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5. Bacterial removal of Fe(III) impurities from clay: a potential new technology.

Author

Styriakova I., 3rd Mid-European clay conference Opatija, Croatia 18-23 Sep. 2006, Styriak I., Styriakova I., 3rd Mid-European clay conference Opatija, Croatia 18-23 Sep. 2006, and Styriak I.

Abstract

The removal is discussed of oxidic Fe-phases from industrial silicates by bioleaching. Results are presented which show that small additions of the chelators AQDS or NTA resulted in enhanced Fe (III) reduction or the stimulation of Fe dissolution under non-controlled anaerobic conditions. The bacteria enhanced Fe dissolution indirectly through microbially promoted pH changes and production of organic acids. AQDS stimulated bacterial iron reduction, and Fe2+ concentration in solution was higher than Fe3+. NTA did not stimulate iron reduction but increased bacterial iron dissolution in the form of Fe3+. The concentration of carbon source in the medium was crucial for Fe dissolution and metabolite production. Cheap alternatives such as molasses and food-sugar were used to optimise costs on an industrial scale. The low toxicity of the chelators and bacterial metabolites (pH 4) makes bioleaching an attractive alternative compared with chemical leaching., The removal is discussed of oxidic Fe-phases from industrial silicates by bioleaching. Results are presented which show that small additions of the chelators AQDS or NTA resulted in enhanced Fe (III) reduction or the stimulation of Fe dissolution under non-controlled anaerobic conditions. The bacteria enhanced Fe dissolution indirectly through microbially promoted pH changes and production of organic acids. AQDS stimulated bacterial iron reduction, and Fe2+ concentration in solution was higher than Fe3+. NTA did not stimulate iron reduction but increased bacterial iron dissolution in the form of Fe3+. The concentration of carbon source in the medium was crucial for Fe dissolution and metabolite production. Cheap alternatives such as molasses and food-sugar were used to optimise costs on an industrial scale. The low toxicity of the chelators and bacterial metabolites (pH 4) makes bioleaching an attractive alternative compared with chemical leaching.

Published
2006

6. Binding of extracellular matrix molecules by probiotic bacteria.

Author

Styriak, I, Nemcová, R, Chang, Y-H, Ljungh, Åsa, Styriak, I, Nemcová, R, Chang, Y-H, and Ljungh, Åsa

Abstract

Aims: The aim of this study was to investigate extracellular matrix (ECM) and mucin binding of selected bacterial isolates with probiotic features in comparison with commercially used probiotic bacteria. Methods and Results: ECM molecules were immobilized in microtitre plates ( mucin and fetuin) or on the surface of latex beads. Porcine mucin was bound by all 13 probiotic strains tested with important inter-strain differences; however, fetuin binding was similar ( weak) for all 14 strains tested. Strongly positive ( three) binding of bovine fibrinogen was expressed by strains from fermented food ( Lactobacillus rhamnosus GG, L. casei Shirota and L. johnsonii La1) as well as by L. casei L. c., Lactobacillus sp. 2I3 and by L. plantarum LP. The other strains expressed moderate ( 2) or weakly positive ( 1) binding of bovine fibrinogen. Strongly positive ( 3) binding of porcine fibronectin was observed only with two strains; however, all other strains also bound this molecule. Bovine lactoferrin was bound to a higher extent than transferrins. Significance and Impact of the Study: Some animal strains ( at least L. casei L. c. and Lactobacillus sp. 2I3) are comparable with the commercially used strains with respect to their ECM binding ability. As this feature is important for probiotic bacteria to be able to colonize intestine, these strains should be considered for their wider use in fermented feed ( or probiotic preparations) for animals.

Published
2003

11. The adherence of three streptococcus bovis strains to cells of rumen epithelium primoculture under various conditions

Author

Styriak, I., Galfi, P., and Kmet, V.

Abstract

Three Streptococcus bovis strains were tested in biotype assay and examined for the adherence to cells of rumen epithelium primoculture. The adherence pattern of ruminal streptococci in phosphate buffered saline at pH values ranging from 4.1 to 8.5 was determined. Our isolates of Streptococcus bovis strains adhered best at pH 7.0-7.3.To characterize the adhesive determinants, the bacterial cells were exposed to various treatments. Protease treatment dramatically decreased the adherence of all Streptococcus bovis strains, thus suggesting that the determinants responsible for the adherence are largely proteinaceous. Carbohydrates could be also significantly involved in the active sites of bacterial surface because metaperiodate-treated cells adhered much more poorly than control, sodium iodate-treated cells. Addition of carbohydrates (lactose, maltose and saccharose) had no significant effect on the adherence of Streptococcus bovis strains although a slight decrease in the adhesion was detected.

