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一氧化氮对可溶性鸟苷酸环化酶激活作用的光谱和动力学研究。

Spectral and kinetic studies on the activation of soluble guanylate cyclase by nitric oxide.

作者信息

Stone J R, Marletta M A

机构信息

Department of Biological Chemistry, School of Medicine, College of Pharmacy, University of Michigan, Ann Arbor 48109-1065, USA.

出版信息

Biochemistry. 1996 Jan 30;35(4):1093-9. doi: 10.1021/bi9519718.

DOI:10.1021/bi9519718
PMID:8573563
Abstract

The soluble form of guanylate cyclase (sGC) is the only definitive receptor for the signaling agent nitric oxide (.NO). The enzyme is a heterodimer of homologous subunits in which each subunit binds 1 equiv of 5-coordinate high-spin heme. .NO increases the Vmax of sGC up to 400-fold and has previously been shown to bind to the heme to form a 5-coordinate complex. Using stopped-flow spectrophotometry, it is demonstrated that the binding of .NO to the heme of sGC is a complex process. .NO first binds to the heme to form a 6-coordinate nitrosyl complex, which then converts to a 5-coordinate nitrosyl complex through one of two ways. For 28 +/- 4% of the heme, the 6-coordinate nitrosyl complex rapidly (approximately 20 s-1) converts to the 5-coordinate complex. For the remaining 72 +/- 4% of the heme, the conversion of the 6-coordinate nitrosyl complex to a 5-coordinate nitrosyl complex is slow (0.1-1.0 s-1) and is dependent upon the interaction of .NO with an unidentified non-heme site on the protein. The heme (200 nM) was completely converted to the 5-coordinate state with as little as 500 nM .NO, and the equilibrium dissociation constant of .NO for activating the enzyme was determined to be < or = 250 nM. Gel-filtration analysis indicates that the binding of .NO to the heme has no effect on the native molecular mass of the protein. Correlation of electronic absorption spectra with activity measurements indicates that the 5-coordinate nitrosyl form of the enzyme is activated relative to the resting 5-coordinate ferrous form of the enzyme.

摘要

可溶性鸟苷酸环化酶(sGC)是信号分子一氧化氮(.NO)的唯一确定性受体。该酶是同源亚基的异二聚体,其中每个亚基结合1当量的五配位高自旋血红素。.NO可使sGC的Vmax增加高达400倍,并且先前已证明其与血红素结合形成五配位复合物。使用停流分光光度法表明,.NO与sGC血红素的结合是一个复杂的过程。.NO首先与血红素结合形成六配位亚硝酰复合物,然后通过两种方式之一转化为五配位亚硝酰复合物。对于28±4%的血红素,六配位亚硝酰复合物迅速(约20 s-1)转化为五配位复合物。对于其余72±4%的血红素,六配位亚硝酰复合物向五配位亚硝酰复合物的转化缓慢(0.1-1.0 s-1),并且取决于.NO与蛋白质上未鉴定的非血红素位点的相互作用。仅用500 nM的.NO就可将200 nM的血红素完全转化为五配位状态,并且确定.NO激活该酶的平衡解离常数≤250 nM。凝胶过滤分析表明,.NO与血红素的结合对蛋白质的天然分子量没有影响。电子吸收光谱与活性测量的相关性表明,相对于酶的静止五配位亚铁形式,酶的五配位亚硝酰形式被激活。

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