Publications
| Title | Abstract | Year Filter | PMID(sorted descending) Filter |
|---|
| in vitro studies on a proteolytic enzyme from aspergillus oryzae (protease i). | 1968 | 4231457 | |
| [extracellular leucine aminopeptidases (ec 3.4.1.1) of aspergillus oryzae (ip 410). glycoprotein nature of the fraction leucine aminopeptidase 1]. | 1974 | 4219346 | |
| [products of proteolysis obtained with the use of complex enzyme preparations at different ph values]. | 1974 | 4219043 | |
| [demonstration of extracellular leucine aminopeptidases (ec 3.4.1) of aspergillus oryzae (ip 410). study of the leucine aminopeptidase 2 fraction]. | 1974 | 4212604 | |
| alpha-d-fucosidase from aspergillus oryzae: characterization of alpha-d-fucosidase with alpha-d-galactosidase activity. | 1973 | 4198930 | |
| the purification and properties of an extracellular protease from aspergillus oryzae nrrl 2160. | 1973 | 4197025 | |
| dynamics of amylolytic enzymes synthesis in aspergillus oryzae. | 1966 | 4161862 | |
| [experimental and clinical studies on a protease from aspergillus oryzae (brinase): fibrinogen turnover, thrombocyte aggregation and occlusion of the scribner shunt]. | 1974 | 4134482 | |
| review of the biochemistry and coagulation physiology of brinolase. (fibrinolytic enzyme from aspergillus oryzae). | 1974 | 4134481 | |
| clinical review on brinase, a protease from aspergillus oryzae. | 1974 | 4134258 | |
| on the pharmacology of brinases, a proteolytic enzyme from aspergillus oryzae. | 1974 | 4134257 | |
| specificity of the dna product of rna-dependent dna polymerase in type c viruses. ii. quantitative analysis. | a number of mammalian type c viruses were analyzed for relatedness by the technique of dna.rna hybridization. viral dnas were prepared in single-stranded form from complexes with 70s viral rna formed during endogenous polymerase reactions. extent of hybridization was assayed with the single-strand nuclease (s-1) from aspergillus oryzae. results obtained indicated a high degree of viral specificity, with significant cross-reactions being observed only with viruses obtained from within a species, ... | 1973 | 4129928 |
| properties of proteases from aspergillus oryzae and aspergillus flavus. a comparative study. | 1971 | 4108471 | |
| heterokaryosis between aspergillus oryzae cyclopiazonic acid-defective strains: method for estimating the risk of inducing toxin production among cyclopiazonic acid-defective industrial strains. | aspergillus oryzae strains are used extensively in the food industry. some of these strains excrete alpha-cyclopiazonic acid (cpa), a mycotoxin which may provoke toxicoses in rats. physicochemical methods may reveal the presence of this toxin, but they are inadequate to screen cpa-nonproducing (cpa-) strains. cpa production is revealed by either bacterial growth inhibition or alkalinization of the culture medium. this first biological property was used to devise a time-saving screening method to ... | 1985 | 4083874 |
| antifungal properties of 3-n-alkyn-1-ols and synergism with 2-n-alkyn-1-ols and ketoconazole. | twelve 3-n-alkyn-1-ols (c4-c12, c14, c16, and c18) were tested against aspergillus oryzae, aspergillus niger, trichoderma viride, and myrothecium verrucaria in sabouraud dextrose agar at ph 5.6 and 7.0. toxicity to candida albicans, candida tropicalis, trichophyton mentagrophytes, and mucor mucedo was determined in the same medium at ph 5.6 and 7.0 in the absence and presence of 10% beef serum. fungitoxicity was strongly influenced by chain length, slightly by ph of the medium, and significantly ... | 1985 | 4020633 |
| a novel enzyme producing isoprimeverose from oligoxyloglucans of aspergillus oryzae. | an enzyme producing isoprimeverose from xyloglucan fragment oligosaccharides has been purified to the electrophoretically pure state from a commercial enzyme preparation of aspergillus oryzae (sanzyme 1000). the purified enzyme showed approximately 1,280-fold increase of the specific activity over the original preparation. the purified enzyme was shown to be an oligomeric protein consisting of two subunits, each of which had a molecular weight of 115,000. the enzyme showed the highest activity a ... | 1985 | 4019436 |
| the subsite structures of guanine-specific ribonucleases and a guanine-preferential ribonuclease. cleavage of oligoinosinic acids and poly i. | in order to estimate the size of the active site of guanylic acid specific rnases (rnase t1 from aspergillus oryzae and rnase st from streptomyces erythreus) and guanine-preferential rnase (rnase ms from a. saitoi), the depolymerization reaction of oligoinosinic acid, (ip)ni greater than p, having various chain lengths was studied. the kinetic parameters for depolymerization of oligoinosinic acids, (pkm, log v and log v/km) by the three rnases increased with increase of the chain length of the s ... | 1985 | 3936847 |
| evidence that the mechanisms of fungitoxicity of 8-quinolinol and its bischelate with copper(ii) are different. | the copper(ii) contents of the growth media, sabouraud dextrose and czapek-dox broths, and of the spore inocula of aspergillus niger (atcc 1004), aspergillus oryzae (atcc 1011), trichoderma viride (atcc 8678), and myrothecium verrucaria (atcc 9095) were determined by atomic absorption spectrophotometry in a graphite furnace. the test systems composed of sabouraud dextrose broth and spore inocula of the four fungi contained only a little over 3% of the copper(ii) required to form a minimal inhibi ... | 1985 | 3935305 |
| purification and characterization of endo-beta-n-acetylglucosaminidase of aspergillus oryzae. | an endo-beta-n-acetylglucosaminidase which hydrolyzes the n,n'-diacetylchitobiosyl linkage in asparagine-linked oligosaccharides was purified from the enzyme product of aspergillus oryzae. its substrate specificity was similar to that of endo-beta-n-acetylglucosaminidase h from streptomyces griseus with respect to the relative activities toward the glycopeptides obtained from ovalbumin and bovine igg. the present endoglycosidase exhibited a broad optimum ph range and was relatively stable. metal ... | 1985 | 3934149 |
| effect of additive on alfalfa silage fermentation characteristics and feedlot performance of steers. | in each of two trials four large plastic bags were filled with approximately 72 mt of first cutting, early bloom alfalfa (35% dry matter). fresh alfalfa in two bags was treated with .5 kg/metric ton of a commercial silage additive (silo-best). two bags were left untreated. when compared with steers fed untreated alfalfa silage, weight gains, intakes, and feed efficiencies were not significantly (p greater than .05) altered for steers fed treated silage. however, laboratory analysis showed silage ... | 1985 | 3928719 |