Published
1994
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14. Colorimetric Glucose Assay Based on Magnetic Particles Having Pseudo-peroxidase Activity and Immobilized Glucose Oxidase.

Author

Martinkova P, Opatrilova R, Kruzliak P, Styriak I, and Pohanka M

Subjects
Female, Humans, Male, Spectrophotometry, Blood Glucose metabolism, Colorimetry methods, Enzymes, Immobilized metabolism, Glucose Oxidase metabolism, Magnetics, Peroxidases metabolism
Abstract

Magnetic particles (MPs) are currently used as a suitable alternative for peroxidase in the construction of novel biosensors, analytic and diagnostic methods. Their better chemical and thermal stabilities predestine them as appropriate pseudo-enzymatic catalysts. In this point of view, our research was focused on preparation of simply and fast method for immobilization of glucose oxidase onto surface of MPs with peroxidase-like activity. Spectrophotometric method (wavelength 450 nm) optimized for glucose determination using modified MPs has been successfully developed. Concentration curve for optimization of method was assayed, and Michaelis-Menten constant (K m) calculated, maximum reaction rate (V max), limit of detection, and correlation coefficient were determined to be 0.13 mmol/l (2.34 mg/dl), 1.79 pkat, 3.74 µmol/l (0.067 mg/dl), and 0.996, respectively. Interferences of other sugars such as sucrose, sorbitol, deoxyribose, maltose, and fructose were determined as well as effect of substances presenting in plasma (ascorbic acid, reduced glutathione, trolox, and urea). Results in comparison with positive and negative controls showed no interferences of the other sugars and no influence of plasma substances to measuring of glucose. The constructed method showed corresponding results with linear dependence and a correlation coefficient of 0.997. Possibility of repeated use of modified MPs was successfully proved.

Published
2016
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15. Probiotics in prevention and treatment of obesity: a critical view.

Author

Kobyliak N, Conte C, Cammarota G, Haley AP, Styriak I, Gaspar L, Fusek J, Rodrigo L, and Kruzliak P

Abstract

The worldwide prevalence of obesity more than doubled between 1980 and 2014. The obesity pandemic is tightly linked to an increase in energy availability, sedentariness and greater control of ambient temperature that have paralleled the socioeconomic development of the past decades. The most frequent cause which leads to the obesity development is a dysbalance between energy intake and energy expenditure. The gut microbiota as an environmental factor which influence whole-body metabolism by affecting energy balance but also inflammation and gut barrier function, integrate peripheral and central food intake regulatory signals and thereby increase body weight. Probiotics have physiologic functions that contribute to the health of gut microbiota, can affect food intake and appetite, body weight and composition and metabolic functions through gastrointestinal pathways and modulation of the gut bacterial community.

Published
2016
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16. Potential of enterococci isolated from horses.

Author

Lauková A, Simonová M, Strompfová V, Styriak I, Ouwehand AC, and Várady M

Subjects
Animals, Anti-Bacterial Agents pharmacology, Apoproteins metabolism, Bacterial Adhesion, Bacterial Proteins analysis, Bridged-Ring Compounds metabolism, Colony Count, Microbial, Drug Resistance, Bacterial, Enterococcus classification, Fibronectins metabolism, Genes, Bacterial, Lactic Acid metabolism, Lactoferrin metabolism, Mucus metabolism, Protein Binding, Slovakia, Transferrin metabolism, Urease analysis, Enterococcus isolation & purification, Enterococcus physiology, Feces microbiology, Horses microbiology, Probiotics isolation & purification, Probiotics metabolism
Abstract

Faecal samples of 122 horses (from farms in Slovakia) were examined to select enterococci to study their probiotic potential for their further use as additives. Each gram of faeces contained 1.0-5.0 cfu (log 10) of enterococci. Of the 43 isolates, 25 (58.1%) were identified as Enterococcus faecium, 3 strains were (6.9%) Enterococcus mundtii and one strain was identified as E. faecalis. Fourteen isolates were not characterized further. A significant proportion of the isolates were resistant to kanamycin, vancomycin and gentamicin. Low urease activity of enterococci dominated. The values of lactic acid ranged from 0.98 to 1.91 mmol/L. Porcine fibronectectin and bovine lactoferrin were bound weakly by tested enterococci, while bovine fibrinogen was bound more strongly. Enterococci from horses did not bind bovine apotransferrin. The isolates adhered with the same ability to human as well as to canine mucus. At least one enterocin gene was detected among 16 analyzed isolates. Ent B gene was detected in all strains tested (16, 100%), followed by the genes ent A, ent P and ent L50B. Three suitable candidates-the strains of E. faecium EF 412, EF 462 and EF 491 were selected for further detail studies and possibilities to be used as additives.

