Studies on soil fungi III. Seasonal variation and distribution of microfungi in some soils of Andhra Pradesh (India)

The seasonal variation and distribution of microfungi in four soil types collected from two districts of Andhra Pradesh (India) were studied.Besides soil type and surface vegetation, it appears from the present study that soil moisture, organic matter, potassium, calcium, iron and phosphorus contents also may affect the fungal numbers favourably, while chlorides, total soluble salts, total nitrogen and manganese contents may have an adverse effect.Even alkaline soils harbour greater numbers of fungi, but small fluctuations in the pH seem to influence the fungal numbers in soils inversely.A total of 101 species representing 43 genera were isolated. These included 18 Phycomycetes, 5 Ascomycetes, 72 Fungi Imperfecti, 5 Mycelia Sterilia and a single Myxomycete. The order of occurrence of the chief genera of fungi isolated wasAspergillus, Penicillium, Fusarium, Pythium, Curvularia, Phoma, Cunninghamella, Rhizopus, Alternaria andTrichoderma.A large number of genera and species were found common to the forest, maize field, garden and uncultivated soils; and the fungal flora was also not very much different from those recorded from various parts of the world.     

Studies on the mechanism of PMN activation III. by lymphokines

The influence of a guinea pig lymphokine preparation on the oxidative metabolism of human and guinea pig granulocytes of various sources was investigated. A dose-dependent increase of the oxidative burst following lymphokine challenge was observed. It occurred in unstimulated guinea pig peripheral polymorphonuclear leukocytes (PMN) and in prestimulated PMN obtained from the peritoneal cavity after glycogen injection as well. The lymphokine effect on the oxidative metabolism is not species-restricted because the guinea pig lymphokine preparation elicits an oxidative burst in human PMN, too. The increase caused by lymphokines is nearly of the same order of magnitude as that obtained with zymosan.     

In vitro activation of inactive nitrogenase component I with molybdate.

The mode of interaction in haploid Saccharomyces cerevisiae of two pso mutations with each other and with rad mutations affected in their excision-resynthesis (rad3), error-prone (rad6), and deoxyribonucleic acid double-strand break (rad52) repair pathways was determined for various double mutant combinations. Survival data for 8-methoxypsoralen photoaddition, 254-nm ultraviolet light and gamma rays are presented. For 8-methoxypsoralen photoaddition, which induces both deoxyribonucleic acid interstrand cross-links and monoadditions, the pso1 mutation is epistatic to the rad6, rad52, and pso2 mutations, whereas it is synergistic to rad3. The pso2 mutation, which is specifically sensitive to photoaddition of psoralens, is epistatic to rad3 and demonstrates a nonepistatic interaction with rad6 and rad52. rad3 and rad6, as well as rad 6 and rad52, show synergistic interactions with each other, whereas rad 3 is epistatic to rad52. Consequently, it is proposed that PSO1 and RAD3 genes govern steps in the independent pathways. The PSO1 activity leading to an intermediate which is repaired via the three incidence pathways controlled by RAD6, RAD52, and PSO2 genes. Since pso1 interacts synergistically with rad3 and rad52 and epistatically with rad6 after UV radiation, the PSO1 gene appears to belong to the RAD6 group. For gamma ray sensitivity, pso1 is epistatic to rad6 and rad52, which suggests that this gene controls a step which is common to the two other independent pathways.     

Studies on Cardiotonic Substances Produced by Microorganisms. (I)

The active substances such as cardiotonics or toxics which were produced in the cultured broths or contained in the mycellia of microorganisms were examined by Ito’s assay method for cardiotonica using the embryonic heart of Japanese killi-fish.

There were some strains obtained from actinomycetes whose cultured broths or methanol mycelial extracts showed these activities, but fewer from moulds, yeasts and bacteria.     

Aeromycology of Gorakhpur III. Seasonal variation in air fungal spora

The present paper deals with air fungal spora in different seasons of a year from January to December 1967. The maximum air fungal spora was obtained in winter season and minimum in hot dry months of summer. Different seasons exhibited different dominant fungal species. The air fungal population varied at three trapping periods i.e. 8 A.M., 1 P.M. and 6 P.M. in different seasons.     

Trypsin activation of inactive renin: plasma blanks and angiotensin I radioimmunoassay.

Divergent conclusions exist as to whether inactive renin is present in nephrectomized rat plasma. A major factor contributing to this conflict may be related to significant changes in the "plasma blank" when trypsin-treated plasma is subjected to angiotensin I (AI) radioimmunoassay (RIA). In normal, but not nephrectomized rat plasma, AI-like substances are present in direct proportion to active renin. These substances are destroyed by trypsin. However, trypsin generates additional AI-like material, in both normal and nephrectomized rat plasma. This material, which is present in proportion to the renin substrate concentration, does not appear to be tetradecapeptide (TDP). In normal plasma, however, exogenous TDP is converted to AI in proportion to the active renin concentration and AI generation from TDP is increased by activation of inactive renin. However, in nephrectomized rat plasma, no AI generation from TDP was evident either before or after trypsin treatment. The coincident tryptic generation of a substance that quenches the levels of AI detected by RIA, combined with significant changes in the levels of endogenous and trypsin generated AI-like substances, may have significant bearing on the measured levels of inactive renin.     