| [mycoses of the orbit and the eye]. | 1985 | 3922126 | |
| enzyme replacement with liposomes containing beta-galactosidase from charonia lumpas in murine globoid cell leukodystrophy (twitcher). | enzyme replacement with liposomes containing beta-galactosidase obtained from charonia lumpas was carried out in murine globoid cell leukodystrophy (gld). charonia lumpas beta-galactosidase was able to hydrolyze galactocerebroside trapped into liposomes prepared from lecithin, cholesterol and sulfatide (molar ratio; 7:2:1). liposomes containing charonia lumpas beta-galactosidase were successfully incorporated into the mouse tissues. 3h-galactocerebroside labeled liposomes were also incorporated ... | 1985 | 3919736 |
| nucleotide sequence of the extracellular glucoamylase gene sta1 in the yeast saccharomyces diastaticus. | the complete nucleotide sequence of the extracellular glucoamylase gene sta1 from the yeast saccharomyces diastaticus has been determined. a single open reading frame codes for a 778-amino-acid protein which contains 13 potential n-glycosylation sites. in the 5'- and 3'-flanking regions of the gene, there are striking sequence homologies to the corresponding regions of adh1 for alcohol dehydrogenase and mat alpha 2 for mating type control in the yeast saccharomyces cerevisiae. the putative precu ... | 1985 | 3918017 |
| [protease and alpha-amylase synthesis by washed cells of aspergillus oryzae 251-90]. | regularities of protease and alpha-amylase production by washed cells of aspergillus oryzae 251-90 were being studied. the results obtained enabled us to assume a constitutive character of the both enzymes synthesis by the given producer. sources of carbon, nitrogen and sulphur take part in regulation of the protease production, whereas in the case of the alpha-amylase synthesis only carbon sources that are important. elimination of phosphorus from the medium affects the synthesis of both enzyme ... | 1985 | 3885211 |
| [interrelation of translation regulation and amino acid uptake into cells]. | 1985 | 3877528 | |
| invasion of paranasal sinuses by aspergillus oryzae. | a 24-year-old male patient receiving chemotherapy for acute promyelocytic leukemia developed fever, right periorbital swelling and mild right proptosis. a head scan showed opacification of the right maxillary and ethmoid sinuses with adjacent soft tissue swelling. biopsy of the nasal mucosa demonstrated the typical septate hyphae of aspergillus species which was later shown on culture to be aspergillus oryzae. a. oryzae has only rarely been reported in human disease and there is confusion as to ... | 1986 | 3796709 |
| the disulphide folding pathway of ribonuclease t1. | the pathway of unfolding and refolding that accompanies, respectively, the breakage and formation of the two disulphide bonds of ribonuclease t1 has been determined kinetically and compared with those of other proteins. | 1986 | 3735429 |
| improved purification of aspergillus oryzae 1,2-alpha-mannosidase by using mannan gel affinity chromatography. | in order to facilitate the purification of 1,2-alpha-mannosidase from an enzyme product of aspergillus oryzae, we have devised a rapid and simple procedure. a partially purified enzyme preparation obtained from the a. oryzae enzyme product, by means of ammonium sulfate fractionation followed by cm-sephadex c-50 chromatography, was subjected to affinity chromatography with baker's yeast mannan gel as an adsorbent. 1,2-alpha-mannosidase was retarded and well separated from the major protein peak o ... | 1986 | 3700367 |
| effect of yeast culture and aspergillus oryzae fermentation extract on ruminal characteristics and nutrient digestibility. | four nonpregnant and nonlactating holstein cows fitted with ruminal fistulas were assigned to each of four diets in a 4 x 4 latin square design. dietary treatments were 1) basal diet containing 50% concentrate; 2) basal diet plus 90 g/d yeast culture; 3) basal diet plus 2.63 g/d aspergillus oryzae fermentation extract; 4) basal diet plus 90 g/d of a. oryzae fermentation extract and yeast culture. cows were fed diets at a rate of 86 g dm/kg bw.75 for 14 d adaptation followed by an 8-d collection ... | 1987 | 3680724 |
| studies on the active site of taka-amylase a: its action on phenyl maltooligosides with a charge at their non-reducing-ends. | five modified moltooligosaccharides, phenyl o-6-amino-6-deoxy-alpha-d- glucopyranosyl- (1----4)-o-alpha-d-glucopyranosyl-(1----4)-o-alpha-d-glucopyranosyl-(1-- --4)- alpha-d-glucopyransoide (ag4p), phenyl o-(alpha-d-glucopyranosyluronic acid)-(1----4)-o-alpha-d-glucopyranosyl-(1----4)-o-alpha-d-glucopyran osy l- (1----4)-alpha-d-glucopyranoside (cg4p), phenyl o-6-amino-6-deoxy-alpha-d-glucopyranosyl-(1----4)-o-alpha-d-glucopyra nos yl- (1----4)-o-alpha-d-glucopyranosyl-(1----4)-o-alpha-d-glucopy ... | 1987 | 3501785 |
| differential scanning calorimetric study of the thermal unfolding of taka-amylase a from aspergillus oryzae. | the thermally induced unfolding of taka-amylase a, isolated from aspergillus oryzae, was studied by differential scanning calorimetry. the experimental curves of excess apparent specific heat vs. temperature showed a single asymmetric peak. curve resolution indicated that this asymmetry is due to the two-state unfolding of three domains in the molecule, with dissociation of the single tightly bound ca2+ ion occurring during the unfolding of the last domain. further indication of the dissociation ... | 1987 | 3498514 |
| nucleotide sequence of the alpha-amylase gene (alp1) in the yeast saccharomycopsis fibuligera. | the complete nucleotide sequence of the secretable alpha-amylase gene alp1 from the yeast saccharomycopsis fibuligera has been determined. the alp1 dna hybridized to a polyadenylated rna of 2.0 kilobases. a single open reading frame encodes a 494-amino acid protein which is highly homologous with alpha-amylase (taka-amylase) of a fungus aspergillus oryzae. | 1987 | 3497057 |