Published
2008
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17. Partial characterization of Enterococcus faecalis bacteriophage F4.

Author

Nigutová K, Styriak I, Javorský P, and Pristas P

Subjects
Bacteriophages physiology, Genome, Viral, Lysogeny, Molecular Sequence Data, Polymerase Chain Reaction, Sequence Analysis, DNA, Viral Proteins genetics, Bacteriophages classification, Bacteriophages genetics, Enterococcus faecalis virology
Abstract

Large Enterococcus faecalis F4 bacteriophage (described earlier) consisting of double-stranded linear DNA of approximately 60 kb was characterized. Library was prepared of its random DNA fragments and selected recombinants were sequenced. Three phage essential genes were characterized: DNA polymerase, replicative DNA helicase and a minor capsid protein, showing only limited homology to other known phage encoded genes. The occurrence of these genes among enterococci was determined by PCR method. Only two out of 40 tested isolates possessed all three genes, another three isolates contained at least one of the genes, demonstrating low frequency F4 lysogens among natural enterococcal isolates.

Published
2008
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18. Species of Enterococcus faecalis associated with free-living rodents.

Author

Laukova A, Strompfova V, Simonova M, Styriak I, and Swiecicka I

Subjects
Animals, Anti-Bacterial Agents pharmacology, Cattle, Enterococcus faecalis drug effects, Enterococcus faecalis genetics, Enterococcus faecalis metabolism, Fibronectins metabolism, Heparin metabolism, Lactoferrin metabolism, Microbial Sensitivity Tests, Poland, Protein Binding, Swine, Animals, Wild microbiology, Enterococcus faecalis isolation & purification, Rodentia microbiology
Abstract

Enterococci from different free-living rodents were isolated and selected. The strains were genotyped and their antibiotic sensitivity and /or resistance, production of lactic acid, urease activity, the presence of enterocin structural genes, plasmid detection, and their binding ability to proteins were determined. Among 24 enterococcal strains, 17 strains were allotted to the species Enterococcus faecalis by tDNA-PCR, 7 strains being not yet identified. Only Enterococcus sp. ES66 possessed the structural genes for the production of enterocins (Ent) A and P. E. faecalis EE61 had the gene for EntL50B. The other isolates were Ent-gene-free. Enterococci were mostly sensitive to antibiotic treatment . The plasmid DNA was detected only in the strain EE97. The average value of lactic acid production reached 896 +/- 90 micromol/L. Most of the strains possessed low ureolytic activity. Enterococci bound very well sub-epithelial proteins, reaching the value of 3 by the particle agglutination assay, especially concerning the heparin, bovine lactoferrin and porcine fibronectin.

Published
2008

19. Isolation of polymerase chain reaction-ready bacterial DNA from Lake Baikal sediments by carboxyl-functionalised magnetic polymer microspheres.

Author

Spanová A, Rittich B, Styriak I, Styriaková I, and Horák D

Subjects
Bacillus chemistry, DNA, Bacterial chemistry, Electrophoresis, Agar Gel, Fresh Water analysis, Polymerase Chain Reaction, DNA, Bacterial isolation & purification, Geologic Sediments analysis, Magnetics, Microspheres, Polymethacrylic Acids chemistry
Abstract

Carboxyl group-containing magnetic nonporous poly(2-hydroxyethyl methacrylate-co-ethylene dimethacrylate) (P(HEMA-co-EDMA)) microspheres were used for the isolation of polymerase chain reaction (PCR)-ready DNA from samples of Baikal sediments. DNA was isolated using the phenol extraction method or the Soil DNA Isolation Kit. The occurrence of false-negative results in PCR caused by the presence of extracellular inhibitors in DNA samples was solved using solid phase reversible DNA immobilisation. PCR-ready DNA was reversibly adsorbed to the microspheres in the presence of 8.0% (w/v) poly(ethylene glycol) (PEG 6000) and 2.0M sodium chloride concentrations. The adsorbed DNA was released from the microspheres in a low ionic strength TE buffer. The quality of isolated DNA was checked by PCR amplification.

Published
2006
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20. Weathering of phlogopite by Bacillus cereus and Acidithiobacillus ferrooxidans.

