Trimboli A J, Barber M J
Department of Biochemistry and Molecular Biology, University of South Florida, College of Medicine, Tampa.
Arch Biochem Biophys. 1994 Nov 15;315(1):48-53. doi: 10.1006/abbi.1994.1469.
Assimilatory nitrate reductase from Chlorella vulgaris catalyzes the rate-limiting step, the conversion of nitrate to nitrite, in nitrate assimilation. Initial rate studies of nitrate reductase activity, performed under optimum conditions of constant ionic strength (mu = 0.2) and pH (8.0) and using NADH as reductant, indicated the absence of substrate inhibition at NADH concentrations below 300 microM and NO3- concentrations less than 3 mM. Chlorella nitrate reductase exhibited a marked preference for NADH (Vmax = 9.2 mumol NADH/min/nmol heme and Km = 2.3 microM) as the physiological electron donor but could also utilize alpha-NADH (Vmax = 5.6 mumol NADH/min/nmol heme and Km = 131 microM) and NADPH (Vmax = 0.6 mumol NADPH/min/nmol heme and Km = 910 microM) though with significantly decreased efficiency. Examination of various NADH-analogs indicated that reduced nicotinamide hypoxanthine dinucleotide (NHDH) was used most efficiently (Vmax = 9.3 mumol NHDH/min/nmol heme and Km = 7.9 microM), while reduced nicotinamide mononucleotide (NMNH) was utilized least efficiently (Vmax = 0.07 mumol NMNH/min/nmol heme and Km = 676 microM). Overall, modifications to the nicotinamide moiety or the addition of a phosphate group were observed to result in the most significant decreases in Vmax, indicating poor reducing substrates. Product inhibition studies indicated both NAD+ (Ki = 2.2 mM) and NADP+ (Ki = 10.5 mM) to be competitive inhibitors of Chlorella NR. A variety of NAD+ analogs were also determined to act as competitive inhibitors with varying degrees of efficiency. 3-Pyridinealdehyde adenine dinucleotide was the most efficient inhibitor (Ki = 0.74 mM) while nicotinamide was the least efficient (Ki = 18.1 mM). Overall, changing substituents on the nicotinamide ring or its complete deletion produced the most effective inhibitors compared to NAD+. In contrast, changes in the adenine or ribose moieties produced less effective inhibitors when compared to NAD+. These results represent the most comprehensive analysis of the effect of modifications of the physiological reductant (NADH) and product (NAD+) on nitrate reductase activity.
小球藻的同化型硝酸还原酶催化硝酸盐同化过程中的限速步骤,即将硝酸盐转化为亚硝酸盐。在恒定离子强度(μ = 0.2)和pH(8.0)的最佳条件下,以NADH作为还原剂进行硝酸还原酶活性的初始速率研究,结果表明在NADH浓度低于300μM和NO3-浓度小于3 mM时不存在底物抑制。小球藻硝酸还原酶对作为生理电子供体的NADH表现出明显的偏好(Vmax = 9.2 μmol NADH/min/nmol血红素,Km = 2.3 μM),但也可以利用α-NADH(Vmax = 5.6 μmol NADH/min/nmol血红素,Km = 131 μM)和NADPH(Vmax = 0.6 μmol NADPH/min/nmol血红素,Km = 910 μM),不过效率显著降低。对各种NADH类似物的研究表明,还原型烟酰胺次黄嘌呤二核苷酸(NHDH)的利用效率最高(Vmax = 9.3 μmol NHDH/min/nmol血红素,Km = 7.9 μM),而还原型烟酰胺单核苷酸(NMNH)的利用效率最低(Vmax = 0.07 μmol NMNH/min/nmol血红素,Km = 676 μM)。总体而言,观察到烟酰胺部分的修饰或磷酸基团的添加会导致Vmax显著降低,表明还原底物较差。产物抑制研究表明,NAD+(Ki = 2.2 mM)和NADP+(Ki = 10.5 mM)都是小球藻硝酸还原酶的竞争性抑制剂。还确定了多种NAD+类似物作为竞争性抑制剂,效率各不相同。3-吡啶醛腺嘌呤二核苷酸是最有效的抑制剂(Ki = 0.74 mM),而烟酰胺是最无效的抑制剂(Ki = 18.1 mM)。总体而言,与NAD+相比,烟酰胺环上取代基的变化或其完全缺失产生了最有效的抑制剂。相比之下,与NAD+相比,腺嘌呤或核糖部分的变化产生的抑制剂效果较差。这些结果代表了对生理还原剂(NADH)和产物(NAD+)修饰对硝酸还原酶活性影响的最全面分析。
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