| new alpha-amylase and trypsin inhibitors among the cm-proteins of barley (hordeum vulgare). | barley cm-proteins are a group of at least five salt-soluble components (cma-e) that can be selectively extracted from endosperm with chloroform/methanol mixtures. n-terminal sequences of proteins cma, cmb and cmc have been determined and found to be homologous to those previously determined for cmd and cme, an observation which confirms that their structural genes are members of a dispersed multi-gene family. the purified cm-proteins were tested against trypsin and against alpha-amylases from s ... | 1986 | 3484638 |
| transformation of aspergillus oryzae using the a. niger pyrg gene. | a transformation system for aspergillus oryzae based on the orotidine-5'-phosphate decarboxylase gene (pyrg) was developed. transformation frequencies of up to 16 transformants per microgram of dna were obtained with the vector pab4-1, which carries the pyrg gene of a. niger. southern blotting analysis showed that vector dna sequences were integrated into the chromosomal dna, in various copy numbers and presumably at different sites. efficient cotransformation of an unselectable gene was also sh ... | 1987 | 3481025 |
| study on immobilization of aminoacylase from aspergillus oryzae on macroporous copolymers. | the aminoacylase from aspergillus oryzae was adsorbed on polymer carriers where the enzyme showed excellent catalyzing activity and operating stability. it was found that the pore structure and functional group were the basic factors which affected the activity of the adsorbed enzyme. the hydrophobility of the carriers did not play an important role in the enzymatic resolution. various factors, such as percentage and nature of cross-linking agent, porogenic agents and functionalizing agents whic ... | 1987 | 3452428 |
| [changes in the composition and unsaturated state of the neutral lipid fraction during the development of the fungus aspergillus oryzae]. | 1988 | 3412198 | |
| nutritive value of whole soybeans fermented with aspergillus oryzae or rhizopus oligosporus as evaluated by neonatal pigs. | two experiments were conducted to evaluate the nutritive effects of heated whole soybeans fermented with the mold aspergillus oryzae (aos) or rhizopus oligosporus (ros) in diets fed to neonatal pigs from 1 to 22 d of age. in experiment 1, either soybean meal or heated whole soybeans fermented with ros replaced 75% of the dried skim milk protein. the average daily gain (adg) and gain-feed (g-f) ratio of pigs fed the diet containing 100% milk protein were greater than those of pigs fed the diets c ... | 1988 | 3357058 |
| studies of protease and protease inhibitors in familial amyloidotic polyneuropathy. | serum levels of 6 protease inhibitors, alpha 1-antitrypsin, cl inactivator, alpha 2-macroglobulin, antithrombin-3, alpha 1-antichymotrypsin and inter-alpha-trypsin inhibitor were measured in patients with familial amyloidotic polyneuropathy (fap) and a control group without neurologic disease. no significant differences were observed between the 2 groups. the proteolytic effect of brinase, an enzyme from aspergillus oryzae, on amyloid tissue sections from patients with fap was also evaluated. am ... | 1987 | 3316509 |
| alpha-amylase structure and activity. | two computerized methods of predicting protein secondary structure from amino acid sequences are evaluated by using them on the alpha-amylase of aspergillus oryzae, for which the three-dimensional structure has been determined. the methods are then used, with amino acid alignments, to predict the structures of other alpha-amylases. it is found that all alpha-amylases of known amino acid sequence have the same basic structure, a barrel of eight parallel stretches of extended chain surrounded by e ... | 1988 | 3267138 |
| [comparison of chemical and thermal stability of soluble and immobilized alpha-amylases from b. licheniformis and a. oryzae]. | alpha-amylases from b. licheniformis and a. oryzae, which differ in their thermal stability, were studied with respect to their resistance to chemical denaturants as guanidine hydrochloride, urea, aliphatic alcohols, and formaldehyde. moreover, the thermal and chemical stabilities of both enzymes were compared after their covalent binding to gamma-aminopropyl silica. the thermolabile alpha-amylase (a. oryzae) as well as the thermostable alpha-amylase (b. licheniformis) are remarkably stabilized ... | 1988 | 3266840 |
| [the role of alpha-amylase in baker's asthma]. | we report a case of asthma in a baker provoked by an additive which is generally used in bread making, namely alpha-amylase, an extract of aspergillus oryzae. skin tests to alpha-amylase were positive in a concentration of 0.1 micrograms/ml. specific ige was detected to this enzyme. a provocation test to alpha-amylase was positive with a fall of the fev1 of 42%. provocation tests to flour gave a negative immediate and delayed reaction. progress was made towards the disappearance of symptoms afte ... | 1988 | 3263674 |
| activation of antioxidant activity in natural medicinal products by heating, brewing and lipophilization. a new drug delivery system. | on the basis of the authors' previous hypothesis (1) that treatment of natural plant products with heating and gastric juice results in liberation of low molecular weight compounds with antioxidant activity that exist in the native products as repeating subunits of high molecular weight polymers, they have developed specially treated natural health or medicinal products in which several identifiable low molecular weight compounds with antioxidant activity are liberated and activated. the princip ... | 1988 | 3219997 |
| amino-acid sequence of ribonuclease t2 from aspergillus oryzae. | the amino acid sequence of ribonuclease t2 (rnase t2) from aspergillus oryzae has been determined. this has been achieved by analyzing peptides obtained by digestions with achromobacter lyticus protease i, staphylococcus aureus v8 protease, and alpha-chymotrypsin of two large cyanogen bromide peptides derived from the reduced and s-carboxymethylated or s-aminoethylated protein. digestion with a. lyticus protease i was successfully used to degrade the n-terminal half of the s-aminoethylated prote ... | 1988 | 3169020 |
| mycological identification of pulmonary aspergilloma caused by aspergillus oryzae with proliferating heads. | 1988 | 3148401 | |