Author

Styriaková I, Bhatti TM, Bigham JM, Styriak I, Vuorinen A, and Tuovinen OH

Subjects
Acidithiobacillus growth & development, Aluminum analysis, Bacillus cereus growth & development, Iron analysis, Iron Compounds metabolism, Magnesium analysis, Potassium analysis, Silicon analysis, Acidithiobacillus metabolism, Aluminum Silicates chemistry, Bacillus cereus metabolism, Soil Microbiology
Abstract

The purpose of this study was to assess the weathering of finely ground phlogopite, a trioctahedral mica, by placing it in contact with heterotrophic (Bacillus cereus) and acidophilic (Acidithiobacillus ferrooxidans) cultures. X-ray diffraction analyses of the phlogopite sample before and after 24 weeks of contact in B. cereus cultures revealed a decrease in the characteristic peak intensities of phlogopite, indicating destruction of individual structural planes of the mica. No new solid phase products or interlayer structures were detected in B. cereus cultures. Acidithiobacillus ferrooxidans cultures enhanced the chemical dissolution of the mineral and formed partially weathered interlayer structures, where interlayer K was expelled and coupled with the precipitation of K-jarosite [KFe3(SO4)2(OH)6].

Published
2004
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21. Testing two Lactobacillus plantarum and Lactobacillus acidophilus strains for their suitability as a lipoid probiotic.

Author

Marsalková S, Cízek M, Vasil' M, Bomba A, Nad' P, Datelinka I, Jonecová Z, Rimková S, Kalinácová V, Styriak I, Bugarský A, and Gréserová G

Subjects
Animals, Bacillus growth & development, Cattle, Dairying methods, Escherichia coli growth & development, Female, Salmonella enteritidis growth & development, Staphylococcus aureus growth & development, Streptococcus growth & development, Antibiosis, Lactobacillus physiology, Lactobacillus acidophilus physiology, Mammary Glands, Animal microbiology, Probiotics
Abstract

Two strains of lactobacilli (Lactobacillus acidophilus T-135 and Lactobacillus plantarum 4/97) were selected in order to study their inhibitory properties against frequent udder pathogens (Escherichia coli, Staphylococcus aureus, Streptococcus agalactiae, Streptococcus uberis, Salmonella enteritidis and Bacillus pumilus), their production of organic acids as well as their ability to survive on the teat skin, the teat duct mucosa and in a lipoid emulsion. Both strains inhibited the tested pathogenic microbes and survived on the investigated surfaces and in an emulsion for more than 6 hours and 11 days, respectively.

Published
2004

22. Lectin-like binding of lactobacilli considered for their use in probiotical preparations for animal use.

Author

Styriak I and Nemcová R

Subjects
Animals, Cattle, Extracellular Matrix metabolism, Extracellular Matrix microbiology, Fibronectins metabolism, Hemagglutination, Lectins metabolism, Mucins metabolism, Protein Binding physiology, Swine, alpha-Fetoproteins metabolism, Bacterial Adhesion, Intestinal Mucosa microbiology, Lactobacillus metabolism, Probiotics
Abstract

Three gut lactobacilli from piglets (Lactobacillus plantarum L 5, Lactobacillus paracasei L 81, Lactobacillus fermentum L 670) and Lactobacillus casei subsp. pseudoplantarum L.c.) from a calf were examined by microtitre plate binding assay for their lectin-like binding activity after their cultivation on Rogosa agar and in MRS broth. Three ECM (extracellular matrix) molecules (fetuin, porcine fibronectin and porcine mucin) were selected for this assay. Additionally, the effect of heparin on the binding of these three ECM molecules by Lactobacillus strains in microtitre plates was tested. Moreover, haemagglutination tests with pig, cattle, sheep, and hen erythrocytes were performed. However, none of the four Lactobacillus strains examined did react with any of the erythrocytes tested. The differences between individual strains were observed in their binding to immobilised ECM molecules. The best adherent was the Lactobacillus plantarum L5, however, the other three strains showed also good ECM binding. With regard to an influence of cultivation medium on lectin-like binding activity, binding of all ECM molecules was expressed in Lactobacillus paracasei L 81 to significantly higher degree (P < 0.001) after cultivation on Rogosa agar than in MRS broth. Similarly, strains Lactobacillus fermentum L 670 and Lactobacillus casei subsp. pseudoplantarum L.c. displayed significantly higher (P < 0.001) binding of fibronectin and mucin after growth on Rogosa agar in comparison with MRS broth cultivation. However, no significant (on fetuin and fibronectin binding) or opposite effect (on mucin binding) of cultivation medium was observed in Lactobacillus plantarum L 5 strain. The influence of cultivation medium on fetuin binding by Lactobacillus fermentum L 670 was also not significant while Lactobacillus casei subsp. pseudoplantarum L.c. bound fetuin significantly better (P < 0.01) after growth on Rogosa agar. Heparin pretreatment increased the binding of the ECM molecules by the Lactobacillus fermentum L 670 strain significantly (P < 0.001 or P < 0.05) with the exception of porcine fibronectin when the strain was cultivated in MRS broth. This result is important especially in the connection with the previous observations that heparin decreased ECM binding of enteropathogens as staphylococci or clinical enterococcal isolates. Following up on some earlier strain characteristics, these results indicate that the selected lactobacilli are probably suitable for probiotic purposes.

