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来自集胞藻属PCC 6803蓝细菌的血红素加氧酶-1与血红素复合物的晶体结构。

Crystal structure of heme oxygenase-1 from cyanobacterium Synechocystis sp. PCC 6803 in complex with heme.

作者信息

Sugishima Masakazu, Migita Catharina T, Zhang Xuhong, Yoshida Tadashi, Fukuyama Keiichi

机构信息

Department of Biology, Graduate School of Science, Osaka University, Toyonaka, Osaka, Japan.

出版信息

Eur J Biochem. 2004 Nov;271(22):4517-25. doi: 10.1111/j.1432-1033.2004.04411.x.

DOI:10.1111/j.1432-1033.2004.04411.x
PMID:15560792
Abstract

Heme oxygenase (HO) catalyzes the oxidative degradation of heme utilizing molecular oxygen and reducing equivalents. In photosynthetic organisms, HO functions in the biosynthesis of such open-chain tetrapyrroles as phyto-chromobilin and phycobilins, which are involved in the signal transduction for light responses and light harvesting for photosynthesis, respectively. We have determined the first crystal structure of a HO-1 from a photosynthetic organism, Synechocystis sp. PCC 6803 (Syn HO-1), in complex with heme at 2.5 A resolution. Heme-Syn HO-1 shares a common folding with other heme-HOs. Although the heme pocket of heme-Syn HO-1 is, for the most part, similar to that of mammalian HO-1, they differ in such features as the flexibility of the distal helix and hydrophobicity. In addition, 2-propanol derived from the crystallization solution occupied the hydrophobic cavity, which is proposed to be a CO trapping site in rat HO-1 that suppresses product inhibition. Although Syn HO-1 and mammalian HO-1 are similar in overall structure and amino acid sequence (57% similarity vs. human HO-1), their molecular surfaces differ in charge distribution. The surfaces of the heme binding sides are both positively charged, but this patch of Syn HO-1 is narrow compared to that of mammalian HO-1. This feature is suited to the selective binding of ferredoxin, the physiological redox partner of Syn HO-1; the molecular size of ferredoxin is approximately 10 kDa whereas the size of NADPH-cytochrome P450 reductase, a reducing partner of mammalian HO-1, is approximately 77 kDa. A docking model of heme-Syn HO-1 and ferredoxin suggests indirect electron transfer from an iron-sulfur cluster in ferredoxin to the heme iron of heme-Syn HO-1.

摘要

血红素加氧酶(HO)利用分子氧和还原当量催化血红素的氧化降解。在光合生物中,HO在诸如植物色素胆素和藻胆素等开链四吡咯的生物合成中发挥作用,它们分别参与光反应的信号转导和光合作用的光捕获。我们已经确定了来自光合生物集胞藻PCC 6803(Syn HO-1)的HO-1与血红素复合物的首个晶体结构,分辨率为2.5埃。血红素-Syn HO-1与其他血红素-HO具有共同的折叠方式。尽管血红素-Syn HO-1的血红素口袋在很大程度上与哺乳动物HO-1的相似,但它们在诸如远端螺旋的柔韧性和疏水性等特征上有所不同。此外,来自结晶溶液的2-丙醇占据了疏水腔,该疏水腔被认为是大鼠HO-1中抑制产物抑制的CO捕获位点。尽管Syn HO-1和哺乳动物HO-1在整体结构和氨基酸序列上相似(与人类HO-1的相似度为57%),但它们的分子表面电荷分布不同。血红素结合侧的表面均带正电荷,但与哺乳动物HO-1相比,Syn HO-1的这片区域较窄。这一特征适合于铁氧还蛋白(Syn HO-1的生理氧化还原伙伴)的选择性结合;铁氧还蛋白的分子大小约为10 kDa,而哺乳动物HO-1的还原伙伴NADPH-细胞色素P450还原酶的大小约为77 kDa。血红素-Syn HO-1与铁氧还蛋白的对接模型表明,电子从铁氧还蛋白中的铁硫簇间接转移至血红素-Syn HO-1的血红素铁。

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