| two-dimensional 1h-nmr investigation of ribonuclease t1. resonance assignments, secondary and low-resolution tertiary structures of ribonuclease t1. | ribonuclease t1 was studied by two-dimensional 1h-nmr spectroscopy. resonance assignments were obtained for the backbone protons of 95 amino acid residues and most of its side-chain protons using sequence-specific assignment procedures. the secondary structure elements of ribonuclease t1 were identified by an investigation of medium- and long-range nuclear overhauser effects between the backbone and c beta protons. a low-resolution three-dimensional structure of ribonuclease t1 was deduced from ... | 1988 | 3143569 |
| molecular dynamics simulations of ribonuclease t1: analysis of the effect of solvent on the structure, fluctuations, and active site of the free enzyme. | molecular dynamics simulations were performed on ribonuclease t1 (rnase t1; ec 3.1.27.3) to determine a structure for the free enzyme. simulations starting with the x-ray coordinates for the 2'gmp-rnase t1 complex were done in vacuo and with an 18-a water ball around the active site using stochastic boundary conditions to understand the influence of water on both the structure and fluctuations of the enzyme. removal of 2'gmp caused structural changes in the loop regions, including those directly ... | 1988 | 3139027 |
| expression of the chemically synthesized gene for ribonuclease t1 in escherichia coli using a secretion cloning vector. | the gene for ribonuclease t1 from aspergillus oryzae has been chemically synthesized using the segmental support technique. an escherichia coli clone producing the ribonuclease at high levels was constructed by linking the gene downstream to the region coding for the signal peptide of the ompa protein (a major outer membrane protein of e. coli), using the secretion cloning vector pin-iii-ompa2. this strategy was employed in order to circumvent a possible toxic effect of the gene product on the h ... | 1988 | 3131142 |
| two histidine residues are essential for ribonuclease t1 activity as is the case for ribonuclease a. | ribonuclease t1 (rnase t1, ec 3.1.27.3) is a guanosine-specific ribonuclease that cleaves the 3',5'-phosphodiester linkage of single-stranded rna. it is assumed that the reaction is generated by concerted acid-base catalysis between residues glu-58 and his-92 or his-40. from the results of chemical modification and nmr studies, it appeared that the residue glu-58 was indispensable for nucleolytic activity. however, we have recently demonstrated that glu-58 is an important but not an essential re ... | 1987 | 3126807 |
| purification of ribonuclease t1. | an improved method for purifying ribonuclease t1 from aspergillus oryzae is described. the method uses gradient elution from deae-cellulose and sulfopropyl-sephadex columns followed by gel filtration on sephadex g-50 to give almost 100 mg (50% yield) of ribonuclease t1 from 100 g of starting material in less than 5 days. | 1987 | 3126677 |
| purification and properties of an extracellular glucoamylase from a diastatic strain of saccharomyces cerevisiae. | the extracellular glucoamylase from certain strains of saccharomyces cerevisiae can be purified from culture medium by a simple chromatographic procedure. the native enzyme is heavily glycosylated and has an mr of about 250,000, but gel filtration indicates the existence of oligomers of larger size. dissociation yields a form of mr about 70,000. the glucoamylase is rich in serine and threonine and in aspartic acid plus asparagine, and has a pi of 4.62 and a ph optimum of 4.5-6.5. the thermostabi ... | 1988 | 3124820 |
| structures of oligosaccharides on beta-galactosidase from aspergillus oryzae. | the carbohydrate portions of beta-galactosidase from aspergillus oryzae were found to be composed of two types of sugar chains. they were released equally well with endo-beta-n-acetylglucosaminidase h, but were distinct in their chain length. the long sugar chains (fraction i), corresponding to 4% of the total carbohydrate chains, were composed of galactomannan-type oligosaccharides, which consisted of mannose, galactose, glucose, and glucosamine in the molar ratios of 30.0, 16.4, 1.4, and 2.1 p ... | 1987 | 3117779 |
| frequency domain measurements of the fluorescence lifetime of ribonuclease t1. | using multifrequency phase/modulation fluorometry, we have studied the fluorescence decay of the single tryptophan residue of ribonuclease t1 (rnase t1). at neutral ph (7.4) we find that the decay is a double exponential (tau 1 = 3.74 ns, tau 2 = 1.06 ns, f1 = 0.945), in agreement with results from pulsed fluorometry. at ph 5.5 the decay is well described by a single decay time (tau = 3.8 ns). alternatively, we have fitted the frequency domain data by a distribution of lifetimes. temperature dep ... | 1987 | 3115328 |
| protein dynamics. a time-resolved fluorescence, energetic and molecular dynamics study of ribonuclease t1. | studies using time-resolved fluorescence depolarization were performed on the internal motion of trp 59 of ribonuclease t1 (ec 3.1.27.3) in the free enzyme, 2'-gmp-enzyme complex and 3'-gmp-enzyme complex. the trp 59 motion was also studied in the free enzyme using molecular dynamics simulations. energetic analysis of activation barriers to the trp 59 motion was performed using both the transition state theory and kramers' theory. the activation parameters showed a dependence on solvent viscosit ... | 1987 | 3111558 |
| does oral enzyme replacement therapy reverse intestinal lactose malabsorption? | the effects of oral enzyme replacement therapy on breath hydrogen excretion and symptoms after milk ingestion were studied in lactase-deficient patients. sixteen symptomatic patients underwent interval hydrogen breath tests using whole milk as substrate. each study was repeated with the addition of 250 mg of beta-d-galactosidase derived from aspergillus oryzae (lactrase) given orally with the milk. subsequently seven of those 11 patients who did not normalize their hydrogen excretion with 250 mg ... | 1987 | 3111243 |
| facile preparation and some applications of an affinity matrix with a cleavable connector arm containing a disulfide bond. | a versatile affinity matrix in which the ligand of interest is linked to the matrix through a connector arm containing a disulfide bond is described. it can be synthesized from any amino-substituted matrix by successive reaction with 2-imino-thiolane, 5,5'-dithiobis(2-nitrobenzoic acid), and a thiol derivative of the ligand of choice. the repertoire of ligands can be significantly increased by the appropriate use of avidin-biotin bridges. after adsorption of the material to be fractionated, elut ... | 1987 | 3110760 |