Published
2003

23. Inhibitory effect of different enterocins against fecal bacterial isolates.

Author

Lauková A, Marenková M, and Styriak I

Subjects
Animals, Animals, Zoo, Antelopes, Bison, Bridged-Ring Compounds metabolism, Cattle, Colony Count, Microbial, Deer, Environmental Microbiology, Horses, Swine, Bridged-Ring Compounds pharmacology, Enterococcus drug effects, Enterococcus metabolism, Feces microbiology, Staphylococcus drug effects
Abstract

Anti-microbial activity of five different enterocins produced by ruminal and environmental enterococci against fecal bacterial isolates was tested. The majority of all 61 strains (80.4%) were inhibited by all enterocins used. The remaining strains were inhibited at least by one enterocin. The highest activity, 51,200 arbitrary units per ml-1 (AU ml-1) was measured when crude extracts of enterocin V24 (CE V24) were used against enterococci. CE AL41 and EK13 showed an activity of 25,600 AU ml-1. The lowest activity was obtained with Enterocin CE EC24 (100-400 AU ml-1). Crude extract of enterocin CCM4231 inhibited the indicator strains with an activity ranging from 100 up to 6400 AU ml-1, which is in accordance with our previous results. It further indicates the probable use of enterocins or its producers in environmental biotechnology with the aim to increase the effectiveness of sanitation of animal excrements after standard treatment.

Published
2003

24. Microbial binding and biodegradation of mycotoxins.

Author

Styriak I and Conková E

Subjects
Animals, Biodegradation, Environmental, Food Contamination analysis, Humans, Mycotoxins analysis, Mycotoxins metabolism, Mycotoxins poisoning
Abstract

This contribution provides an overview of literature data on the microbial binding and biodegradation of mycotoxins. These data and preliminary results from our own laboratory suggest that mycotoxin-bacterial binding or biodegradation is a realistic process and encourages the screening of bacterial strains and their biodegradation potential.

Published
2002

25. Lectin-like binding and antibiotic sensitivity of enterococci from wild herbivores.

Author

Styriak I, Lauková A, and Ljungh A

Subjects
Animals, Culture Media, Enterococcus metabolism, Extracellular Matrix metabolism, Microbial Sensitivity Tests, Periodic Acid pharmacology, Anti-Bacterial Agents pharmacology, Bison microbiology, Camelus microbiology, Enterococcus drug effects, Equidae microbiology, Lectins metabolism
Abstract

Fifty eight enterococcal isolates from wild herbivores were tested for their antibiotic sensitivity pattern and lectin-like binding of extracellular matrix (ECM) and serum proteins. Kanamycin resistance was very frequent; many multiresistant strains were also isolated. All isolates were sensitive to rifampicin. Resistance to gentamicin, novobiocin, and tetracycline was widely distributed in the microflora of wild herbivores breeded in zoological garden in Kosice. No autoaggregating strains were detected among these 58 enterococcal isolates. Various degrees of binding of mucins, fetuin, heparin, fibrinogen, and fibronectin were observed in individual strains. However, bovine lactoferrin binding by enterococci from deers and chamoises was either negative (0) or strongly positive (3). With regard to influence of growth media, TH agar was found to be better for the expression of lectin-like binding than blood agar, TH broth and Nutrient broth. A significant effect (P < 0.001 or P < 0.05) of proteolytic treatment was observed in six selected strains. However, there is a difference between the effect of trypsin and pronase P. Pronase treatment more effectively decreased binding of some strains (1H, 6A, EF 1111, EC 1292), while trypsin treatment decreased more binding of other enterococcal strains (EF 953 and 1E). Significant (P < 0.001) influence of metaperiodate, which cleaves the C-C bond between vicinal groups of sugars, on collagen I binding by three selected strains (1E, 1H, 6A) and bovine lactoferrin binding (by EF 1111, EC 1292, EF 953) was also observed. However, its influence was very different. In two strains (1H and EC 1292), ECM binding was decreased, while in four other strains (1E, 6A, EF 1111, EF 953) it was increased.

Published
2002
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26. Binding of E. coli isolates from pigs with postweaning diarrhea or edema disease to crude intestinal mucin of a weaned pig.

