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反硝化细菌可溶性一氧化二氮还原酶的首个实用检测方法及部分动力学特性研究

First practical assay for soluble nitrous oxide reductase of denitrifying bacteria and a partial kinetic characterization.

作者信息

Kristjansson J K, Hollocher T C

出版信息

J Biol Chem. 1980 Jan 25;255(2):704-7.

PMID:7356639
Abstract

Lysis of spheroplasts made from denitrification-adapted Paracoccus denitrificans released a soluble nitrous oxide reductase which was assayed spectrophotometrically under anaerobic conditions by following the oxidation of methyl or benzyl viologen cation radical upon reduction of N2O to N2. Other classes of reductants so far tested, including dithionite, could not substitute for viologen dyes. Viologen dyes, therefore, afford the first practical assay for this previously elusive enzyme of denitrifying bacteria. The assay is specifically an in vitro assay, because the dyes cannot couple with intracellular nitrous oxide reductase. The enzyme exhibited simple saturation kinetics with respect to both N2O and reduced viologen dye. The Km for N2O was about 5 microM at 22 degrees C and pH 7.1 and the apparent Km for reduced benzyl and methyl viologen was 0.9 and 0.5 microM, respectively. Both dyes afforded the same Vmax value. Oxidized viologen dyes were not inhibiting to 1 mM nor was N2 to 1 atm. In fresh lysates, Vmax was about 1.2 mumol of N2O X min-1 x mg of protein-1 or about twice that for intact cells or spheroplasts utilizing yeast extract or lactate. Enzyme activity was observed to be labile in crude preparations under anaerobic conditions. Nitrous oxide reductase was inhibited by acetylene, CO, azide, and cyanide with Ki values of 28, 3.5, 0.35, and 0.045 microM, respectively. All showed noncompetitive inhibition with respect to N2O.

摘要

对适应反硝化作用的脱氮副球菌制成的原生质球进行裂解,释放出一种可溶性一氧化二氮还原酶。在厌氧条件下,通过跟踪一氧化二氮还原为氮气时甲基紫精或苄基紫精阳离子自由基的氧化,用分光光度法对该酶进行测定。到目前为止所测试的其他种类的还原剂,包括连二亚硫酸盐,都不能替代紫精染料。因此,紫精染料为这种以前难以捉摸的反硝化细菌的酶提供了首个实用的测定方法。该测定方法具体是一种体外测定方法,因为染料不能与细胞内的一氧化二氮还原酶偶联。该酶对一氧化二氮和还原型紫精染料均表现出简单的饱和动力学。在22℃和pH 7.1条件下,一氧化二氮的Km约为5微摩尔,还原型苄基紫精和甲基紫精的表观Km分别为0.9和0.5微摩尔。两种染料的Vmax值相同。氧化型紫精染料在1毫摩尔时无抑制作用,氮气在1个大气压时也无抑制作用。在新鲜裂解物中,Vmax约为1.2微摩尔一氧化二氮×分钟-1×毫克蛋白-1,约为利用酵母提取物或乳酸的完整细胞或原生质球的两倍。在厌氧条件下,观察到粗制品中的酶活性不稳定。一氧化二氮还原酶受到乙炔、一氧化碳、叠氮化物和氰化物的抑制,Ki值分别为28、3.5、0.35和0.045微摩尔。所有这些都对一氧化二氮表现出非竞争性抑制作用。

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