Characterization of a membrane-bound nitrate reductase from Azotobacter chroococcum.

Nitrate reductase from the aerobic bacterium $\text{Azotobacter chroococcum}$ is a soluble enzyme with the characteristic features of Pichinoty's type B nitrate reductase. When cell suspensions of $\text{A. chroococcum}$ are repeatedly subcultured in liquid medium with nitrate as the nitrogen source, most of the nitrate-reducing activity is incorporated into the cytoplasmic membrane. The properties of the particulate nitrate reductase closely resemble Pichinoty's type A enzyme.     

Energy-dependence of the Assimilatory Nitrate Uptake in Azorhizobium caulinodans Strain IRBG 46

Nitrate assimilation by suspensions of Azorhizobium caulinodans strain IRBG 46, as determined by disappearance of nitrate ions from the external medium, displayed the requirement of readily utilizable carbon source. Nitrate uptake was blocked by the uncouplers of oxidative phosphorylation such as 2,4-dinitrophenol, carbonyl cyanide m-chlorophenyl hydrazone and by an inhibitor of ATPase, N, N — dicyclohexyl carbodiimide. The inhibition of nitrate assimilation in the absence of appropriate carbon source was not overcome by the non-physiological terminal electron donor ascorbate plus N-methyl phenazinium methyl sulphate, a substrate combination that allows electron transfer to O₂ without the synthesis of ATP. These data suggest that transport of nitrate into the cell is directly dependent on ATP.     

Nitrate reductase from Azotobacter chroococcum. Inactivation by oxidizing agents and reactivation with dithioerythritol

Treatment of a partially purified nitrate reductase preparation from the aerobic bacterium $\text{Azotobacter chroococcum}$ with a variety of oxidizing agents, such as glutathione, ferricyanide and illuminated flavins, results in inactivation of the enzyme. Independently of the mode of inactivation, incubation in the presence of dithioerythritol causes almost full recovery of nitrate reductase activity. Our data suggest that $\text{Azotobacter}$ nitrate reductase might be regulated through an interconversion process between an oxidized inactive form and a reduced active one.     

Control of mitochondrial respiration by the phosphate potential

The rate of respiration of suspensions of mitochondria in the presence of excess oxygen and substrate is shown to be dependent on the ratio of the concentration of adenosine triphosphate (ATP) to the product of the concentrations of adenosine diphosphate and orthophosphate. The mitochondrial respiratory chain is essentially in equilibrium with the reactions for ATP synthesis. The rate of mitochondrial respiration is controlled by the free energy requirement for ATP synthesis and this control is expressed on the rates of the reactions for reduction of the dehydrogenases by substrate and the oxidation of cytochrome $\text{a}{}_3$ by molecular oxygen.     

Measurement of the intramitochondrial P/O ratio

Measurements of the initial rate of ATP synthesis and the initial rate of oxygen consumption in mitochondria in which transport of ADP, Pi and ATP were inhibited were used to obtain a value for the intramitochondrial $\text{P}\text{O}$ ratio. With succinate as substrate this method yielded a $\text{P}\text{O}$ ratio of 2.8 for the phosphorylation of intramitochondrial ADP.     

Studies on the red oxidase (cytochrome o) of Azotobacter vinelandii

In an attempt to isolate and to study the electron transport system of $\text{Azotobacter vinelandii}$, we have isolated and purified a membrane-bound cytochrome $\text{o}$. The cytochrome $\text{o}$, purified as a detergent (Triton X-100) and hemoprotein complex, contained 1.6 nmoles heme per mg of protein. Cold-temperature spectrum showed that no other cytochrome was associated with the purified preparation, and electrophoresis revealed that only one type of hemoprotein was obtained. The purified cytochrome $\text{o}$ reacted with both carbon monoxide and cyanide readily. Only in the reduced form did it combine with carbon monoxide, whereas the oxidized form reacted with cyanide. An “oxygenated” form of the cytochrome $\text{o}$ was demonstrated to be spectrally distinguishable from both the oxidized and the reduced forms.     

