On the action of sulfanilamide

Summary A. According toMellon,Locke andShinn, the bacteriostatic action of sulfanilamide is due to the inactivation of (bacterial) catalase and the resulting accumulation of hydrogen peroxide. The probability of this theory is discussed. B. Catalase activity was studied by means ofPhotobacterium Fischeri, as an oxygen indicator. By adding hydrogen peroxide to the tested cultures of bacteria it has been demonstrated, that: I.Bacterium coli, Photobacterium Fischeri andStreptococcus haemolyticus (strainAronson) contain catalase. II. Sulfanilamide does not inactivate the catalase in blood. III. Sulfanilamide does not inactivate bacterial catalase nor does it affect the production of catalase in the growing culture containing the drug. So we have to conclude that the assumption of catalase inactivation to be the essential factor in sulfanilamide action on bacteria will not lead us to the solution of the problem. First communication:L. K. Wolff andH. W. Julius, Ann. de l'Inst. Pasteur62, 616, 1939.     

Some Notes on Fluorescence Intensity

The fluorescent emission spectra for 5 × 10^-6 M p-aminohippuric and p-aminobenzoic acids in mixtures of methyl alcohol and 1,2-propanediol have been determined. The results indicate that at almost invariant dielectric constant the quantum yield of fluorescence is a function of the viscosity of the solvent. The suggestion is made that a collisional quenching mechanism, which involves the rotational diffusion of solvent molecules, is significant in solutions of low viscosity and less so at high viscosities. A prediction, on the basis of the proposed mechanism, of augmentation of the emission spectra of p-aminohippuric acid, after binding to homologous antihapten antibody, is confirmed. A small red shift is also noted at higher viscosities in protein-free solutions or after binding to homologous antibody. It is suggested that, contrary to some interpretations in the literature, a red shift and/or an augmentation of quantum yield of fluorescence may, in specific instances, not be significant of a transfer of the fluorochrome to an environment of lower dielectric constant.     

Unequivocal evidence in support of the nonenzymatic redox coupling between glutathione/glutathione disulfide and ascorbic acid/dehydroascorbic acid.

Experiments were performed to evaluate the nonenzymatic reaction between glutathione (GSH) and dehydroascorbic acid (DHA). Though both ascorbic acid and glutathione disulfide (GSSG) are formed from this reaction, previous work has focused almost exclusively on measurements of ascorbic acid. In contrast, there is very little information about the formation of GSSG under the same conditions as those used to produce ascorbic acid. The emphasis on ascorbic acid stems from the fact that a spectrophotometric technique is available for its measurement, whereas 1H-NMR or an amino acid analyzer has been used to measure GSSG. The present experiments use a simple, rapid method for accurately and precisely measuring the concentrations of GSSG in a solution. The spectrophotometric (340 nm) procedure uses NADPH and glutathione reductase; analysis time is very short, many replicate samples can be tested and as little as 0.05-0.1 mM GSSG can be detected. Using this method, it is shown that there is an equimolar production of GSSG and ascorbic acid from GSH and DHA and that the decrease in GSH is stoichiometrically related to the increase in the concentration of GSSG. The present findings provide additional insight into the interaction between the GSH/GSSG redox couple and the ascorbic acid/DHA redox couple.     

Sulfhydryl Groups Modulate the Allosteric Interaction Between Glycine Binding Sites at the Inhibitory Glycine Receptor

We have investigated the effect of chemical reagents that modify sulfhydryl groups on the ligand binding properties of the glycine receptor (GlyR). The Hill coefficient (nH) for the displacement of [3H]strychnine binding by glycine was increased from approximately 0.8 to values significantly above 1 (approximately 1.2-1.4) in membranes pretreated with the disulfide-reducing agent dithiothreitol or glutathione. However, the affinity of strychnine or glycine for the GlyR was not affected by these treatments. This indicates that several glycine binding sites interact cooperatively for displacing bound strychnine under such experimental circumstances. A similar increase in the nH for glycine has been observed when the temperature of the binding assay was increased to 37 degrees C. Combination of dithiothreitol pretreatment and increased binding temperature led to nH variations similar to those observed with either of these treatments alone, a finding suggesting that their mechanisms of action are not independent. Conversely, modification of rat spinal cord membranes or of purified and reconstituted GlyR preparations with the sulfhydryl-alkylating agent N-ethylmaleimide or fluorescein-maleimide decreased nH values to approximately 0.5, without affecting glycine or strychnine affinities. This effect may be caused by an increased heterogeneity of GlyR populations. It is interesting that occupancy of the receptor by glycine or beta-alanine (but not by antagonists) specifically protects from the effects of the different sulfhydryl reagents. Moreover, the presence of some of the Eccles' anions, i.e., anions that permeate through the channels associated with GlyRs and gamma-aminobutyric acidA receptors, seems to be required for the action of both dithiothreitol and N-ethylmaleimide.(ABSTRACT TRUNCATED AT 250 WORDS)     

