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磷酸甘露糖异构酶的硒代蛋氨酸标记改变了其动力学性质。

Selenomethionine labelling of phosphomannose isomerase changes its kinetic properties.

作者信息

Bernard A R, Wells T N, Cleasby A, Borlat F, Payton M A, Proudfoot A E

机构信息

Glaxo Institute for Molecular Biology, Geneva, Switzerland.

出版信息

Eur J Biochem. 1995 May 15;230(1):111-8. doi: 10.1111/j.1432-1033.1995.0111i.x.

DOI:10.1111/j.1432-1033.1995.0111i.x
PMID:7601089
Abstract

Phosphomannose isomerase (PMI) is an essential enzyme in the early steps of the protein glycosylation pathway in both prokaryotes and eukaryotes. Lack of the enzyme is lethal for fungal organisms and it is thus a potential fungicidal target. To facilitate the solution of the three-dimensional structure of the enzyme from the pathogen Candida albicans, we have produced the recombinant selenomethionine-labelled enzyme (SeMet-PMI). DL41, a methionine auxotroph Escherichia coli strain, was transformed with a PMI expression plasmid and grown on an enriched selenomethionine-containing medium to high-cell densities. The SeMet-PMI protein has been purified and found by amino acid analysis to have its methionine residues replaced by selenomethionine residues. Electrospray mass spectroscopy showed a major species of 49,063 +/- 10 Da for SeMet-PMI compared to 48,735 +/- 6 Da for the normal recombinant enzyme, accounting for the incorporation of seven selenomethionine residues. SeMet-PMI crystallised isomorphously with the normal PMI protein and the crystals diffract to 0.23 nm. Kinetic characterisation of SeMet-PMI showed that its Km for the substrate mannose-6-phosphate was fourfold higher than that of its methionine-containing counterpart. The inhibition constant for zinc ions was also increased by a similar factor. However, the Vmax was unaltered. These results suggested that one or more methionine residues must be in close proximity to the substrate-binding pocket in the active site, rendering substrate access more difficult compared to the normal enzyme. This hypothesis was confirmed by the finding of four methionine residues lying along one wall of the active site.

摘要

磷酸甘露糖异构酶(PMI)是原核生物和真核生物蛋白质糖基化途径早期步骤中的一种必需酶。缺乏该酶对真菌生物体是致命的,因此它是一个潜在的杀真菌靶点。为了便于解析病原体白色念珠菌中该酶的三维结构,我们制备了重组硒代蛋氨酸标记的酶(SeMet-PMI)。用PMI表达质粒转化甲硫氨酸营养缺陷型大肠杆菌菌株DL41,并在富含硒代蛋氨酸的培养基上培养至高细胞密度。SeMet-PMI蛋白已被纯化,通过氨基酸分析发现其甲硫氨酸残基被硒代蛋氨酸残基取代。电喷雾质谱显示SeMet-PMI的主要分子量为49,063±10 Da,而正常重组酶为48,735±6 Da,这表明掺入了7个硒代蛋氨酸残基。SeMet-PMI与正常PMI蛋白同晶型结晶,晶体衍射分辨率达到0.23 nm。SeMet-PMI的动力学特征表明,其对底物6-磷酸甘露糖的Km值比含甲硫氨酸的对应物高四倍。锌离子的抑制常数也增加了类似的倍数。然而,Vmax未改变。这些结果表明,一个或多个甲硫氨酸残基必须靠近活性位点中的底物结合口袋,与正常酶相比,这使得底物进入更加困难。沿着活性位点的一侧壁发现四个甲硫氨酸残基,这一发现证实了这一假设。

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