The relationship of hydrogen peroxide to the inhibition of the glyoxalase activity of intact erythrocytes by x-radiation

The x-irradiation of a dilute suspension of erythrocytes results in a decrease in the glyoxalase activity of the cells as a result of a fall in the reduced glutathione level. The present paper deals with the possible role of H₂O₂ in this reaction. The addition of intact erythrocytes to physiological saline previously irradiated with 150,000 r or 225,000 r results in a fall in the glyoxalase activity of the cells. The inhibition is prevented by the preincubation of the irradiated saline with catalase and is reversed by the addition of plasma, glucose, adenosine, and inosine to the cell suspension. An inhibition of the glyoxalase activity is also produced by the addition of H₂O₂ to the suspension of erythrocytes. The inhibitory effect of H₂O₂ can be prevented and largely reversed by plasma, glucose, adenosine, and inosine. Methylglyoxal is also protective under these conditions. Hydrogen peroxide formed continuously and in low concentrations by enzyme systems appears to be more effective than added H₂O₂ in inhibiting the glyoxalase system. The inhibition by H₂O₂-producing enzyme systems is minimized by the addition of catalase, plasma, glucose, methylglyoxal, and to a lesser extent, by adenosine and inosine, and is accentuated by the addition of sodium azide. The results are discussed in relation to the role of H₂O₂ and catalase in the toxicity of ionizing radiations.     

Alteration of the rate of cell division independent of the rate of DNA synthesis in a mutant of Salmonella typhimurium

Summary Salmonella typhimurium strain IIG has a temperature—sensitive DNA synthesis initiation apparatus and completes rounds of DNA replication when shifted to 38°. At this temperature there is a period of apparently normal division followed by a second phase in which DNA-less cells are produced. The rate of division in this second phase can be markedly increased if a culture growing in MM is shifted to nutrient broth at the time of the temperature shift. The extra divisions induced by the nutritional shift are not due to extra replication forks being introduced by this process nor to the rapid growth of ts ⁺ revertants. It is concluded that in this strain at 38°, the rate of division can be increased without altering the rate of DNA synthesis. The extra divisions induced by the shift-up do not take place for about 90 min. The possible occurrence of such a period between the triggering of division and the division event in normal cells is discussed.     

Regulation of the formation of protease inBacillus megaterium

Protease is synthesized by the cultures growing in a glucose-containing mineral medium. However, it is formed even during incubation of the washed cells in a nitrogen free medium. The enzyme synthesis is decreased substantially by the addition of the individual amino acids or their mixture. Threonine, isoleucine, leucine and valine are the most inhibitory. Arginine, cysteine, glycine, lysine and tryptophan in concentrations of 10³ m do not inhibit the production of protease. The growth of the culture is also somewhat inhibited by threonine and isoleucine, the repression of protease being, however, much higher. Concentrations of 10³ m inhibit its synthesis by 80–90%. However, the enzyme activity is not influenced. The inhibition is caused byl,-isomers. Repression of the enzyme synthesis after the addition of threonine into the medium is much greater in a growing culture than in a culture starving in a nitrogen-free medium. However the level of free threonine in the pool is roughly the same in both growing and non-growing cultures. A mixture of 13 amino acids, which themselves are little inhibitory, suppresses the synthesis of protease much more than threonine or isoleucine. The inhibitory effect of the individual amino acids on the enzyme formation is apparently additive.     

Components of error in predictions of species compositional change

Abstract. A method is given for measuring two components of error (rate and direction) in predictions of compositional change through time. Observed compositional change between two times can be represented as a vector between two points in multidimensional species space. The point at the tail of this vector is the species composition at one particular time. A vector of predicted compositional change will diverge from the vector of observed change to some degree. The error in the predicted rate of change is measured by the difference between the lengths of the two vectors. The error in the predicted direction of change is measured by the angle between the vectors. The cosine of this angle is a non-standardized correlation coefficient (r_n) between the predicted and observed species compositions. The quantity 1 - r_n² measures the error in direction of the predicted dynamics without being influenced by the overall rate of change. These measures in Euclidean space have useful counterparts in city-block space. The method is illustrated by comparing actual long-term changes in Midwestern old-growth forests with the changes predicted by a growth and yield model, TWIGS.     