Nitrate reductase from Penicilliumchrysogenum: Kinetic mechanism at sub-optimum pH

The steady-state kinetics of the NADPH + FAD-dependent reduction of nitrate by nitrate reductase from $\text{Penicillium}\text{chrysogenum}$ was studied at pH 6.18. At this sub-optimum pH, V_max was about 83 units × mg protein^?1 compared with 225 units × mg protein^?1 at pH 7.20. All initial velocity reciprocal plot patterns at pH 6.18 as well as the NADP⁺/nitrate product inhibition pattern were intersecting. In contrast, the NADP(H)/nitrate plots at pH 7.20 were parallel (Renosto, F. $\text{et}\text{al.}$ J. Biol. Chem. $\text{256}$, 8616, 1981). A major effect of lowering the assay pH was to change the K_m for FAD from 0.17 μM at pH 7.20 to 4 μM at pH 6.18. The results suggest that nitrate reductase has a steady-state random kinetic mechanism in which k_cat in the forward direction at pH 7.20 (ca. 375 sec^?1) is greater that k_off for the dissociation of one or more substrates. Several observations suggest that k_off for FAD is extremely small at pH 7.20.     

Role of proteins and lipids in non-linear Arrhenius plots of Drosophila mitochondrial succinate-cytochrome c reductase studied by rebinding experiments

Abrupt changes in the Arrhenius activation energy of membrane-bound enzymes have often been correlated with changes in the physical state of membrane phospholipids. Similar changes in activation energy have also been found in soluble enzymes. The possibility exists, therefore, that in some of the membrane-bound enzymes the changes might reflect intrinsic changes of the proteins independent of changes in the membrane phospholipids. This hypothesis was investigated using Drosophila mitochondria isolated from wild type and the mutant Ocd^ts-1. In this mutant it has been shown that succinate-cytochrome $\text{c}$ reductase exhibits a change in Arrhenius activation energy at 18°C which is not found in the wild type (Sondergaard, L., Nielsen, N.C. and Smillie, R.M. (1975) FEBS lett. 50, 126–129). A quantitative thin-layer chromatographic analysis of mitochondrial phospholipids showed sphingomyelin to be more abundant in the wild type than in the mutant (5.2% and 4.3% of the total phospholipids, respectively). Since it was shown that the succinate-cytochrome $\text{c}$ reductase had a lipid requirement for full activity, reciprocal rebinding experiments were done. These experiments showed that the reconstituted membranes exhibited the change in activation energy at 18°C only when the protein moiety came from mutant mitochondria, that is, the change was independent of the source of the phospholipids used.     

Effects of Energy Substrates on Nitrate Reduction and Nitrate Reductase Activity in a Ruminal Bacterium, Selenomonas ruminantium

The factors affecting the rate of nitrate reduction and the nitrate reductase content in Selenomonas ruminantium were examined. The rate of nitrate reduction per cell mass was higher when S. ruminantium was grown on lactate than when grown on glucose, and the rate was further enhanced when grown on succinate. The nitrate reduction rate was parallel to the nitrate reductase content in cells, suggesting that the amount of nitrate reductase limits the rate of nitrate reduction. The amount of nitrate reductase was inversely related to growth rate. The growth rate was related to the level of intracellular ATP, which was inversely related to the levels of ADP and AMP. The ratio of NADH to NAD⁺was related to the rate of nitrate reduction and to the amount of nitrate reductase. From these results, it is conceivable that the synthesis of nitrate reductase is regulated in response to the sufficiency of energy and electron supply. Intracellular concentrations of adenine nucleotides and pyridine nucleotides may be the regulating factors. The amount of nitrate reductase was increased by the presence of nitrate, suggesting that the synthesis of nitrate reductase is enhanced by nitrate. In addition, nitrate reduction altered the fermentation pattern as a result of electron consumption.     

Adenine nucleotide extraction from multicellular organisms and beach sand: ATP recovery,energy charge ratios and determination of carbon/ATP ratios

Investigations were conducted comparing the efficiency of adenine nucleotide extraction from bacteria, unicellular algae, invertebrates (copepods, isopods and polychaetes), and beach sand using boiling buffers and cold acid extraction procedures. Cellular levels of ATP, ADP, and AMP obtained by these procedures were used to calculate the adenylate energy charge ratio ($\text{EC}{}_{\mathrm{<mtext>A</mtext>}}\text{= [}\text{ATP}\text{] +}\text{1}\text{2}\text{[}\text{ADP}\text{]/[}\text{ATP}\text{] + [}\text{ADP}\text{] + [}\text{AMP}\text{]}$). Although both extraction procedures efficiently extract ATP from unicellular micro-organisms, the results with multicells and beach sand indicate that the cold acid procedure preserves a greater percentage of the total adenine nucleotides ([A_T] = [ATP] + [ADP] + [AMP]) in the form of ATP, resulting in higher energy charge ratios. There were relatively large losses of ATP when multicellular organisms were extracted in boiling buffers. These data suggest that ATP hydrolysis may be important in certain fluid-solid mixtures, and also adds experimental support to the thermal gradient hypothesis.The C/ATP ratios calculated from these data indicate that multicellular organisms have C/ATP ratios < 100, as compared with the 250 ratio commonly found in micro-organisms. These results are discussed in terms of the proportion of structural (non-living) carbon vs protoplasm (living) carbon within each of these groups of organisms, as well as the relative intracellular levels of non-adenine nucleotide triphosphates. These differences in the C/ATP ratios must be considered whenever ATP measurements are used for biomass determinations.     