| effective reduction of lactose maldigestion in preschool children by direct addition of beta-galactosidases to milk at mealtime. | we examined the efficiency of two beta-galactosidase preparations--one derived from the yeast, kluyveromyces lactis (lactaid), the other derived from the fungus, aspergillus oryzae (takamine)--to assist the in vivo digestion of lactose consumed by healthy guatemalan preschool children. milk prehydrolyzed by in vitro incubation with enzymes was used as the standard of reference, and the degree of incomplete digestion of lactose from 240 ml of milk was determined using the hydrogen breath test. in ... | 1987 | 3106927 |
| simple method for screening aflatoxin-producing molds by uv photography. | uv absorption by aflatoxins was monitored in gy agar medium by uv photography. in the uv photographs, aflatoxin-producing molds were identified as gray or black colonies, whereas aflatoxin-nonproducing molds appeared as white colonies. by cellophane transplantation experiments and silica gel thin-layer chromatography, the products absorbing uv light substantially were found to be mainly aflatoxins b1 and g1 excreted from the mold mycelium into the agar medium. uv absorption did not occur when th ... | 1987 | 3105453 |
| actions of aspergillus oryzae alpha-amylase, potato phosphorylase, and rabbit muscle phosphorylase a and b on phosphorylated (1----4)-alpha-d-glucan. | aspergillus oryzae alpha-amylase [(1----4)-alpha-d-glucan glucanohydrolase, ec 3.2.1.1] produced o-(6-phosphoryl-alpha-d-glucopyranosyl)-(1----4)-o-alpha-d-glucopyran osy l-(1----4)-d-glucopyranose (6(3)-phosphorylmaltotriose) and o-alpha-d-glucopyranosyl-(1----4)-o-(3-phosphoryl-alpha-d-glucopyranosyl )- (1----4)-o-alpha-d-glucopyranosyl-(1----4)-d-glucopyranose (3(3)-phosphorylmaltotetraose) from potato starch upon exhaustive hydrolysis. these products indicate that the enzyme hydrolyses the s ... | 1986 | 3096568 |
| production of aflatoxins by strains of the aspergillus flavus group maintained in atcc. | a total of 169 strains of the aspergillus reference cultures in the aspergillus flavus group maintained in the american type culture collection (atcc) were studied for their aflatoxin-producing abilities in rice, peanut and semisynthetic medium, utilizing high pressure liquid chromatography. fifty-nine of the strains examined were positive for aflatoxin formation. no strains of the food fungi a. oryzae or a. sojae produced detectable levels of aflatoxins, while 33-85% of the strains of a. flavus ... | 1986 | 3083260 |
| jokichi takamine (1854-1922). | 1988 | 3057095 | |
| [enzymatic isolation of the pyramidal neurons of the rat hippocampus]. | 1987 | 3034680 | |
| an immunochemical study of neurospora nucleases. | nucleases derived from neurospora crassa mycelia with neutral single-strand (ss) endodeoxyribonuclease activity have been examined by immunochemical techniques and by sodium dodecyl sulfate - dna gel electrophoresis. all of the intracellular nucleases, which have different divalent metal ion requirements, different strand specificities with single- and double-strand dna, different modes of action on dna and rna, and other distinguishing characteristics, are immunochemically related to neurospora ... | 1986 | 3013242 |
| [development of new plate tests for the detection of microbial hydrolysis of esters and oxidation of 2-hydroxycarboxylic acids]. | the application of the thin-agar-layer coated filter culture technique (z. naturforsch. 42c, 1082 (1987)) has been extended to the detection of ester hydrolysis and 2-hydroxyacid oxidation by microbial colonies. the former was performed by spraying with bromocresol purple and the latter with a salicylhydrazide reagent. under the optimized conditions, the hydrolysis activity of more than 20 mumol/h.g-wet cells and the oxidation activity of more than 40 mumol/h.g-wet cells were usually detected di ... | 1987 | 2966500 |
| 5-iodoribose 1-phosphate, an analog of ribose 1-phosphate. enzymatic synthesis and kinetic studies with enzymes of purine, pyrimidine, and sugar phosphate metabolism. | the 5'-deoxy-5'-iodo-substituted analogs of adenosine and inosine are cytotoxic to tumor cells that have high activities of 5'-methylthioadenosine phosphorylase and purine nucleoside phosphorylase, respectively (savarese, t.m., chu, s-h., chu, m.y., and parks, r. e., jr. (1984) biochem. pharmacol. 34, 361-367). 5-iodoribose 1-phosphate (5-irib-1-p), the common intracellular metabolite of these 5'-iodonucleosides, has been synthesized enzymatically from 5'-deoxy-5'-iodoadenosine via adenosine dea ... | 1986 | 2934389 |
| 1h-nmr investigation of the interaction between rnase t1 and a novel substrate analog, 2'-deoxy-2'-fluoroguanylyl-(3'-5')uridine. | the interaction between rnase t1 and a non-hydrolysable substrate analog, 2'-deoxy-2'-fluoroguanylyl-(3'-5')uridine (gfpu), was investigated using 1h-nmr spectroscopy. in the complex, the gfp portion takes the syn form around the glycosidic bond and the 3'-endo form for the ribose moiety, similar to those found in 3'-gmp and 2'-deoxy-2'-fluoroguanosine 3'-monophosphate (gfp). however, in contrast to the cases of these two inhibitors, the complex formation with gfpu at ph 6.0 was found to shift t ... | 1988 | 2841155 |
| action of gamma endonuclease on clustered lesions in irradiated dna. | irradiation of dna in situ i.e. in phage particles or in the cell leads to alterations of single dna nucleotides as well as to clustered lesions such as double strand breaks or unpaired dna regions the latter being sensitive to digestion by s1 nuclease. a contribution will be made to the configuration of such s1-nuclease-sensitive sites (s1 sites). dna from irradiated lambda phage containing s1 sites was treated with gamma endonuclease from m. luteus which is known to split the nucleotide strand ... | 1988 | 2839862 |
| immobilization of single-strand specific nuclease (s1 nuclease) from aspergillus oryzae. | s1 nuclease from aspergillus oryzae (ec 3.1.30.1) was coupled to gelatin-alginate composite matrix using the residual free aldehyde groups on the surface of glutaraldehyde crosslinked matrix. the immobilized enzyme retained approximately 10% activity of the soluble enzyme. when partially purified enzyme was bound to the matrix, the immobilized preparation did not show any detectable enzyme activity. however, the activity could be restored when the coupling was carried out in the presence of a co ... | 1987 | 2820305 |
