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来自集胞藻6803的二聚体血红素加氧酶-2与血红素复合物的晶体结构。

Crystal structure of dimeric heme oxygenase-2 from Synechocystis sp. PCC 6803 in complex with heme.

作者信息

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

机构信息

Department of Biology, Graduate School of Science, Osaka University, Toyonaka, Osaka 560-0043, Japan.

出版信息

Biochemistry. 2005 Mar 22;44(11):4257-66. doi: 10.1021/bi0480483.

DOI:10.1021/bi0480483
PMID:15766254
Abstract

Phycobiliproteins, light-harvesting proteins in cyanobacteria, red algae, and cryptophytes, contain phycobilin pigments. Phycobilins are synthesized from biliverdin, which is produced by the oxidative cleavage of the heme porphyrin ring catalyzed by heme oxygenase (HO). Two paralogs of ho (ho1 and ho2) have been identified in the genome of the cyanobacterium, Synechocystis sp. PCC 6803. The recombinant proteins of both paralogs (Syn HO-1 and Syn HO-2) possess in vitro heme degradation activity. We have determined the crystal structures of Syn HO-2 in complex with heme (heme-Syn HO-2) and its reduced and NO bound forms. The heme-Syn HO-2 crystal was a nonmerohedral twin, and detwinned diffraction data were used to refine the structure. Although heme-Syn HO-2 shares common folding with other HOs, the C-terminal segment is ordered and turns back to the heme-binding side. Gel-filtration chromatography analysis and molecular packing in the crystal indicate that heme-Syn HO-2 forms a homodimer, in which the C-terminal ordered segments interact with each other. Because Syn HO-2 is a monomer in the apo state, the dimeric interaction may aid in the selection of the reducing partner but likely does not interfere with heme binding. The heme iron is coordinated by a water molecule in the ferric form, but the distal water is absent in the ferrous form. In all of the Syn HO-2 structures, several water molecules form a hydrogen-bond network at the distal hemepocket, which is involved in HO activity. Upon NO binding, the side-chain conformation of Tyr 156 changes. Tyr 156 is located at the hydrophobic cluster, which interrupts the possible H(+) pathway from the molecular surface to the hemepocket. Thus, Tyr 156 may function as a H(+) shuttle by changing conformation.

摘要

藻胆蛋白是蓝藻、红藻和隐藻中的捕光蛋白,含有藻胆色素。藻胆色素由胆绿素合成,胆绿素是由血红素加氧酶(HO)催化血红素卟啉环氧化裂解产生的。在蓝藻集胞藻PCC 6803的基因组中已鉴定出ho的两个旁系同源物(ho1和ho2)。这两个旁系同源物的重组蛋白(Syn HO-1和Syn HO-2)都具有体外血红素降解活性。我们已经确定了与血红素结合的Syn HO-2(血红素-Syn HO-2)及其还原态和结合NO形式的晶体结构。血红素-Syn HO-2晶体是一个非等轴孪晶,使用解孪晶的衍射数据对结构进行了优化。尽管血红素-Syn HO-2与其他HO具有共同的折叠方式,但C末端片段是有序的,并折回到血红素结合侧。凝胶过滤色谱分析和晶体中的分子堆积表明,血红素-Syn HO-2形成同二聚体,其中C末端有序片段相互作用。由于Syn HO-2在脱辅基状态下是单体,二聚体相互作用可能有助于选择还原伴侣,但可能不会干扰血红素结合。血红素铁在三价铁形式下由一个水分子配位,但在二价铁形式下远端水分子不存在。在所有的Syn HO-2结构中,几个水分子在远端血红素口袋处形成氢键网络,这与HO活性有关。NO结合后,Tyr 156的侧链构象发生变化。Tyr 156位于疏水簇中,该疏水簇中断了从分子表面到血红素口袋的可能的H(+)途径。因此,Tyr 156可能通过改变构象起到H(+)穿梭的作用。

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