首页> 美国卫生研究院文献>Journal of Bacteriology >Effects of Molybdate Tungstate and Selenium Compounds on Formate Dehydrogenase and Other Enzyme Systems in Escherichia coli
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Effects of Molybdate Tungstate and Selenium Compounds on Formate Dehydrogenase and Other Enzyme Systems in Escherichia coli

机译:钼酸盐钨酸盐和硒化合物对大肠杆菌中的甲酸盐脱氢酶和其他酶系统的影响

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摘要

The role of selenium and molybdenum in the metabolism of Escherichia coli was explored by growing cells in a simple salts medium and examining the metabolic consequences of altering the concentration of molybdenum and selenium compounds in the medium. The addition of tungstate increased the molybdate deficiency of this medium, as reflected by lowered levels of enzyme systems previously recognized to require compounds of molybdenum and selenium for their formation [formate-dependent oxygen reduction, formate dehydrogenase (FDH) (EC 1.2.2.1), and nitrate reductase (EC 1.9.6.1)]. The requirement for selenium and molybdenum appears to be unique to the enzymes of formate and nitrate metabolism since molybdate- and selenite-deficient medium had no effect on the level of several dehydrogenase and oxidase systems, for which the electron donors were reduced nicotinamide adenine dinucleotide, succinate, d- or l-lactate, and glycerol. In addition, no effect was observed on the growth rate or cell yield with any carbon source tested (glucose, glycerol, dl-lactate, acetate, succinate, and l-malate) when the medium was deficient in molybdenum and selenium. dl-Selenocystine was about as effective as selenite in stimulating the formation of formate dehydrogenase, whereas dl-selenomethionine was only 1% as effective. In aerobic cells, an amount of FDH was formed such that 3,200 or 3,800 moles of formate were oxidized per min per mole of added selenium (added as dl-selenocystine or selenite, respectively).
机译:通过在简单的盐培养基中培养细胞并研究改变培养基中钼和硒化合物浓度的代谢后果,探索了硒和钼在大肠杆菌代谢中的作用。钨酸盐的添加增加了该培养基的钼酸盐缺乏,这反映在以前公认需要钼和硒化合物形成的酶体系水平降低的情况下(依赖于甲酸的氧还原,甲酸脱氢酶(FDH)(EC 1.2.2.1))。 ,和硝酸盐还原酶(EC 1.9.6.1)]。硒和钼的需求似乎是甲酸和硝酸盐代谢酶所特有的,因为缺乏钼酸盐和亚硒酸盐的培养基对几种脱氢酶和氧化酶系统的水平没有影响,为此电子供体被还原为烟酰胺腺嘌呤二核苷酸,琥珀酸,d-或l-乳酸和甘油。另外,当培养基中的钼和硒缺乏时,使用任何测试的碳源(葡萄糖,甘油,dl-乳酸盐,乙酸盐,琥珀酸盐和l-苹果酸盐),均未观察到对生长速率或细胞产量的影响。 dl-硒代胱氨酸在刺激甲酸脱氢酶形成方面与亚硒酸盐一样有效,而dl-硒代甲硫氨酸的功效仅为亚硒酸钠。在好氧细胞中,形成一定量的FDH,使得每摩尔添加的硒(分别以dl-硒代胱氨酸或亚硒酸盐添加)每分钟氧化3,200或3,800摩尔甲酸盐。

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