| analysis of the alpha-amylase gene of schwanniomyces occidentalis and the secretion of its gene product in transformants of different yeast genera. | we have cloned and characterized the alpha-amylase gene (amy1) of the yeast schwanniomyces occidentalis. a cosmid gene library of s. occidentalis dna was screened in saccharomyces cerevisiae for alpha-amylase secretion. the positive clone contained a dna fragment harbouring an open reading frame of 1536 nucleotides coding for a 512-amino-acid polypeptide with a calculated mr of 56,500. the deduced amino acid sequence reveals significant similarity to the sequence of the saccharomycopsis fibulige ... | 1989 | 2806251 |
| studies on antifungal properties of phenol complexes with secondary amines. 1. the effect of complex formation of nitro- and chlorophenols with dicyclohexylamine on the antifungal activity in vitro. | inhibitory doses (id50) of phenols complexed with dicyclohexylamine are lower (21.4-47.7%) than the inhibitory doses of free phenols. this is demonstrated in vitro by experiments with aspergillus oryzae and penicillium expansum on solid medium. | 1989 | 2797052 |
| aspergillus oryzae has two nearly identical taka-amylase genes, each containing eight introns. | cdna and genomic dna for two nearly identical genes, amyi and amyii, coding for the enzyme taka-amylase a (ta-a) of the fungus aspergillus oryzae have been cloned and characterized. these genes are apparently unlinked, differing by only 3 nucleotides (nt) out of the 2720 nt that span the coding regions. the 617-nt 5'-flanking regions differ only at nt -372 (t or a) from the putative atg start codon and contain four sets of short, inverted repeats (ir) upstream from the putative tataaa box at nt ... | 1989 | 2789162 |
| three alpha-amylase genes of aspergillus oryzae exhibit identical intron-exon organization. | we have cloned three genes (amy1, amy2 and amy3) encoding alpha-amylase in the filamentous fungus aspergillus oryzae. the established overall sequences have a very high degree of homology, showing divergences mainly in the 3'-untranslated regions. the positions and the sequences of the eight introns were found to be absolutely identical in the three genes. the sequence analysis of the 5'-regions revealed presumptive tata, caat and gc boxes. primer extension analysis was performed to determine th ... | 1989 | 2785629 |
| studies on the accessibility of nascent non-helical peptide chains on the ribosome. | the accessibility of nascent polypeptides with special structural elements to the ribosome was investigated. poly(c), poly(c, u) and poly(c, a) mrnas were translated by e. coli ribosomes in vitro. the resulting peptides which were rich in prolines, remained on the ribosomal particles or were released after addition of puromycin. a protease from aspergillus oryzae hydrolyzed the released peptides rapidly, whereas the degradation of the unreleased ones was only slightly affected. this result shows ... | 1989 | 2699792 |
| a full length cdna clone for the alkaline protease from aspergillus oryzae: structural analysis and expression in saccharomyces cerevisiae. | we have cloned and determined the nucleotide sequence of a cdna fragment for the entire coding region of the alkaline protease (alp) from a filamentous ascomycete aspergillus oryzae. according to the deduced amino acid sequence, alp has a putative prepro region of 121 amino acids preceding the mature region, which consists of 282 amino acids. a consensus sequence of a signal peptide consisting of 21 amino acids is found at the n-terminus of the prepro region. the primary structure of the mature ... | 1989 | 2693947 |
| a gene transfer system based on the homologous pyrg gene and efficient expression of bacterial genes in aspergillus oryzae. | a homologous transformation system for aspergillus oryzae is described. the system is based on an a. oryzae strain deficient in orotidine-5'-phosphate decarboxylase (pyrg) and the vector pao4-2, which contains a functional a. oryzae pyrg gene as selection marker. transformation of the a. oryzae pyrg mutant with circular pao4-2 resulted in the appearance of pyr+ transformants at a frequency of up to 20 per micrograms of dna, whereas with linear pao4-2 up to 200 transformants per micrograms dna we ... | 1989 | 2688930 |
| conformational stability and activity of ribonuclease t1 and mutants. gln25----lys, glu58----ala, and the double mutant. | ribonuclease t1 (rnase t1) and mutants gln25----lys, glu58----ala, and the double mutant were prepared from a chemically synthesized gene, cloned and expressed in escherichia coli. the wild-type rnase t1 prepared from the cloned gene was identical in every functional and physical property examined to rnase t1 prepared from aspergillus oryzae. urea and thermal unfolding experiments show that gln25----lys is 0.9 kcal/mol more stable and glu58----ala is 0.8 kcal/mol less stable than wild-type rnase ... | 1989 | 2663837 |
| free flow electrophoresis as a method for the purification of enzymes from e. coli cell extract. | the application of the four techniques of free flow electrophoresis (zone electrophoresis, isotachophoresis, isoelectric focusing and field step electrophoresis) for the purification of proteins from a complex protein mixture was investigated. for this purpose alpha-amylase (ec 3.2.1.1) from aspergillus oryzae was added and reisolated from e. coli cell extract. the chosen enzyme and the biological extract are models for many industrial separation problems. in optimized experiments purity, purifi ... | 1989 | 2651110 |
| probing the anticodon loop structure in yeast trna(phe-y) with single strand-specific nuclease s1. | yeast trna(phe) and trna(phe-y) are cleaved by single strand-specific endonuclease s1 at the same positions within the anticodon loop (phosphates 34, 36 and 37) and at the 3'-terminus (phosphates 75 and 76). the efficiency of the anticodon loop hydrolysis is much higher in trna(phe-y) while the cutting at the 3'-terminus is not influenced considerably by the y-base1 removal from yeast trna(phe). the effect of the y-base excision on the structure of the anticodon loop is discussed on the basis of ... | 1989 | 2618244 |