Author

Styriak I, Zatkovic B, and Kmet V

Subjects
Agar, Animals, Bacterial Proteins genetics, Base Sequence, Diarrhea microbiology, Diarrhea veterinary, Enterotoxins genetics, Escherichia coli physiology, Polymerase Chain Reaction veterinary, Swine, Bacterial Adhesion genetics, Edema Disease of Swine microbiology, Escherichia coli genetics, Escherichia coli Proteins, Fimbriae Proteins, Mucins physiology
Abstract

The presence of the fedA (gene coding F18 fimbriae) and genes coding STa and LTI enterotoxins and verotoxin Stx2v was determined in 30 E. coli strains isolated from weaned pigs with postweaning diarrhea (PWD) and edema disease (ED). The fedA gene was detected in 22 strains (73.3%). It was mostly associated with the presence of ST gene determinant (14 from 22 fedA positive strains, 63.6%). Two strains possessed ST/Stx2v or LTI/Stx2v combination of genes for both toxins and two strains were negative for investigated toxin determinants. Among 8 fedA-negative strains, five strains without gene determinants for toxins were detected. All 30 E. coli strains were investigated for their binding to crude intestinal mucin of a weaned pig fixed in wells of microtitre plates. Positive mucin binding was observed in most of strains, however, great differences were shown between individual strains. Nineteen strains were classified as strongly adherent, 10 strains as weakly adherent, and only one nonadherent strain was found. Three E. coli strains, selected among the best mucin binders, bound to mucin in a concentration-dependent manner. A high mucin binding by E. coli strains was observed only after their cultivation on blood agar plates. Their cultivation in LB broth or on McConkey agar plates had negative effect on the mucin binding by these strains. The mucin binding is not restricted by the presence of fedA gene because the strains displaying very good binding are found either among fedA positive (1, 602/2, 4/3, 576/6) or fedA negative (DK 6, DK 8) E. coli strains. E. coli strains with the highest mucin binding ability belong to potential ST producents (strains 1, 602/2, 4/3, 6/2, 602/4) while the strains without genes coding toxin production displayed lower binding to mucin substratum with exception of the strains ZV5 and 13.

Published
2001

27. The use of yeast for microbial degradation of some selected mycotoxins.

Author

Styriak I, Conková E, Kmec V, Böhm J, and Razzazi E

Abstract

Several biodegradation experiments were carried out using 10 different yeast strains.Saccharomyces spp., Kluyveromyces spp. andRhodotorula spp. were tested for biodegradation of selected mycotoxins (ochratoxin A, nivalenol, deoxynivalenol and fumonisin B1) standardsin vitro. There was confirmed that some yeast strains are able to degrade some mycotoxins. However, great differences between individual strains were observed. Moreover, 12Saccharomyces cerevisiae strains were tested for their potential capability to degrade zearalenone and fumonisins in Sabouraud broth. Two strains were capable to degrade zearalenone totally, one strain decreased the mycotoxin concentration up to 25%, and one strain up to 75% of original amount. Two strains were capable to degrade fumonisins partially.

Published
2001
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28. Binding of extracellular matrix proteins by lactobacilli.

Author

Styriak I, Zatkovic B, and Marsalková S

Subjects
Animals, Cattle, Collagen metabolism, Female, Stomach microbiology, Swine, Vagina microbiology, Extracellular Matrix Proteins metabolism, Lactobacillus metabolism
Abstract

Ten gut and ten vaginal Lactobacillus strains were investigated for their ability to bind type I collagen (Cn-I) and four selected gut lactobacilli were investigated for their binding to other extracellular matrix (ECM) molecules. Immobilized Cn-I (100 mg/L) in wells of microtitre plates was bound by all 10 autoaggregating vaginal strains and by 3 strains of gut lactobacilli from piglets in the range of A570 readings 0.114-1.806. L. acidophilus strain SV31 was much more adherent than the rest of strains. All four gut lactobacilli tested for binding to other ECM molecules displayed good binding to porcine fibronectin and heparin and some of them bound weakly to fetuin and porcine mucin. No binding of these strains was observed to bovine mucin, bovine fibrinogen and bovine lactoferrin.

Published
2001
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29. Lack of GATC sites in the genome of Streptococcus bovis bacteriophage F4.