ATP/ADP exchange activity of gastric (H+ + K+)-ATPase

The ATP/ADP exchange is shown to be a partial reaction of the $\text{(}\text{H}{}^{\mathrm{+}}\text{+}\text{K}{}^{\mathrm{+}}\text{)-}\text{ATPase}$ by the absence of measurable nucleoside diphosphokinase activity and the insensitivity of the reaction to $\text{P}{}^1$, $\text{P}{}^5$ -di(adenosine-5′) pentaphosphate, a myokinase inhibitor. The exchange demonstrates an absolute requirement for Mg²⁺ and is optimal at an ADP/ATP ratio of 2. The high ATP concentration ($\text{K}{}_{0.5}\text{= 116 μ}\text{M}$) required for maximal exchange is interpreted as evidence for the involvement of a low affinity form of nucleotide site. The ATP/ADP exchange is regarded as evidence for an ADP-sensitive form of the phosphoenzyme. In native enzyme, pre-steady state kinetics show that the formation of the phosphoenzyme is partially sensitive to ADP while modification of the enzyme by pretreatment with 5,5′-dithiobis(2-nitrobenzoic acid) (DTNB) in the absence of Mg²⁺ results in a steady-state phosphoenzyme population, a component of which is ADP sensitive. The ATP/ADP exchange reaction can be either stimulated or inhibited by the presence of K⁺ as a function of pH and Mg²⁺.     

Transport of alpha-methyl glucoside in mutants of Escherichia coli K12 deficient in Ca2+, Mg2+-activated adenosine triphosphatase.

The initial rate of uptake of methyl α-D-glucopyranoside by $\text{Escherichia coli}$ is inhibited by respiration. The inhibition is more pronounced in mutant strains which cannot use the energy-rich state of the membrane to form ATP because of a defective Ca²⁺, Mg²⁺-activated ATPase. In both mutant and normal strains, the inhibition of glucoside uptake is not accompanied by an increase of the ATP content of the cells and is abolished by carbonyl cyanide $\text{m}$-chlorophenylhydrazone, a drug which dissipates membrane energy. It appears, therefore, that the inhibitory effect of respiration is mediated by the energy-rich state of the membrane and that ATP does not participate in the inhibition.     

On the regulation of histidinol dehydrogenase induction in Arthrobacter histidinolovorans

In order to investigate the control mechanism of histidinol dehydrogenase [HDH(I)] induction in $\text{Arthrobacter histidinolovorans}$, growth curves and induction experiments were carried out in presence of inhibitors of protein synthesis, namely chloramphenicol and actinomycin D. The evidence obtained from the gel electrophoresis patterns of the HDH activities in extracts of $\text{Arthrobacter}$ cultures suggest that HDH(I) induction is regulated at the protein synthesizing complex level rather than at mRNA synthesis. A working model is proposed to explain the mode of control of HDH formation in this bacterium, which involves stable messenger formation and post-translation control by histidinol.     

Molybdenum and chlorate resistant mutants in Escherichiacoli K12

Radioactive molybdenum is used to detect the existence of molybdo compounds in $\text{E.}\text{coli}$ K12. Three membrane bound Mo-proteins are found, using sodium dodecyl sulfate. One of them is the nitrate reductase. The nature of the other two is discussed. The soluble fraction of the cellular extract contains a small Mo binding molecule which could be peptidic in nature (MW is about 1,500). Different chlorate resistant mutants are analyzed on the basis of these molybdo-compounds. None of the mutants is found to contain radioactivity bound to nitrate reductase protein. Defects in the biosynthesis of a molybdenum coenzyme is deduced for chlorate resistant pleiotropic mutants.     