| characterization of three enzymatic forms of glucose-6-phosphate dehydrogenase from aspergillus oryzae. | three forms (i, ii and iii) of glucose-6-phosphate dehydrogenase were isolated from mycelium of aspergillus oryzae grown on ribose as the carbon source, by ion-exchange chromatography. the km values determined for the three forms with respect to glucose-6-phosphate were nearly identical; however the km for nadp+ were different and the vmax for the isoenzymatic form ii was higher than those for i and iii. inhibition by nadph was competitive with respect to nadp+, isoenzyme ii showing the highest ... | 1989 | 2616874 |
| isolation of a cdna encoding aspergillus oryzae taka-amylase a: evidence for multiple related genes. | complementary and genomic dnas encoding aspergillus oryzae taka-amylase a (taa) were cloned and sequenced. the coding sequence of the cdna comprised the signal peptide [21 amino acids (aa)] and mature taa (478 aa). the deduced aa sequence agrees well with the published aa sequence, except for one insertion, one deletion and ten aa substitutions. these differences might be due to the difference in the strains used. sequence comparison of the cdna and genomic dna indicates the presence of eight in ... | 1989 | 2612911 |
| purification and characterization of an insect alpha-amylase inhibitor/endochitinase from seeds of job's tears (coix lachryma-jobi). | a protein inhibitor of locust gut alpha-amylase was purified from seeds of job's tears (coix lachryma-jobi) using ammonium sulphate precipitation, affinity chromatography on red sepharose and reversed-phase hplc. it consisted of two major isomers, each a dimer of two closely similar or identical subunits of mr about 26,400, and associated by inter-chain disulphide bonds. these isomers also had closely similar amino acid compositions. the major isomer showed no inhibitory activity against amylase ... | 1989 | 2605263 |
| preparation and properties of rnase t2 immobilized on concanavalin a-sepharose. | partially purified rnase t2 (ec 2.7.7.17) from aspergillus oryzae was bound through its carbohydrate moiety to concanavalin a-sepharose. the retention of activity was high, ranging from 70% at low enzyme load to approximately 9% at high enzyme load. though there was no change in the ph and temperature optima, the ph stability and the km decreased after immobilization. compared to the soluble enzyme, the immobilized rnase t2 showed enhanced temperature stability and more resistance to metal ions. ... | 1989 | 2596845 |
| [the stimulating effect of n-nitroso-ethylurea on the biosynthetic ability of aspergillus oryzae]. | the mutagenic action of n-nitroso-n-ethylurea (neu) taken at shock and prolonged doses together on aspergillus oryzae yielded 98% of populations with an elevated synthesis of proteolytic enzymes. the combined action of shock and prolonged neu doses had an advantage over a shock pulse dose because the frequency of mutations rose 2-16 times and the populations accumulated proteolytic enzymes within the range of 9 to 24 activity units. as was shown using a certain number of populations selected at ... | 1989 | 2586348 |
| rhizomucor miehei triglyceride lipase is processed and secreted from transformed aspergillus oryzae. | the cdna encoding the precursor of the rhizomucor miehei triglyceride lipase was inserted in an aspergillus oryzae expression vector. in this vector the expression of the lipase cdna is under control of the aspergillus oryzae alpha-amylase gene promoter and the aspergillus niger glucoamylase gene terminator. the recombinant plasmid was introduced into aspergillus oryzae, and transformed colonies were selected and screened for lipase expression. lipase-positive transformants were grown in a small ... | 1989 | 2586234 |
| three-dimensional structure of ribonuclease t1 complexed with guanylyl-2',5'-guanosine at 1.8 a resolution. | the enzyme ribonuclease t1 (rnase t1) isolated from aspergillus oryzae was cocrystallized with the specific inhibitor guanylyl-2',5'-guanosine (2',5'-gpg) and the structure refined by the stereochemically restrained least-squares refinement method to a crystallographic r-factor of 14.9% for x-ray data above 3 sigma in the resolution range 6 to 1.8 a. the refined model consists of 781 protein atoms, 43 inhibitor atoms in a major site and 29 inhibitor atoms in a minor site, 107 water oxygen atoms, ... | 1989 | 2541256 |
| synergistic antifungal action of 8-quinolinol and its bischelate with copper(ii) and with mixed ligand chelates composed of copper(ii), 8-quinolinol, and aromatic hydroxy acids. | antifungal studies were made of mixtures of minimal inhibitory concentrations (mics) of 8-quinolinol and its bischelates with copper(ii), zinc(ii), and manganese(ii) and with mixed ligand chelates composed of 8-quinolinol, copper(ii) and a second ligand including salicylic acid, 3-hydroxy-2-naphthoic acid, 3,5-diiodosalicylic acid, and 4-bromo-3-hydroxy-2-naphthoic acid. mixtures of the mics of the bischelates of 8-quinolinol with copper(ii) and zinc(ii) and copper(ii) and manganese(ii), as well ... | 1989 | 2516124 |
| binding of vanadate (v) to ribonuclease-t1 and inosine, investigated by 51v nmr spectroscopy. | ribonuclease t1 (rnase-t1) from aspergillus oryzae cleaves ribonucleic acid specifically at guanosine to yield oligonucleotides with terminal guanosine-3'-phosphate. it forms a complex with vanadate (association constant k approximately 145 +/- 30 m-1; delta (51v) = -514 ppm) with spectral features similar to the less stable complexes obtained with di- and tripeptides (gly-his, pros-his-ala, gly-his-lys, val-glu) containing amino acids that are constituents at the active site of the enzyme. guan ... | 1989 | 2513377 |
| enzyme replacement for lactose malabsorption using a beta-d-galactosidase. | we evaluated 10 healthy symptomatic lactose malabsorbers for effect of an oral beta-d-galactosidase derived from aspergillus oryzae (lactrase, kremers urban company, milwaukee, wi, u.s.a.) on symptom and breath hydrogen response to challenge with 50 g lactose. basally and at 30-min intervals for 8 h after lactose challenge, end-alveolar breath samples were collected and analyzed for hydrogen using gas chromatography. symptoms were scored at 30 min and hourly for 8 h, rating bloating, cramps, nau ... | 1989 | 2502573 |
| hydrophobic cluster analysis of the primary sequences of alpha-amylases. | the amino acid sequences of 18 alpha-amylases have been compared by hydrophobic cluster analysis. the method was first calibrated with two alpha-amylases (aspergillus oryzae and pig pancreas) whose three-dimensional structures are known. it was then applied to the other alpha-amylases resulting in straightforward sequence alignments which could be used for structure prediction. it was found that all alpha-amylases which were investigated display the same basic super-secondary structure with a (b ... | 1989 | 2489084 |
