McMillan K, Bredt D S, Hirsch D J, Snyder S H, Clark J E, Masters B S
Department of Biochemistry, University of Texas Health Science Center, San Antonio 78284-7760.
Proc Natl Acad Sci U S A. 1992 Dec 1;89(23):11141-5. doi: 10.1073/pnas.89.23.11141.
The endogenous formation of nitric oxide (NO) has become an area of intense interest as evidence for its biological functions has been obtained in three distinct tissues: circulating macrophages, in which it exerts cytotoxic effects; blood vessels, in which it has been identified as endothelium-derived relaxing factor; and neuronal cells, in which it functions as a neurotransmitter. The formation of NO in brain extracts has been shown to be catalyzed by an enzyme, termed NO synthase, which generates the NO responsible for stimulation of cGMP formation, the highest levels of which occur in the cerebellum. NO synthase catalyzes the formation of citrulline from arginine with the coincident production of NO and has been shown to be a flavoprotein, containing 1 mol each of FAD and FMN, tetrahydrobiopterin, and iron. It is also reported to contain an alpha-helical, calmodulin-binding consensus sequence consistent with its stimulation by calmodulin in the presence of Ca2+. The formation of NO requires incorporation of one of the atoms of molecular oxygen into one of the guanidinium nitrogen atoms of arginine with the coincident formation of citrulline. This communication reports that rat cerebellar NO synthase, cloned and stably expressed in human kidney 293 cells, contains heme in amounts stoichiometric with the flavins FAD and FMN as evidenced by the appearance of a pyridine hemochrome and a reduced CO difference spectrum with an absorbance maximum at approximately 445 nm. The finding of a CO-binding heme moiety explains the presence of iron in the enzyme and suggests a role for prosthetic heme as an oxygenase reaction center. This report also presents evidence for incorporation of delta-[14C]aminolevulinate specifically into immunoprecipitable NO synthase in stably transfected human kidney 293 cells but not in nontransfected cells. Simultaneously, K. A. White and M. A. Marletta [(1992) Biochemistry 31, 6627-6631] have demonstrated a CO-binding heme prosthetic group in purified murine macrophage NO synthase and have suggested the identity of these reaction centers in both the constitutive (cerebellar) and inducible (macrophage) forms of NO synthase.
一氧化氮(NO)的内源性生成已成为一个备受关注的领域,因为在三种不同组织中已获得其生物学功能的证据:循环巨噬细胞,其中NO发挥细胞毒性作用;血管,其中NO被确定为内皮衍生舒张因子;以及神经元细胞,其中NO作为神经递质发挥作用。已证明脑提取物中NO的生成由一种称为NO合酶的酶催化,该酶生成负责刺激cGMP生成的NO,其中cGMP的最高水平出现在小脑中。NO合酶催化精氨酸生成瓜氨酸,同时产生NO,并且已证明它是一种黄素蛋白,含有1摩尔的FAD和FMN、四氢生物蝶呤和铁。据报道,它还含有一个α-螺旋、钙调蛋白结合共有序列,这与其在Ca2+存在下受钙调蛋白刺激一致。NO的生成需要将分子氧的一个原子掺入精氨酸的一个胍基氮原子中,同时生成瓜氨酸。本通讯报道,在人肾293细胞中克隆并稳定表达的大鼠小脑NO合酶含有与黄素FAD和FMN化学计量相当的血红素,这由吡啶血红素的出现和在约445nm处有最大吸收的还原CO差光谱证明。发现与CO结合的血红素部分解释了该酶中铁的存在,并表明辅基血红素作为加氧酶反应中心的作用。本报告还提供了证据,表明在稳定转染的人肾293细胞中,δ-[14C]氨基乙酰丙酸特异性掺入可免疫沉淀的NO合酶中,但在未转染的细胞中则不然。同时,K.A.怀特和M.A.马莱塔[(1992年)《生物化学》31,6627 - 6631]已在纯化的小鼠巨噬细胞NO合酶中证明了一个与CO结合的血红素辅基,并提出了在组成型(小脑)和诱导型(巨噬细胞)NO合酶中这些反应中心的一致性。
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