A further study of the fine structure and membrane properties of neuroglia in the optic nerve of Necturus

The optic nerve of Necturus maculosus consists of a homogeneous population of astroglia and bundles of unmyelinated axons. The glial cell processes ramify within the nerve roughly delineating fascicles of axons and come together at the periphery to form a complete external limiting membrane interrupted only by narrow clefts between adjacent processes. They are frequently “attached” to one another, forming specialized junctions. Blood vessels are entirely outside the nerve which is surrounded by a basal lamina. The temperature dependence of the glial membrane potential is accurately predicted by the Nernst relation. The membrane potential is unaffected by changes in Cl, Na, Li, and guanidinium which are apparently impermeant. The permeability of the glial membrane to other cations is in the sequence Tl> K> Rb> Cs> NH₄. This suggests that the chemical nature of the site of potassium permeability in glial cells is similar to that in the neuron.     

Ultrastructure of the Eyespot and its Possible Significance in Phototaxis of Tetracystis excentrica*†

SYNOPSIS. The eyespot of the zoospore of Tetracystis excentrica (a green alga) has been studied by light and electron microscopy. In Tetracystis the eyespot consists of about 110 osmiophilic granules which form a plate in the anterior third of the cell. The granules are about 80 Å in diameter and are found in the outermost portion of the chloroplast; they commonly show hexagonal close packing and a hexagonal shape. The granules are confined positionally by the chloroplast envelope and an inner thylakoid. The plasmalemma over the eyespot is thickened and is separated from the chloroplast envelope by a 50 mμ space. The eyespot of Tetracystis is compared with others reported in the literature and the possible functional significance of these studies is discussed. The possibility that the eyespot plate in Tetracystis serves as a shading device rather than the primary photoreceptor is considered.     

In vitro activation of a galactosyl transferase involved in the osmotic regulation of ochromonas

Osmotic regulation in the flagellate Ochromonas malhamensis Pringsheim is mainly mediated by fluctuations in the pool size of α-galactosyl-(1→1)-glycerol (isofloridoside). A regulated key enzyme of isofloridoside metabolism is the galactosyl transferase producing isofloridoside phosphate. The activity of this enzyme in crude extracts can be increased 5- to 20-fold by incubation at pH 6. The activation occurs in a reaction with a Q₁₀ of 1.5 to 3 and is dependent on time and pH value. Inactivation of the activated form of the enzyme is also time-dependent, and is minimal at the pH value at which activation is optimal. The data suggest a regulation of the enzyme by chemical modification due to the action of auxiliary enzymes.     

Mechanism of action of chalcone isomerase

The pH profile of the rate of isomerization of 4,2′,4′-trihydroxychalcone catalyzed by chalcone isomerase shows dependence on the basic form of a group with a pK of 7.25. The same pH dependence is seen for the reverse reaction. Enzyme activity is lost in the presence of diethylpyrocarbonate at pH 6.0. In the presence of 20% formamide in imidazole buffers, the pK for the forward reaction is modified by a second pK of 7.1. This behavior represents a perturbed pK of a neutral acid group and is attributable to the 2′ hydroxyl of the chalcone substrate. These results suggest a mechanism of enzyme action involving nucleophilic addition of an imidazole group in the active site to the double bond followed by nucleophilic attack by the 2′ phenolate group, resulting in ring closure with inversion of configuration at C-2.     

