved in the presence of MnAMPPNP and GalNAc or MgATP and GalNAc (which resulted in bound products in the active site). The enzyme displays a distinctly bilobal appearance with its active site wedged between the two domains. The N-terminal region is dominated by a seven-stranded mixed beta-sheet, whereas the C-terminal motif contains two layers of anti-parallel beta-sheet. The overall topology displayed by GalNAc kinase places it into the GHMP superfamily of enzymes, which generally function as small molecule kinases. From this investigation, the geometry of the GalNAc kinase active site before and after catalysis has been revealed, and the determinants of substrate specificity have been defined on a molecular level.

摘要

半乳糖激酶通过催化α - d - 半乳糖转化为1 - 磷酸半乳糖,在正常半乳糖代谢中起关键作用。近年来,已确定了人半乳糖激酶和该酶的两种细菌形式的三维结构。最初,人类中编码半乳糖激酶的基因被定位到17号染色体。随后,另一个编码与半乳糖激酶序列相似的蛋白质的基因被定位到15号染色体。最近的报道表明,这第二个基因(GALK2)编码的一种酶对N - 乙酰半乳糖胺(GalNAc)的活性比对半乳糖的活性更高。这种酶,即GalNAc激酶,参与了一条用于重新利用从复合碳水化合物降解中产生的游离GalNAc的补救途径。在此,我们报道了GalNAc激酶的首次结构分析。在存在锰 - AMPPNP和GalNAc或镁 - ATP和GalNAc的情况下(这导致活性位点结合产物)解析了人源该酶的结构。该酶呈现出明显的双叶外观,其活性位点楔入两个结构域之间。N端区域以一个七链混合β - 折叠为主,而C端基序包含两层反平行β - 折叠。GalNAc激酶展示的整体拓扑结构使其属于GHMP酶超家族,该超家族通常作为小分子激酶发挥作用。通过这项研究,揭示了GalNAc激酶催化前后活性位点的几何结构,并在分子水平上确定了底物特异性的决定因素。

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