Author

Styriak I, Pristas P, and Javorský P

Subjects
Animals, Binding Sites, DNA Restriction-Modification Enzymes, DNA, Viral analysis, Electrophoresis, Agar Gel, Bacteriophages genetics, Genome, Viral, Ruminants microbiology, Streptococcus bovis virology
Abstract

A strong bias against GATC sites was observed in the genome of phage F4, a lytic Streptococcus bovis bacteriophage. Only three GATC sites were found within the 60.4-kbp genome of this phage. The comparative lack of GATC sequences within the F4 genome was probably not due to dam methylation, as no modification within this site was detected using methylation-sensitive isoschizomer pair restriction endonuclease analysis. The short oligonucleotide composition of available S. bovis DNA sequences suggested the existence of an unknown mechanism for counterselection of GATC sites in S. bovis bacteriophages.

Published
2000
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30. Binding of selected extracellular matrix proteins to enterococci and Streptococcus bovis of animal origin.

Author

Styriak I, Lauková A, Fallgren C, and Wadström T

Subjects
Agglutination, Animals, Cattle, Coturnix, Enterococcus growth & development, Feces microbiology, Hemagglutination, Particle Size, Rabbits, Rumen microbiology, Streptococcus bovis growth & development, Surface Properties, Swine, Enterococcus metabolism, Extracellular Matrix Proteins metabolism, Streptococcus bovis metabolism
Abstract

Thirty-three enterococcal strains and 10 Streptococcus bovis strains were investigated for their protein-binding cell surface components. Seven extracellular matrix (ECM) proteins were immobilized on Difco latex beads to detect these components on the surface of all enterococcal strains and eight non-autoaggregating S. bovis strains by a particle agglutination assay (PAA). Twenty-three selected strains were also examined in microtiter plate assays. According to the absorbance readings (A(570nm)), 11 strains were classified as nonadherent (A(570nm) < 0.1), 10 strains as weakly adherent (0.1 < A(570nm) > 0.3), and 2 strains as strongly adherent (A(570nm) > 0.3) in these assays. A direct correlation was found between the values obtained in PAA and A(570nm) readings of microtiter plate assays. Binding of (125)I-labeled bovine lactoferrin to enterococci and streptococci was in the range of 6%-30% and of (125)I-labeled human vitronectin in the range of 9%-33% to streptococci. The binding of(125)I-labeled ECM proteins to selected strains was much more effectively inhibited by sulfated carbohydrates than by non-sulfated hyaluronic acid, indicating the importance of the sulfate groups of these inhibitors. An inhibition effect of heparin on bLf binding to four selected strains was higher in comparison with fucoidan in the microtiter plates. Thirty-five out of 44 strains had agglutinated rabbit erythrocytes. However, these strains showed no ability to agglutinate bovine or sheep erythrocytes.

Published
1999
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31. Collagen (Cn-I) binding by gut lactobacilli.

Author

Styriak I, Demecková V, and Nemcová R

Subjects
Animals, Ileum, Jejunum, Lactobacillus classification, Lactobacillus isolation & purification, Lacticaseibacillus casei metabolism, Collagen metabolism, Intestinal Mucosa microbiology, Lactobacillus metabolism, Swine microbiology
Abstract

Four gut Lactobacillus strains displaying the features which make them particularly promising for the preparation of probiotic products were investigated together with 5 fresh isolates and one collection strain of Lactobacillus plantarum for their ability to bind type I collagen (Cn-I). Immobilised Cn-I in microtitre plates was bound only by 3 strains of gut lactobacilli from piglets and the collection strain Lactobacillus plantarum LHI 10 from Prague in range of A570nm readings 0.114-0.221. Six strains (isolates from turkeys and a calf) did not bind Cn-I (A570nm < 0.1) in this assay. An influence of cultivation medium on Cn-I binding was significant (P < 0.001) in all four adherent strains. Significantly higher (P < 0.001) binding of Cn-I was observed for Lactobacillus casei L 81 and Lactobacillus plantarum LHI 10 grown on solid medium (MRS agar) than for MRS broth-grown cells, however, Lactobacillus plantarum L 5 and Lactobacillus fermentum L 435 expressed significantly (P < 0.001) higher Cn-I binding during cultivation in MRS broth. The specificity of the binding was confirmed because the Cn-I binding by lactobacilli after their preincubation with this protein was completely abolished. Three selected inhibitors (fucoidan, heparan sulphate and hyaluronic acid) significantly (P < 0.001) reduced Cn-I binding by the Lactobacillus plantarum L 5 strain. Following up on some earlier strain characteristics, these results suggest that the selected piglets lactobacilli are also able to bind Cn-I and therefore should antagonize collagen niche colonization by various enteropathogens when used for probiotic purposes.

Published
1999

32. Lack of surface receptors not restriction-modification system determines F4 phage resistance in Streptococcus bovis II/1.