Solubility Improvement of Drugs using N-Methyl Pyrrolidone

The solubilization efficiency of N-methyl pyrrolidone (NMP) has been determined and compared to that of ethanol and propylene glycol for 13 poorly soluble drugs. NMP is found to be a more efficient solubilizer for all the drugs studied. The solubility enhancement as high as about 800-fold is obtained in 20% v/v NMP solution as compared to water. The mechanism of drug solubilization by NMP has also been investigated. It is proposed that NMP enhances drug solubility by simultaneously acting as a cosolvent and a complexing agent. A mathematical model is used to estimate the drug solubility in NMP–water mixture, according to which the total solubility enhancement is a sum of the two effects. This model describes the experimental data well and is more accurate than other models. A large and uniform reduction in the surface tension of water as a function of NMP concentration demonstrates its cosolvent effect. The complexation is supported by the fact that it’s strength is affected by the temperature and the polarity of the medium. A strong correlation exists between log K _ow of the drugs and the cosolvency coefficients. The correlation between log K _ow and the complexation coefficients is weak suggesting that factors such as molecular shape and aromaticity of the drug molecule are significant in determining the complexation strength. This has been confirmed by the absence of a significant complexation between NMP and linear drug-like solutes.     

Anionic modulation of the catalytic activity of hydrogenase from Chlamydomonas reinhardtii

Hydrogen production by cell-free extracts of Chlamydomonas reinhardtii is stimulated by anions when methyl viologen, reduced by dithionite, is used as the electron donor to hydrogenase. The increasing effectiveness of various anions closely follows their position in the Hofmeister chaotropic sequence. The most stimulatory anion tested, I^?, gives a six-fold increase in activity at a concentration of 0.5 n. The K_m of the enzyme for methyl viologen is not affected by anions, while the V is greatly increased. H₂ oxidation coupled to methyl viologen reduction is also greatly stimulated by anions. However, when reduced ferredoxin is used as the electron donor to hydrogenase, there is a very strong inhibition of H₂ production by salts. In this case, the V of the enzyme is unaffected, but there is a large increase in the K_m of the enzyme for ferredoxin. The most inhibitory salt tested, KI, decreases hydrogenase activity by 93% at a concentration of 0.2 n.     

Regulation of DNA synthesis in mouse macrophages. II. Studies on mechanisms of action of the macrophage growth factor

When mouse macrophages are incubated with medium conditioned by mouse fibroblasts, they are induced to synthesize DNA and divide. This phenomenon is triggered by a macrophage growing factor (MGF) released by the fibroblasts. The presence of a serum cofactor is essential to the activity of the MGF; this cofactor can be removed by dialysis and seems unrelated to the “growth-promoting substances” normally present in serum. The kinetics of DNA synthesis in macrophages stimulated by conditioned medium (CM) is characterized by a lag phase of 24–48 h and a peak synthesis at 4–5 days, followed by a rapid decrease. This decrease is caused by depletion of the MGF from the CM by the growing macrophages.     

Inotropism and Contracture of Aplysiid Ventricles as Related to the Action of Neurohumors on Resting and Action Potentials of Molluscan Hearts

The postsynaptic actions of neurohumors on molluscan musclemay be exerted through control of force as well as by meansof excitation and inhibition. The control of force may appearas potentiation of the response to excitation, as increasedinotropism in spontaneous contractions, or as an increase intonus. We have directed our attention to the alterations offorce induced in aplysiid ventricles by applied postulated neurohumors.The results are interpreted in terms of the known effects ofneurohumors on resting potential and action potentials of molluscanhearts. We recorded compound membrane potentials of aplysiidventricles extracellularly, using a single sucrose gap apparatustogether with a force-displacement transducer to measureforcein contractions or contracture. Aplysia californica ventriclehas a membrane potential of –52.5 ± 9.4 mV. Ventriclesof Aplysia dactylomela or Aplysia californica are depolarizedby increased concentrations of external potassium ion, withan accompanying contracture. After incubation in calcium-freemedium, KCl contracture-force is directly dependent on calciumion concentration. A depolarization of 8.3 ±2.14 mV inpotassium-free medium is blocked by substitution of lithiumfor sodium in the medium, suggesting an electrogenic sodiumpump. There is a sustained depolarization in low chloride medium,which suggests a significant chloride contribution to the restingpotential. Ventricles of Dolabella auriculana or Aplysia dactylomelaare depolarized by acetylcholine (ACh). Threshold for depolarizationis lower than threshold for contracture-force. The ventricleof A. dactylomela is depolarized by 5- hydroxytryptamine (5HT)with threshold at 10^–9 M and a maximum depolarizationof 30 mV at 10^–4M. Depolarization by 5HT may induce beatingbut does not induce contracture. Ventricles of Aplysia californicaare not depolarized by ACh although beating ventricles are inhibited,and a depolarized ventricle in a tonic contracture may be hyperpolarizedand relaxed by low concentrations. The force of contractionof the ventricle of Dolabella auricularia is dependent on theduration of the plateau phase of the cardiac action potential.The plateau is lengthened by 5HT with an accompanying increasein force of beat, and shortened by ACh, with an accompanyingdecrease in force of beat. The action potential in the ventricleof Aplysia californica is not differentiated into spike andplateau phases, and neither ACh nor 5HT has any marked effecton the form of the action potential. Nevertheless, isolatedventricles of Dolabella auricularia, Aplysia dactylomela, andAplysia californica are all excited by 5-hydroxytryptamine,with a threshold at about 10^–M. Both spontaneous beatingand excitation induced in A. californica ventricles by 5HT areblocked by lack of the sodium ion, which may be responsiblefor pacemaker potentials in molluscan hearts.     