Synthesis and structural characterization of silver(I), aluminium(III) and cobalt(II) complexes with 4-isopropyltropolone (hinokitiol) showing noteworthy biological activities. Action of silver(I)-oxygen bonding complexes on the antimicrobial activities

Through two unequivalent oxygen donor atoms of the hinokitiol (Hhino; C10H12O2; 4-isopropyltropolone) ligand that showed noteworthy biological activities, the dimeric, silver(I)-oxygen bonding complex [Ag(hino)]2 1, the monomeric aluminium(III) complex [Al(hino)3].0.5H2O 4 and the cobalt(II) complex "[Co(hino)2]2.H2O" 6 were synthesized and characterized with elemental analysis, thermogravimetric and differential thermal analysis (TG/DTA), FTIR and solution (1H and 13C) NMR spectroscopy. The crystal structure of 1 was determined by Rietveld analysis based on X-ray powder diffraction (XPD) data and those of [Al(hino)3].MeOH 4a and [Co(hino)2(EtOH)]2 6a, being obtained as yellow block crystals and red platelet crystals, respectively, by crystallization of 4 and 6, were determined by single-crystal X-ray analysis. The antimicrobial activities of 1, 4 and 6, evaluated with minimum inhibitory concentration (MIC; microg ml(-1)), were compared with those of other metal complexes (M=Na, Li, Cs, Ca, V, Zn) with the hino- ligand. The antimicrobial activities observed in the alkali-metal salts strongly suggested that they were attributed to the effect of the anionic hino- species. The antimicrobial activities of 1 were significantly enhanced, whereas those of other metal complexes were suppressed, compared with those of the neutral Hhino and anionic hino- molecules. The antimicrobial activities observed in 1 were comparable with those of other recently found silver(I)-oxygen bonding complexes, the ligands of which had no activity. Thus, it is proposed that the antimicrobial activities of the silver(I)-oxygen bonding complexes are due to a direct interaction or complexation of the silver(I) ion with biological ligands such as protein, enzyme and membrane, and the coordinating ligands of the silver(I) complexes play the role of a carrier of the silver(I) ion to the biological system.     

Inhibition of hydrolytic enzymes by gold compounds. I. beta-Glucuronidase and acid phosphatase by sodium tetrachloroaurate (III) and potassium tetrabromoaurate (III)

Purified bovine liver beta-glucuronidase (beta-D-glucuronide glucuronohydrolase, EC 3.2.1.32) and wheat germ acid phosphatase (orthophosphoric monoesterphosphohydrolase, EC 3.1.3.2) were inhibited with freshly dissolved and 24 h aquated tetrahaloaurate (III) compounds. Rate and equilibrium inhibition constants were measured. From this data two acid phosphatases species were observed. Equilibrium inhibition constants ranged from 1 to 12.5 microM for the various gold compounds toward both enzymes. The first order rate constants ranged between 0.005 and 0.04 min.-1 for most reactions with the exception of the fast reacting acid phosphatase which had values as high as 2.6 and 2.8 min.-1. It is observed that the beta-glucuronidase is rapidly inhibited during the equilibrium phase before the more slower reaction covalent bond formation takes place. The acid phosphatases form the covalent bonds more rapidly, especially the faster reacting species suggesting a unique difference in the active site geometry to that of the more slowly reacting species. The tightly bonded gold (III)-enzyme complex is probably the reason for its toxicity and non-anti-inflammatory use as a drug.     

Exchange inert Co (III)-carboxypeptidase A: a catalytically inactive metallocarboxypeptidase.

Exposure of cobalt (II) carboxypeptidase A_α, [(CPD)Co(II)], to small molar excesses of the oxidizing agent m-chloroperbenzoate rapidly destroys (< 30 sec) both its peptidase and esterase activities in parallel. Concomitantly, the characteristic Co(II) electron paramagentic resonance (EPR) signal is abolished. [(CPD)Co(III)], isolated from the reaction mixture, has the same molecular weight and amino acid composition as [(CPD)Co(II)], contains 0.95 g-atom of Co and 0.01 g-atom of Zn per mole of protein, does not exhibit an EPR spectrum and is catalytically completely inactive towards both peptide and ester substrates. Identical treatment of the native zinc enzyme affects neither its catalytic activity nor its metal content. The reaction of m-chloroperbenzoate with [(CPD)Co(II)] follows saturation kinetics and is prevented by the inhibitor β-phenylpropionate. Furthermore, under the conditions found to oxidize [(CPD)Co(II)] effectively, there is no reaction with Co(II) $\text{E. coli}$ alkaline phosphatase. Thus, m-chloroperbenzoate has the characteristics of an active-site directed oxidizing reagent for [(CPD)Co(II)].     

Native arbuscular mycorrhizal fungi (AMF) from mountain grassland (Cordoba, Argentina) I. Seasonal variation of fungal spore diversity

Arbuscular mycorrhizal fungi (AMF) were studied in the rhizosphere of 3 Poaceae with metabolic pathway C(3) (Briza subaristata Lam., Deyeuxia hieronymi (Hack.) Türpe and Poa stuckertii (Hack.) Parodi), 2 Poaceae with C(4) metabolic type (Eragrostis lugens Nees and Sorghastrum pellitum (Hack.) Parodi.), and a Rosaceae (Alchemilla pinnata Ruíz & Pav.) from a natural mountain grassland in Central Argentina (South America). Host species, their metabolic type, seasonal changes, and grazing effects over AM fungal diversity were analyzed. Seventeen mycorrhizal fungi taxa were found, widespread in all families of Glomales. Density of endomycorrhizal fungi was found to be strongly influenced with seasons and host metabolic pathway, although biodiversity (H), richness (S) and evenness (E) did not change. In most cases grazing did not affect these variables.