氧铁血红素而非酪氨酸自由基可能是前列腺素H合酶-1过氧化物酶失活的罪魁祸首。
Oxyferryl heme and not tyrosyl radical is the likely culprit in prostaglandin H synthase-1 peroxidase inactivation.
作者信息
Wu Gang, Rogge Corina E, Wang Jinn-Shyan, Kulmacz Richard J, Palmer Graham, Tsai Ah-Lim
机构信息
Department of Internal Medicine, University of Texas Health Science Center, Houston, Texas 77030, USA.
出版信息
Biochemistry. 2007 Jan 16;46(2):534-42. doi: 10.1021/bi061859h.
Prostaglandin H synthase-1 (PGHS-1) is a bifunctional heme protein catalyzing both a peroxidase reaction, in which peroxides are converted to alcohols, and a cyclooxygenase reaction, in which arachidonic acid is converted into prostaglandin G2. Reaction of PGHS-1 with peroxide forms Intermediate I, which has an oxyferryl heme and a porphyrin radical. An intramolecular electron transfer from Tyr385 to Intermediate I forms Intermediate II, which contains two oxidants: an oxyferryl heme and the Tyr385 radical required for cyclooxygenase catalysis. Self-inactivation of the peroxidase begins with Intermediate II, but it has been unclear which of the two oxidants is involved. The kinetics of tyrosyl radical, oxyferryl heme, and peroxidase inactivation were examined in reactions of PGHS-1 reconstituted with heme or mangano protoporphyrin IX with a lipid hydroperoxide, 15-hydroperoxyeicosatetraenoic acid (15-HPETE), and ethyl hydrogen peroxide (EtOOH). Tyrosyl radical formation was significantly faster with 15-HPETE than with EtOOH and roughly paralleled oxyferryl heme formation at low peroxide levels. However, the oxyferryl heme intensity decayed much more rapidly than the tyrosyl radical intensity at high peroxide levels. The rates of reactions for PGHS-1 reconstituted with MnPPIX were approximately an order of magnitude slower, and the initial species formed displayed a wide singlet (WS) radical, rather than the wide doublet radical observed with PGHS-1 reconstituted with heme. Inactivation of the peroxidase activity during the reaction of PGHS-1 with EtOOH or 15-HPETE correlated with oxyferryl heme decay, but not with changes in tyrosyl radical intensity or EPR line shape, indicating that the oxyferryl heme, and not the tyrosyl radical, is responsible for the self-destructive peroxidase side reactions. Computer modeling to a minimal mechanism was consistent with oxyferryl heme being the source of peroxidase inactivation.
前列腺素H合酶-1(PGHS-1)是一种双功能血红素蛋白,它既能催化过氧化物酶反应(在此反应中过氧化物被转化为醇),又能催化环氧化酶反应(在此反应中花生四烯酸被转化为前列腺素G2)。PGHS-1与过氧化物反应形成中间体I,其具有氧合铁血红素和卟啉自由基。从Tyr385到中间体I的分子内电子转移形成中间体II,它包含两种氧化剂:一种氧合铁血红素和环氧化酶催化所需的Tyr385自由基。过氧化物酶的自失活从中间体II开始,但尚不清楚两种氧化剂中哪一种参与其中。在用血红素或锰原卟啉IX重构的PGHS-1与脂质氢过氧化物、15-氢过氧化二十碳四烯酸(15-HPETE)和乙基过氧化氢(EtOOH)的反应中,研究了酪氨酸自由基、氧合铁血红素和过氧化物酶失活的动力学。15-HPETE形成酪氨酸自由基的速度明显快于EtOOH,并且在低过氧化物水平下大致与氧合铁血红素的形成平行。然而,在高过氧化物水平下,氧合铁血红素的强度比酪氨酸自由基的强度衰减得快得多。用MnPPIX重构的PGHS-1的反应速率大约慢一个数量级,并且形成的初始物种显示出宽单重态(WS)自由基,而不是用血红素重构的PGHS-1所观察到的宽双重态自由基。在PGHS-1与EtOOH或15-HPETE反应期间过氧化物酶活性的失活与氧合铁血红素的衰减相关,但与酪氨酸自由基强度或电子顺磁共振谱线形状的变化无关,这表明氧合铁血红素而非酪氨酸自由基是过氧化物酶自毁性副反应的原因。对最小机制的计算机建模与氧合铁血红素是过氧化物酶失活的来源一致。
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