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嗜气栖热菌磷酸葡萄糖异构酶中磷酸甘露糖异构酶活性的结构基础:远缘相关酶之间的细微差异。

Structural basis for phosphomannose isomerase activity in phosphoglucose isomerase from Pyrobaculum aerophilum: a subtle difference between distantly related enzymes.

作者信息

Swan Michael K, Hansen Thomas, Schönheit Peter, Davies Christopher

机构信息

Department of Biochemistry and Molecular Biology, Medical University of South Carolina, Charleston, South Carolina 29425, USA.

出版信息

Biochemistry. 2004 Nov 9;43(44):14088-95. doi: 10.1021/bi048608y.

Abstract

The crystal structure of a dual-specificity phosphoglucose/phosphomannose isomerase from the crenarchaeon Pyrobaculum aerophilum (PaPGI/PMI) has been determined in complex with glucose 6-phosphate at 1.16 A resolution and with fructose 6-phosphate at 1.5 A resolution. Subsequent modeling of mannose 6-phosphate (M6P) into the active site of the enzyme shows that the PMI activity of this enzyme may be due to the additional space imparted by a threonine. In PGIs from bacterial and eukaryotic sources, which cannot use M6P as a substrate, the equivalent residue is a glutamine. The increased space may permit rotation of the C2-C3 bond in M6P to facilitate abstraction of a proton from C2 by Glu203 and, after a further C2-C3 rotation of the resulting cis-enediolate, re-donation of a proton to C1 by the same residue. A proline residue (in place of a glycine in PGI) may also promote PMI activity by positioning the C1-O1 region of M6P. Thus, the PMI reaction in PaPGI/PMI probably uses a cis-enediol mechanism of catalysis, and this activity appears to arise from a subtle difference in the architecture of the enzyme, compared to bacterial and eukaryotic PGIs.

摘要

嗜热栖热袍菌(Pyrobaculum aerophilum)的双特异性磷酸葡萄糖/磷酸甘露糖异构酶(PaPGI/PMI)的晶体结构已分别在与1.16 Å分辨率的6-磷酸葡萄糖和1.5 Å分辨率的6-磷酸果糖结合的情况下得以确定。随后将6-磷酸甘露糖(M6P)模拟到该酶的活性位点中,结果表明该酶的PMI活性可能归因于苏氨酸赋予的额外空间。在来自细菌和真核生物来源的PGI中,它们不能将M6P用作底物,其对应的残基是谷氨酰胺。增加的空间可能使M6P中的C2-C3键旋转,从而便于Glu203从C2提取一个质子,并且在所得顺式烯二醇盐的C2-C3进一步旋转之后,由同一残基将质子重新供体给C1。一个脯氨酸残基(取代PGI中的甘氨酸)也可能通过定位M6P的C1-O1区域来促进PMI活性。因此,PaPGI/PMI中的PMI反应可能采用顺式烯二醇催化机制,与细菌和真核生物的PGI相比,这种活性似乎源于该酶结构上的细微差异。

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