Fluoride Inhibition of Respiration and Fermentation in Cultured Cells of Acer pseudoplatanus

Low concentrations of sodium fluoride severely inhibit anaerobic CO₂ evolution in Acer pseadoplatanus L. cells but have relatively little effect on aerobic respiration. The insensitivity of respiratory O₂ uptake to fluoride is due in part to the fact that fluoride reduces the intracellular pyruvate concentration to only a relatively minor extent under aerobic conditions, although it prevents the several fold increase in endogenous private which is normally brought about by anoxia. The respiratory insensitivity is also ascribable to the existence of a respiratory component which is unaffected by the decrease in endogenous private resulting from fluoride treatment. The extremely severe respiratory inhibition brought about by fluoride plus dinitrophenol is not appreciably relieved by exogenous private, indicating that this inhibition is the result of interference with the aerobic oxidation process per se and is not solely a consequence of glycolytic inhibition.     

The glucose-dependent transport of l-malate in Zygosaccharomyces bailii

Zygosaccharomyces bailii possesses a constitutive malic enzyme, but only small amounts of malate are decomposed when the cells ferment fructose. Cells growing anaerobically on glucose (glucose cells) decompose malate, whereas fructose cells do not. Only glucose cells show an increase in the intracellular concentration of malate when suspended in a malate-containing solution. The transport system for malate is induced by glucose, but it is repressed by fructose. The synthesis of this transport system is inhibited by cycloheximide. Of the two enantiomers l-malate is transported preferentially. The transport of malate by induced cells is not only inhibited by addition of fructose but also inactivated. This inactivation is independent of the presence of cycloheximide. The transport of malate is inhibited by uranyl ions; various other inhibitors of transport and phosphorylation were of little influence. It is assumed that the inducible protein carrier for malate operates by facilitated diffusion. Fructose cells of Z. bailii and cells of Saccharomyces cerevisiae do not contain a transport system for malate.This research was supported in part by a grant from the Forschungsring des Deutschen Weinbaus.     

The reversible phosphorylation of isocitrate dehydrogenase of Salmonella typhimurium

The 46,000 dalton phosphoprotein in Salmonella typhimurium is isocitrate dehydrogenase, an enzyme at the branch point between the glyoxylate and Krebs cycle pathways. The enzyme is phosphorylated by a kinase which is controlled by growth conditions; and it is dephosphorylated by a phosphatase. Acetate, ethanol, α-methylglucoside, and deoxyglucose cause an activation of the phosphorylation reaction in intact cells. A number of other compounds are found to affect the kinase and phosphatase activities. The reversible phosphorylation of isocitrate dehydrogenase plays a major role in the control of the Krebs cycle and glyoxylate pathways.     

Chloride dependence of the K+-stimulated release of taurine from synaptosomes

Exposure of a crude synaptosomal fraction to K⁺ concentrations ranging from 25 to 100 mM evokes the release of [³H]taurine and [³H]GABA. These high concentrations of K⁺ induce, besides depolarization, a marked synaptosomal swelling, which is prevented by replacing chloride in the solutions with the largely impermeant anion gluconate. The depolarizing effect of K⁺ is unaffected by omission of chloride. The K⁺-evoked release of taurine seems related to K⁺-induced changes in synaptosomal volume rather than to a depolarizing effect, since it is totally calcium-independent but is abolished by reducing chloride and by making solutions hypertonic with mannitol. The release of [³H]GABA, in contrast is unaffected in chloride-free or hypertonic solutions.     