The role of molybdenum in formation of the NADPH-nitrate reductase by Aspergillus nidulans

Non-nitrate reducing mutants of $\text{Aspergillus}$$\text{nidulans}$ have been noted to produce either a nitrate inducible or constitutive NADPH-cytochrome $\text{c}$ reductase which resides in either a 4.5s or a 7.8s protein. The latter closely resembles the nitrate inducible, FAD dependent NADPH-nitrate reductase from the wild type. Measurement of flavin adenine dinucleotide (FAD) and molybdenum (Mo) in these two proteins revealed significant differences particularly in Mo. The concepts that a nitrate inducible $\text{nia}$ gene product constitutes the major flavin bearing component of the enzyme and that a constitutively produced $\text{cnx}$ gene product is implicated in formation of the larger Mo bearing multimer are further supported.     

Effect of N oxyanions on anaerobic induction of nitrate reductase in subcellular fractions of <Emphasis Type="Italic">Bradyrhizobium</Emphasis> sp. (Lupinus)

Anaerobic induction of nitrate reductase in subcellular fractions of Bradyrhizobium sp. strain USDA 3045 showed fivefold increase of the enzyme activity in spheroplasts, considered as the source of intact-membrane-bound nitrate reductase, within a 3 h time frame after nitrate addition. Such a dynamics was confirmed at the protein level, with antibodies specific to membrane-bound nitrate reductase. Nitrate reductase activity in the periplasm was one order of magnitude lower and significant only at initial 3 h of induction, within a narrow range of nitrate added. Nitrite induced the membrane-bound nitrate reductase at least 70% as effectively as nitrate, as judged from its activity pattern and Western blot analysis. The limited ability of Bradyrhizobium sp. to dissimilate ≥5 mM nitrate is not due to direct inhibition of respiratory nitrate reductase by accumulated nitrite. Moreover, a synergistic induction of membrane-bound nitrate reductase by nitrate and nitrite was indicated due to a twofold higher protein synthesis after simultaneous addition of these N oxyanions than when they were given separately.     

Microsomal benzo(a)pyrene hydroxylase in Aspergillus ochraceus TS: Assay and characterization of the enzyme system

Microsomal preparations of $\text{Aspergillus ochraceus}$ TS oxidised benzo(a)pyrene very efficiently in the presence of NADPH and O₂ and exhibits a pH optimum of 8.0–8.2. The hydroxylation is also effected in presence of NaI04. Hydroxylation was inhibited by metyrapone, SKF-525A, PCMB, imidazole, carbon monoxide and flavone but not by cyanide, azide and antimycin A indicating thereby the involvement of cytochrome P-450 in this reaction. Inhibition by cytochrome C is consistant with the participation of NADPH-cytochrome C reductase in this hydroxylation. Reduced microsomes and its solubilized preparation, when treated with carbon monoxide, showed absorption maxima at 453 and 449 respectively. Different classical inducers of cytochrome P-450 induce the benzo(a)pyrene hydroxylase activity to varying degree and as such suggests the existence of multiple forms of cytochrome P-450 in this fungus.     

Interaction between the nitrate respiratory system of Escherichia coli K12 and the nitrogen fixation genes of Klebsiella pneumoniae.

Hybrids were constructed between $\text{E. coli}$ K12 $\text{chl}$^? mutants defective in nitrate respiration and an F′ plasmid carrying nitrogen fixation genes from $\text{K. pneumoniae}$. Examination of these hybrids showed that expression of $\text{nif}$_Kp⁺ genes does not require a functional nitrate respiratory system, but that nitrate reductase and nitrogenase do share some Mo-processing functions. For nitrate repression of nitrogenase activity, reduction of nitrate to nitrite is not necessary, but the Mo-X cofactor encoded by $\text{chl}$ genes is essential. Nitrate probably inhibits nitrogen fixation by affecting the membrane relationship of the nitrate and fumarate reduction systems such that the membrane cannot be energized for nitrogenase activity.     

Photosynthetic electron transport,ATP synthesis and nitrogenase activity in isolated heterocysts of Anabaena cylindrica

Isolated heterocysts of the N₂-fixing blue-green alga Anabaena cylindrica contain the Photosystem I components P-700, bound and soluble ferredoxins and ferredoxin-NADP reductase. They also show Photosystem I activity being able to photoreduce both methylviologen and NADP when ascorbate+dichlorophenol-indophenol acts as reductant. They photophosphorylate (64 μmol ATP produced/mg chlorophyll $\text{a}\text{h}$) and carry out oxidative phosphorylation (8.7 μmol ATP produced/mg chlorophyll $\text{a}\text{h}$). Ninety per cent of the total cell-free extract nitrogenase activity is located in the heterocyst fraction of aerobic cultures.