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诱导型一氧化氮合酶的一氧化氮复合物:光谱表征及其对催化活性的影响。

Nitric oxide complexes of inducible nitric oxide synthase: spectral characterization and effect on catalytic activity.

作者信息

Hurshman A R, Marletta M A

机构信息

Interdepartmental Program in Medicinal Chemistry, College of Pharmacy, University of Michigan, Ann Arbor 48109-1065, USA.

出版信息

Biochemistry. 1995 Apr 25;34(16):5627-34. doi: 10.1021/bi00016a038.

DOI:10.1021/bi00016a038
PMID:7537092
Abstract

Nitric oxide synthase (NOS) catalyzes the oxidation of L-arginine to citrulline and nitric oxide (.NO). NOS is a hemoprotein containing a cytochrome P-450-type heme that has been shown to be involved in catalysis. It has been suggested that .NO is able to bind tightly to the heme of NOS and may in this way serve to regulate enzymatic activity. We report here the formation of both ferric and ferrous heme nitrosyl complexes with the inducible NOS from murine macrophages. The ferric nitrosyl complex is characterized by a Soret peak at 443 nm and two distinct peaks in the alpha/beta region at 549 and 585 nm. The ferrous nitrosyl complex has absorbance maxima at 436 and 566 nm. A transient spectral intermediate is observed under conditions of NOS turnover. This intermediate appears to be a mixture of ferric and ferrous nitrosyl complexes and is unstable in the presence of oxygen. Binding of L-arginine decreases the affinity of .NO for the ferric heme but does not appear to decrease the affinity of .NO for the ferrous heme. Addition of either oxyhemoglobin or methemoglobin to NOS assays results in a nearly 2-fold increase in enzymatic activity. This result is attributed to the ability of both forms of hemoglobin to decrease the concentration of .NO in solution and is consistent with .NO inhibition of NOS under assay conditions. Our results show that NOS nitrosyl complexes form under certain conditions but suggest that the relevance of such complexes to activity in vivo may be limited by their instability in an aerobic environment.

摘要

一氧化氮合酶(NOS)催化L-精氨酸氧化为瓜氨酸和一氧化氮(·NO)。NOS是一种含细胞色素P-450型血红素的血红蛋白,已证明其参与催化作用。有人提出,·NO能够紧密结合到NOS的血红素上,并可能以此方式调节酶活性。我们在此报告了与小鼠巨噬细胞诱导型NOS形成的高铁和亚铁血红素亚硝酰复合物。高铁亚硝酰复合物的特征是在443nm处有一个Soret峰,在α/β区域的549和585nm处有两个不同的峰。亚铁亚硝酰复合物在436和566nm处有最大吸收峰。在NOS周转条件下观察到一个瞬态光谱中间体。这个中间体似乎是高铁和亚铁亚硝酰复合物的混合物,在有氧存在时不稳定。L-精氨酸的结合降低了·NO对高铁血红素的亲和力,但似乎没有降低·NO对亚铁血红素的亲和力。在NOS测定中加入氧合血红蛋白或高铁血红蛋白会导致酶活性增加近2倍。该结果归因于两种形式的血红蛋白都能降低溶液中·NO的浓度,并且与在测定条件下·NO对NOS的抑制作用一致。我们的结果表明,NOS亚硝酰复合物在某些条件下形成,但表明此类复合物在体内对活性的相关性可能受到其在有氧环境中不稳定性的限制。

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