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从杆状病毒过表达系统中纯化的神经元型一氧化氮合酶及其C415H突变体的特性分析。

Characterization of neuronal nitric oxide synthase and a C415H mutant, purified from a baculovirus overexpression system.

作者信息

Richards M K, Marletta M A

机构信息

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

出版信息

Biochemistry. 1994 Dec 13;33(49):14723-32. doi: 10.1021/bi00253a010.

DOI:10.1021/bi00253a010
PMID:7527656
Abstract

Nitric oxide synthase (NOS) catalyzes the conversion of L-arginine to citrulline and nitric oxide (.NO). A baculovirus overexpression system has been developed for a constitutive NOS isoform, cloned originally from rat cerebellum (B-NOS). Recombinant virus was used at a multiplicity of infection of 5 to infect Spodoptera frugiperda cells in culture, and NOS was expressed to 10% of the total soluble protein at 48 h postinfection. In order to express catalytically active enzyme, it was necessary to supplement the culture media with hemin. This increased the activity of the enzyme 7-fold. A two column affinity purification was developed for the recombinant enzyme, which gave homogeneous protein that migrated at 150 kDa on a denaturing polyacrylamide gel. A Km for L-arginine was determined to be 2.0 +/- 0.4 microM. As isolated, recombinant B-NOS exhibited a Soret maximum at 402 nm, which shifted to 394 nm in the presence of L-arginine. The Soret maximum of the reduced enzyme in the presence of CO was 444 nm. Initial rate steady-state kinetic analysis of the recombinant B-NOS showed evidence of substrate inhibition by L-arginine, which could also be seen in a partially purified preparation of B-NOS from rat cerebella. This substrate inhibition was not observed with the inducible isoform of NOS, purified from immunostimulated murine macrophages. A C415H mutant was overexpressed and purified using the same conditions established for the wild-type recombinant B-NOS. This C415H mutant exhibited no activity and did not bind heme, providing the first experimental evidence to support previously reported primary amino acid comparisons which suggest that C415 provides the coordinating thiolate to the heme moiety in B-NOS.

摘要

一氧化氮合酶(NOS)催化L-精氨酸转化为瓜氨酸和一氧化氮(·NO)。已开发出一种杆状病毒过表达系统用于组成型NOS同工型,该同工型最初从大鼠小脑克隆而来(B-NOS)。重组病毒以感染复数5用于感染培养中的草地贪夜蛾细胞,感染后48小时,NOS表达量达到总可溶性蛋白的10%。为了表达具有催化活性的酶,有必要在培养基中添加血红素。这使酶的活性提高了7倍。针对重组酶开发了两步亲和纯化法,得到的纯蛋白在变性聚丙烯酰胺凝胶上迁移时分子量为150 kDa。L-精氨酸的米氏常数测定为2.0±0.4微摩尔。刚分离出来时,重组B-NOS在402纳米处有一个索雷特峰最大值,在L-精氨酸存在时该峰最大值移至394纳米。在一氧化碳存在下,还原态酶的索雷特峰最大值为444纳米。对重组B-NOS的初始速率稳态动力学分析显示有L-精氨酸对底物的抑制作用,这在从大鼠小脑部分纯化得到的B-NOS制剂中也能看到。从免疫刺激的小鼠巨噬细胞中纯化得到的诱导型NOS同工型未观察到这种底物抑制作用。使用为野生型重组B-NOS建立的相同条件对C415H突变体进行了过表达和纯化。该C415H突变体无活性且不结合血红素,为先前报道的一级氨基酸比较提供了首个实验证据,该比较表明C415为B-NOS中的血红素部分提供配位硫醇盐。

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