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拟南芥中siro血红素生物合成末端酶的鉴定与表征:一种定位于质体的含2FE-2S中心的尿卟啉原Ⅲ亚铁螯合酶

Identification and characterization of the terminal enzyme of siroheme biosynthesis from Arabidopsis thaliana: a plastid-located sirohydrochlorin ferrochelatase containing a 2FE-2S center.

作者信息

Raux-Deery Evelyne, Leech Helen K, Nakrieko Kerry-Ann, McLean Kirsty J, Munro Andrew W, Heathcote Peter, Rigby Stephen E J, Smith Alison G, Warren Martin J

机构信息

School of Biological Sciences, Queen Mary, University of London, Mile End Rd., London E1 4NS, United Kingdom.

出版信息

J Biol Chem. 2005 Feb 11;280(6):4713-21. doi: 10.1074/jbc.M411360200. Epub 2004 Nov 15.

DOI:10.1074/jbc.M411360200
PMID:15545265
Abstract

Higher plant sulfite and nitrite reductases contain siroheme as a prosthetic group. Siroheme is synthesized from the tetrapyrrole primogenitor uroporphyrinogen III in three steps involving methylation, oxidation, and ferrochelation reactions. In this paper we report on the Arabidopsis thaliana sirohydrochlorin ferrochelatase At-SirB. The complete precursor protein of 225 amino acids and shorter constructs in which the first 46 or 79 residues had been removed were shown to complement a defined Escherichia coli sirohydrochlorin ferrochelatase mutant. The mature form of the protein appeared to consist of only 150 amino acids, making it much smaller than previously characterized ferrochelatases. Green fluorescent protein tagging revealed that it is located in the chloroplast. The enzyme was easily produced in E. coli as a recombinant protein, and the isolated enzyme was found to have a specific activity of 48.5 nmol/min/mg. Significantly, the protein purified as a brown-colored solution with a UV-visible spectrum containing maxima at 415 and 455 nm, suggestive of an Fe-S center. EPR analysis of the recombinant protein produced a rhombic spectrum with G-values of 2.04, 1.94, and 1.90 and with temperature dependence consistent with a 2Fe-2S center. Redox titration demonstrated that the Fe-S center is highly unstable, with an apparent midpoint reduction potential of about -370 mV. This is the first Fe-S center to be reported in a higher plant ferrochelatase. The implications of the Fe-S center in an enzyme that is so closely associated with the metabolism of sulfur and iron are discussed.

摘要

高等植物的亚硫酸盐和亚硝酸盐还原酶含有 siro 血红素作为辅基。Siro 血红素由四吡咯前体尿卟啉原 III 经甲基化、氧化和亚铁螯合反应三步合成。在本文中,我们报道了拟南芥 siro 氢氯血红素亚铁螯合酶 At-SirB。225 个氨基酸的完整前体蛋白以及去除了前 46 或 79 个残基的较短构建体被证明可以互补一个明确的大肠杆菌 siro 氢氯血红素亚铁螯合酶突变体。该蛋白的成熟形式似乎仅由 150 个氨基酸组成,比先前表征的亚铁螯合酶小得多。绿色荧光蛋白标记显示它位于叶绿体中。该酶很容易在大肠杆菌中作为重组蛋白产生,分离出的酶的比活性为 48.5 nmol/min/mg。值得注意的是,纯化的蛋白呈棕色溶液,其紫外可见光谱在 415 和 455 nm 处有最大值,表明存在 Fe-S 中心。对重组蛋白的 EPR 分析产生了一个菱形光谱,G 值为 2.04、1.94 和 1.90,并且温度依赖性与 2Fe-2S 中心一致。氧化还原滴定表明 Fe-S 中心非常不稳定,表观中点还原电位约为 -370 mV。这是首次在高等植物亚铁螯合酶中报道 Fe-S 中心。讨论了 Fe-S 中心在与硫和铁代谢密切相关的酶中的意义。

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