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刚地弓形虫蝶呤-4a-氨基甲醇脱水酶的晶体结构及其与哺乳动物和寄生虫同源物的比较。

Crystal structures of Toxoplasma gondii pterin-4a-carbinolamine dehydratase and comparisons with mammalian and parasite orthologues.

作者信息

Cameron Scott, Fyffe Stewart A, Goldie Simon, Hunter William N

机构信息

Division of Biological Chemistry and Drug Discovery, College of Life Sciences, University of Dundee, Dundee DD1 5EH, UK.

出版信息

Mol Biochem Parasitol. 2008 Apr;158(2):131-8. doi: 10.1016/j.molbiopara.2007.12.002. Epub 2007 Dec 15.

Abstract

The enzyme pterin-4a-carbinolamine dehydratase (PCD) is important for the recycling of pterins within eukaryotic cells. A recombinant expression system for PCD from the apicomplexan parasite Toxoplasma gondii has been prepared, the protein purified and crystallised. Single crystal X-ray diffraction methods have produced a high-resolution structure (1.6A) of the apo-enzyme and a low-resolution structure (3.1A) of a complex with a substrate-like ligand dihydrobiopterin (BH(2)). Analysis of the hydrogen bonding interactions that contribute to binding BH(2) suggest that the ligand is present in an enol tautomeric state, which makes it more similar to the physiological substrate. The enzyme can process (R)- and (S)-forms of pterin-4a-carbinolamine and the ligand complex suggests that His61 and His79 are placed to act independently as general bases for catalysis of the individual enantiomers. Comparisons with orthologues from other protozoan parasites (Plasmodium falciparum and Leishmania major) and with rat PCD, for which the structure is known, indicate a high degree of sequence and structure conservation of this enzyme. The molecular determinants of ligand recognition and PCD reactivity are therefore highly conserved across species.

摘要

蝶呤-4a-甲醇胺脱水酶(PCD)对于真核细胞内蝶呤的循环利用很重要。已构建了来自顶复门寄生虫刚地弓形虫的PCD重组表达系统,对该蛋白质进行了纯化和结晶。单晶X射线衍射方法得到了脱辅基酶的高分辨率结构(1.6埃)以及与底物类似配体二氢生物蝶呤(BH(2))形成的复合物的低分辨率结构(3.1埃)。对有助于结合BH(2)的氢键相互作用的分析表明,该配体以烯醇互变异构体状态存在,这使其更类似于生理底物。该酶能够处理蝶呤-4a-甲醇胺的(R)-和(S)-形式,配体复合物表明His61和His79的位置可独立作为催化各个对映体的通用碱。与其他原生动物寄生虫(恶性疟原虫和硕大利什曼原虫)的直系同源物以及已知结构的大鼠PCD进行比较,表明该酶在序列和结构上具有高度保守性。因此,配体识别和PCD反应性的分子决定因素在物种间高度保守。

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