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Two-iron rubredoxin of Pseudomonas oleovorans: Production, stability, and characterization of the individual iron-binding domains by optical, CD and NMR spectroscopies

机译:pseudomonas oleovorans的双铁红素氧化物:通过光学,CD和NmR光谱法制备,稳定和表征各个铁结合域

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摘要

A minigene encoding the C-terminal domain of the 2Fe rubredoxin of Pseudomonas oleovorans was created from the parental alk G gene contained in the expression plasmid pKK223-3. The vector directed the high-level production of the C-terminal domain of this rubredoxin; a simple procedure was used to purify the recombinant domain in the 1Fe form. The 1Fe form of the C-terminal domain was readily converted into the apoprotein and cadmium forms after precipitation with trichloroacetic acid and resolubilization in the presence or absence of cadmium chloride respectively. In steady-state assays, the recombinant 1Fe C-terminal domain is redox-active and able to transfer electrons from reduced rubredoxin reductase to cytochrome c. The absorption spectrum and dichroic features of the CD spectrum for the iron- and cadmium-substituted C-terminal domain are similar to those reported for the iron- and cadmium-substituted Desulfovibrio gigas rubredoxin [Henehen, Pountney, Zerbe and Vasak (1993) Protein Sci. 2, 1756-1764]. Difference absorption spectroscopy of the cadmium-substituted C-terminal domain revealed the presence of four Gaussian-resolved maxima at 202, 225, 240 and 276 nm; from Jørgensen's electronegativity theory, the 240 nm band is attributable to a CysS-Cd(II) charge-transfer excitation. Attempts to express the N-terminal domain of the 2Fe rubredoxin directly from a minigene were unsuccessful. However, the N-terminal domain was isolated through cleavage of an engineered 2Fe rubredoxin in which a factor Xa proteolysis site had been introduced into the putative interdomain linker. The N-terminal domain is characterized by absorption spectra typical of the 1Fe rubredoxins. The domain is folded as determined by CD and NMR spectroscopies and is redox-active. However, the N-terminal domain is less stable than the isolated C-terminal domain, a finding consistent with the known properties of the full-length 2Fe and cadmium-substituted Ps. oleovorans rubredoxin.
机译:从表达质粒pKK223-3中包含的亲代alk G基因产生一个编码油酸假单胞菌2Fe氧化还原酶C端结构域的小基因。该载体指导了该氧化还蛋白的C末端结构域的高水平产生。使用简单的程序纯化1Fe形式的重组结构域。在分别用三氯乙酸沉淀并在存在或不存在氯化镉的情况下再溶解后,C末端结构域的1Fe形式很容易转变为载脂蛋白和Cd形式。在稳态分析中,重组的1Fe C末端结构域具有氧化还原活性,并且能够将电子从还原的氧化还原酶还原酶转移至细胞色素c。铁和镉取代的C末端结构域的CD光谱的吸收光谱和二向色性特征与报道的铁和镉取代的Desulfovibrio gigas rubredoxin的吸收光谱和二向色性特征相似[Henehen,Pountney,Zerbe and Vasak(1993)Protein科学2,1756-1764]。镉取代的C末端结构域的差吸收光谱表明,在202、225、240和276 nm处存在四个高斯分辨的最大值。根据约根森(Jørgensen)的电负性理论,240 nm谱带可归因于CysS-Cd(II)电荷转移激发。尝试直接从小基因表达2Fe氧还蛋白的N末端结构域的尝试未成功。然而,通过切割工程化的2Fe氧化还原蛋白分离了N-末端结构域,其中将因子Xa蛋白水解位点引入假定的域间接头中。 N-末端结构域的特征在于1Fe氧化还原蛋白的典型吸收光谱。通过CD和NMR光谱确定该结构域是折叠的,并且具有氧化还原活性。但是,N末端结构域的稳定性低于分离的C末端结构域,这一发现与全长2Fe和镉取代的Ps的已知特性一致。油橄榄核糖蛋白。

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