Mendel's experiments: A reinterpretation

Conclusion My conclusion is that Mendel deliberately, though without any real falsification, tried to suggest to his audience and readers an unlikely and substantially wrong reconstruction of the first and most important phase of his research. In my book I offer many reasons for this strange and surprising behavior,⁵³ but the main argument rests on the fact of linkage. Mendelian genetics cannot account for linkage because it was based on the idea of applying probability theory to the problem of species evolution. Central to the theory is the law of probability according to which the chance occurrence of a combination of independent events is the product of their separate probabilities. This is the common basis of Mendel's first and second laws, but this is why Mendel's second law on independent assortment is enunciated in too general a way. From Morgan's work we now know that characters may not always be independent if their genes are located very close one to the other on the same chromosome. And this was also the basis of Mendel's personal drama: he surely observed the effects of linkage, but he had no theoretical tools with which to explain it. So he presented his results in a logical structure consistent with the central idea of his theory. Had he described the real course of his experiments he would have had to admit that his law worked for only a few of the hundreds of Pisum characters — and it would thus have been considered more of an exception than a rule. This is why he insisted on the necessity of testing the law on other plants, and this is why in his second letter to Carl Nägeli he admits that the publication of his data was untimely and dangerous.⁵⁴.We can argue that already in 1866 Mendel was less confident that his so-called second law had the same general validity as the first — and that later he lost his confidence altogether. Contemporary testimony indicates that in the end he became as skeptical as all his contemporaries as to the scientific relevance of his theory.⁵⁵ But he was wrong. His research is in no way the fruit of methodological mistakes or forgery, and it remains a landmark in the history of science. He was only the victim of a strange destiny in which the use of probability theory was responsible, at the same time, for the strength and for the weakness of his theory. We must still consider him the father and founder of genetics.     

Modelling of cyclic fed-batch plus batch polygalacturonase production by Aureobasidium pullulans on raw orange peel

Summary Cyclic fed-batch plus batch polygalacturonase production by Aureobasidium pullulans in slurry fermentation systems using raw orange peel as substrate was studied in a 3-dm³ stirred fermentor by setting the main operating variables (T=297°K; pH₀=3.2; OP₀=3% w/v; n=700 rpm) to optimal values determined previously. In this way, it was possible to stabilize enzyme excretion at 130–140 VU cm^–3. The time course of this fermentation process in terms of cell growth, substrate consumption and enzyme synthesis was reconstructed with a mean standard error less than 10%, by applying an unstructured model set up in a batch run and further refined in a series of cyclic fed-batch plus batch operations. In particular, the enzyme formation rate was related to the effect of reducing sugars as inhibitors at higher concentrations and as activators at lower levels by using an exponential equation. Moreover, the consumption rate of reducing sugars was found to be linearly related to the cell growth rate, its specific date being of pseudo-first order with respect to the reducing sugar concentration.Offprint requests to: M. Moresi     

Identification and initial topological analysis of the Rickettsia prowazekii ATP/ADP translocase.

The Rickettsia prowazekii ATP/ADP translocase was identified by sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis (PAGE) and immunoblot analysis using antibodies raised against a synthetic peptide corresponding in sequence to the carboxyl-terminal 17 amino acids of the carrier. Both the translocase of R. prowazekii and that expressed by Escherichia coli transformants containing the rickettsial gene had an apparent molecular mass of 36,500 Da by SDS-PAGE analysis, a mass considerably less than that deduced from the sequence of the gene. The SDS-solubilized translocase aggregated upon heating at 100 degrees C in the presence of disulfide bond-reducing agents. Similar concentrations of disulfide bond-reducing agents inhibited the exchange transport of adenine nucleotides by both R. prowazekii and translocase-expressing E. coli. These data suggested that an intramolecular disulfide bond in the translocase was essential for transport activity. The antipeptide antibodies used for identification of the translocase bound preferentially to inside-out membrane vesicles of translocase-expressing E. coli relative to right-side-out spheroplasts, thus indicating that the carboxyl terminus of the carrier is located on the cytoplasmic side of the bacterial inner membrane. Protease studies were unable to localize the carboxyl terminus because of the resistance of this region of the native translocase to proteolytic cleavage. These data in conjunction with hydrophobicity analysis were used to construct an initial topological model of the translocase within the cell membrane.     

Microhabitat selection of ostracods in relation to predation and food

Experiments with the cyprinid fishVimba vimba as predator and the ostracodsCypridopsis vidua, Darwinula stevensoni andCytherissa lacustris as prey show that conspicuous coloration enhances predation risk for the ostracods. When the ostracods are allowed to retreat into sediment, risk is markedly reduced. ostracods show clear microhabitat preferences which are influenced by habitat structure and food supply. Exposed plant surfaces are visited only if they bear food and if the ostracods are not satiated.