| biosynthesis, in calf pancreas microsomes, of three lipid-linked oligosaccharide diphosphates from a synthetic dolichyl diphosphate tetrasaccharide. | incubation of calf pancreas microsomes with synthetic alpha-d-manp-(1----6)-beta-d-manp-(1----4)-beta-d-glcpnac-(1 ----4)-alpha-d- glcpnac-pp-dol and gdp-d-[14c]-mannose gave three major lipid-linked oligosaccharide diphosphates. after release of the phospholipid residue by mild acid hydrolysis, the corresponding [14c]oligosaccharides were analyzed by gel-filtration, liquid chromatography, degradation by endo-n-acetyl-beta-d-glucosaminidases d and h, by jack bean alpha-d-mannosidase and aspergil ... | 1988 | 2463085 |
| conformational stability and activity of ribonuclease t1 with zero, one, and two intact disulfide bonds. | ribonuclease t1 has two disulfide bonds linking cysteine residues 2-10 and 6-103. we have prepared a derivative of ribonuclease t1 in which one disulfide bond is broken and the cysteine residues carboxymethylated, (2-10)-rcm-t1, and three derivatives in which both disulfides are broken and the cysteine residues reduced, r-t1, carboxamidomethylated, rcam-t1, or carboxymethylated, rcm-t1. the rna hydrolyzing activity of these proteins has been measured, and urea and thermal denaturation studies ha ... | 1988 | 2457027 |
| properties of the complex between alpha 2-macroglobulin and brinase, a proteinase from aspergillus oryzae with thrombolytic effect. | the proteinase, brinase (mr approximately 35000), from aspergillus oryzae, which has been used in therapeutic attempts as a thrombolytic agent in arterial thrombosis, binds to purified human alpha 2-macroglobulin (alpha 2m) with a stoichiometry of 1.7-1.9 mol of enzyme/mol inhibitor. this binding leads to quantitative cleavage of the bait region of the inhibitor and to release of 3.6 thiol groups per molecule of alpha 2m, reflecting cleavage of the thioester bonds. the reaction with brinase is a ... | 1988 | 2450410 |
| allergic bronchopulmonary aspergillosis due to aspergillus oryzae. | a 19-year-old female student with allergic bronchopulmonary aspergillosis (abpa) due to aspergillus oryzae is reported. this organism was used for fermentation starter to make soybean paste in her father's workshop adjacent to the home where she lived. abpa might be considered an occupational disease in certain situations. | 1987 | 2433099 |
| role of aspergillus amylase in baker's asthma. | 1986 | 2417074 | |
| effects of aspergillus oryzae fermentation extract on fermentation of amino acids, bermudagrass and starch by mixed ruminal microorganisms in vitro. | the objective of this study was to examine the effects of aspergillus oryzae fermentation extract (amaferm) on the in vitro ruminal fermentation of coastal bermudagrass, soluble starch and amino acids. mixed ruminal microorganisms were incubated in anaerobic media for either 24 h (amaferm alone, soluble starch, amino acids) or 48 h (bermudagrass). amaferm was added to the incubation bottles (n = 4) at concentrations of 0, .4 or 1.0 g/liter. when mixed ruminal microorganisms were incubated with o ... | 1990 | 2384404 |
| characteristics of immobilized aminoacylase from aspergillus oryzae on macroporous copolymers. | aminoacylase from aspergillus oryzae was adsorbed on functionallized macroporous copolymers where the enzyme showed excellent catalyzing activity and operation stability. various factors which effect the activity of the immobilized aminoacylase such as temperature, ph and ionic strength were investigated. the continuous operation of the enzyme immobilized on macroporous copolymers was compared with that of the enzyme immobilized on deae-sephadex. | 1990 | 2383665 |
| localization of pyruvate carboxylase in organic acid-producing aspergillus strains. | the localization of pyruvate carboxylase (cytosolic or mitochondrial) was studied in nine different aspergillus species (14 strains). in some species (a. aculeatus, a. flavus, a. foetidus, a. nidulans, a. ochraceus, and a. sojae), the pyruvate carboxylase activity could be detected only in the cytosolic fraction of the cells. pyruvate carboxylase has been found only in the mitochondrial fraction of two strains of aspergillus wentii. in aspergillus oryzae and in five strains of aspergillus niger, ... | 1990 | 2383004 |
| influence of cultures of aspergillus oryzae on rumen and total tract digestibility of dietary components. | three trials were conducted to evaluate the effect of dried cultures of aspergillus oryzae on nutrient utilization by mature holstein cows fitted with ruminal and duodenal cannulas. in trial 1, four cows (two dry and two lactating) were used to test aspergillus oryzae (3 g/d) and a control treatment at two forage amounts in a 4 x 4 latin square. trial 2 compared control, a. oryzae, and saccharomyces cerevesiae using six lactating cows in a repeated 3 x 3 latin square design. for trial 3, four la ... | 1990 | 2341646 |
| [baking ingredients, especially alpha-amylase, as occupational inhalation allergens in the baking industry]. | baker's asthma is the most frequent occupational lung disease in switzerland and west germany. cereal flours, and more rarely flour parasites, are implicated as the responsible allergens. based on an observation of a case of baker's asthma due to monovalent sensitization to alpha-amylase used as additive to flour, 31 bakers with occupational asthma and/or rhinitis were routinely tested by skin tests and serological rast examinations for allergic sensitivity to flour, alpha-amylase and other bake ... | 1990 | 2326614 |
| simultaneous comparison of several sequences. | 1990 | 2314287 | |
| conserved residues of liquefying alpha-amylases are concentrated in the vicinity of active site. | three dimensional structure of three liquefying type bacillus alpha-amylases were modeled based on sequence analyses and refined structure of aspergillus oryzae enzyme. the models suggest that the overall folding motif of alpha-amylases is conserved. the active site, substrate binding and stabilizing calcium binding residues are conserved and concentrated in a cleft between two domains. they constitute the core of alpha-amylases to which other, less conserved regions are attached. the bacterial ... | 1990 | 2302216 |