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血红素 A 合酶的晶体结构来自.

Crystal structure of heme A synthase from .

机构信息

Department of Chemistry, Graduate School of Science, Kyoto University, 606-8502 Kyoto, Japan.

School of International Health, Graduate School of Medicine, University of Tokyo, Hongo, Bunkyo-ku, Tokyo 113-0033, Japan.

出版信息

Proc Natl Acad Sci U S A. 2018 Nov 20;115(47):11953-11957. doi: 10.1073/pnas.1813346115. Epub 2018 Nov 5.

Abstract

Heme A is an essential cofactor for respiratory terminal oxidases and vital for respiration in aerobic organisms. The final step of heme A biosynthesis is formylation of the C-8 methyl group of heme molecule by heme A synthase (HAS). HAS is a heme-containing integral membrane protein, and its structure and reaction mechanisms have remained unknown. Thus, little is known about HAS despite of its importance. Here we report the crystal structure of HAS from at 2.2-Å resolution. The N- and C-terminal halves of HAS consist of four-helix bundles and they align in a pseudo twofold symmetry manner. Each bundle contains a pair of histidine residues and forms a heme-binding domain. The C-half domain binds a cofactor-heme molecule, while the N-half domain is vacant. Many water molecules are found in the transmembrane region and around the substrate-binding site, and some of them interact with the main chain of transmembrane helix. Comparison of these two domain structures enables us to construct a substrate-heme binding state structure. This structure implies that a completely conserved glutamate, Glu57 in , is the catalytic residue for the formylation reaction. These results provide valuable suggestions of the substrate-heme binding mechanism. Our results present significant insight into the heme A biosynthesis.

摘要

血红素 A 是呼吸末端氧化酶的必需辅因子,对需氧生物的呼吸至关重要。血红素 A 生物合成的最后一步是血红素 A 合酶 (HAS) 将血红素分子的 C-8 甲基甲酰化。HAS 是一种含血红素的整合膜蛋白,其结构和反应机制仍不清楚。因此,尽管 HAS 很重要,但对其了解甚少。在这里,我们报道了来自 的 HAS 的晶体结构,分辨率为 2.2 Å。HAS 的 N 端和 C 端两半由四个螺旋束组成,并以伪二倍对称方式排列。每个束包含一对组氨酸残基并形成血红素结合结构域。C 半结构域结合辅助因子血红素分子,而 N 半结构域为空。在跨膜区域及其周围的底物结合位点发现了许多水分子,其中一些与跨膜螺旋的主链相互作用。这两个结构域的比较使我们能够构建一个底物血红素结合状态的结构。该结构表明,一个完全保守的谷氨酸,即 中的 Glu57,是甲酰化反应的催化残基。这些结果为底物血红素结合机制提供了有价值的建议。我们的研究结果为血红素 A 的生物合成提供了重要的见解。

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