Kinetics of photosynthetic membrane protein assembly in Rhodopseudomonas spheroides

Glycogen phosphorylase in cell-free extracts of Neurospora crassa is activated 10- to 15-fold by incubation with MgATP^2?. When the MgATP^2? is removed, the active form (a form) reverts to the inactive form (b form). The inactivation requires Mg²⁺ and is inhibited by NaF. The results confirm that Neurospora crassa glycogen phosphorylase exists in two interconvertible forms and strongly suggests that the interconversion is catalyzed by a kinase and phosphatase. The a form was partially purified. The enzyme has a molecular weight of 320,000. Uridine diphosphate glucose is a linear competitive inhibitor with respect to glucose-1-phosphate and a linear non-competitive inhibitor with respect to glycogen. Glucose-6-phosphate is a hyperbolic (partial) noncompetitive inhibitor with respect to all substrates in both directions. The b form of the enzyme in crude cell-free extracts is stimulated 2- to 3-fold by 5′-AMP. As the b form is purified, the 5′-AMP activation is diminished. The molecular weight of the partially purified “b” form was also 320,000.     

Citrate Synthase of Plants: Sensitivity to Sulfhydryl Reagents and Molecular Weight of the Enzyme

Citrate synthase of wheat (Triticum aestivum L.), bean (Phaseolus vulgaris L.), cauliflower (Brassica oleracea L.), and a marine blue-green alga (Coccochloris elabens) is inhibited by sulfhydryl binding reagents. The inhibitions are partially reversed by dithiothreitol. Pig heart citrate synthase is only slightly inhibited by the same reagents and this is completely reversed by dithiothreitol. All citrate synthases in this study are inhibited by adenosine triphosphate. The inhibition is relieved by increasing the concentration of acetyl coenzyme A. Citrate synthase of wheat, cauliflower, bean, and pig heart was estimated by gel filtration to have a molecular weight of 100,000 daltons. The Coccochloris citrate synthase was estimated to have a molecular weight greater than 250,000 daltons. The evolutionary implications of these findings are discussed. This enzyme is comparable in size to the 100,000 dalton mammalian enzyme (Singh et al. 1970) making it somewhat larger than the 65,000 dalton mango enzyme (Srere et al. 1971). The PHMB-treated enzyme also shows changes in its electrophoretic properties (Greenblatt and Sarkissian unpublished). The evidence presented here demonstrates that citrate synthase of various plants is sensitive to sulfhydryl reagents suggesting that sulfhydryl reactivity is a not unusual property of plant citrate synthase. In addition we show that molecular weight as large as or larger than that reported in microbial systems can occur in a blue-green alga.     

The morphology of the apical organ and adjacent epithelium of pilidium prorecurvatum, a pelagic larva of an unknown heteronemertean (Nemertea)

The morphology of pilidia ex gr. recurvatum from Peter the Great Bay (Sea of Japan) was studied by confocal laser scanning and transmission-electron microscopy. The studied pilidium larvae differ from pilidium recurvatum in lacking a posterior ciliary ring and by the presence of a caudal tuft. On this basis, pilidium prorecurvatum is proposed as a new name for the lavae. The apical organ of pilidium prorecurvatum is represented by a thickened epithelium, which consists of uniform columnar monociliary collar cells and is innervated by a pair of serotonergic intraepithelial neurons. The bodies of the serotonergic neurons are located outside of the apical organ, but occasional axons were found at the organ base. The rest of the pilidial epithelium is represented by flattened polygonal multiciliated cells with sparse microvilli; the bodies of two neurons lie in the helmet epithelium immediately adjacent to the apical organ. Morphologically, the apical organ of the pilidium corresponds well to that of other lophotrochozoan larvae, but their homology remains unclear.