Author

Styriak I, Pristas P, and Javorský P

Subjects
DNA, Viral isolation & purification, Streptococcus Phages ultrastructure, Streptococcus bovis ultrastructure, DNA Restriction-Modification Enzymes, Receptors, Virus, Streptococcus Phages growth & development, Streptococcus bovis virology
Abstract

The resistance of Streptococcus bovis strain II/1, the producer of SbvI restriction endonuclease, to F4 phage infection was demonstrated by the double-agar-layer method. Despite the presence of restriction endonuclease SbvI which can cleave F4 phage DNA to numerous fragments in vitro, the evidence that adsorption inhibition is the most important defence mechanism in phage resistance of S. bovis II/1 strain was obtained by adhesion experiments in vivo. Electron microscopy of phage-host mixtures showed many phage particles on the bacterial surface of phage-sensitive S. bovis 47/3 control strain in comparison with no phage particles seen on S. bovis II/1 (phage-resistant) strain surface.

Published
1998
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33. Occurrence of Fusarium sacchari var. subglutinans and its mycotoxin production ability in broiler feed.

Author

Styriak I, Conková E, and Böhm J

Subjects
Animals, Aspergillus isolation & purification, Chickens, Mucor isolation & purification, Penicillium isolation & purification, Slovakia, Spores, Fungal isolation & purification, Animal Feed microbiology, Fusarium isolation & purification, Fusarium metabolism, Mycotoxins biosynthesis
Abstract

Spores of Fusarium sacchari var. subglutinans isolated from broiler feed BR1 were obtained at an average concentration of 1.5/mg in 25% of tested samples. The spore concentration was increased from 1 to 100/mg of solid substrate (BR2; biscuit) or to 1/nL of Sabouraud broth after 3 weeks of cultivation. Mycotoxin analyses of these three substrates showed negative reactions for T-2 toxin and zearalenone but a positive reaction for deoxynivalenol (DON) which was found in concentrations of 5 ppm in Sabouraud broth, 50 ppm in BR2 and 220 ppm in biscuit. Therefore, our F. sacchari isolate appeared to be a DON producer.

Published
1994
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34. Isolation and partial characterization of three rumen Lactobacillus plantarum bacteriophages.

Author

Nemcová R, Styriak I, Stachová M, and Kmet V

Subjects
Acetates pharmacology, Animals, Bacteriophages drug effects, Bacteriophages ultrastructure, Cattle, DNA, Viral metabolism, Deoxyribonucleases, Type II Site-Specific metabolism, Gastrointestinal Contents, Hot Temperature, Viral Plaque Assay, Bacteriophages isolation & purification, Lactobacillus, Rumen microbiology
Abstract

The first isolation of Lactobacillus plantarum bacteriophages from ruminal fluid is reported. Three bacteriophages were characterized on the basis of plaque morphology, host ranges, stability, electron microscopic morphology and DNA restriction endonuclease digestion patterns. They formed clear plaques and are placed in group A of Bradley's scheme and have identical host ranges. Bacteriophages were stable to urea and chloroform. They were relatively thermostable but partially inactivated by rumen fluid and by acetate. DNA restriction analysis showed that phage L20 had different numbers of cleavage sites in comparison with the next two phages.

Published
1993

35. Adherence of ruminal Streptococcus bovis and Lactobacillus strains to primary and secondary cultures of rumen epithelium.

Author

Styriak I, Gálfi P, and Kmet V

Subjects
Animals, Cattle, Culture Techniques, Epithelium microbiology, Sheep, Species Specificity, Bacterial Adhesion physiology, Lactobacillus physiology, Rumen microbiology, Streptococcus bovis physiology
Abstract

Six strains of rumen Lactobacillus and four Streptococcus bovis strains isolated from rumen wall and fluid samples were examined for the adherence to cells of primary and secondary cultures of ruminal epithelium (REC) prepared from sheep and calf. S. bovis adhered to the keratinized REC. Ruminal lactobacilli did not adhere. The presence of rumen lactobacilli in mixture had no influence on the adherence of S. bovis strains. No difference was observed in the adherence of tested bacteria to epithelial cells of primary or secondary cultures, but adhesion was only detected on keratinized cells.

Published
1992

36. Preliminary observations of interaction between bacteriophages and Streptococcus bovis bacteria on ruminal epithelium primoculture.

Author

Styriak I, Gálfi P, and Kmet V

Subjects
Animals, Cattle, Cells, Cultured, Epithelium microbiology, Streptococcus bovis metabolism, Bacterial Adhesion, Bacteriophages physiology, Rumen microbiology, Streptococcus bovis physiology
Abstract

Five Streptococcus bovis strains (47/3, 59/2, 4/1, 46/2 and 44/9) isolated from calf ruminal fluid samples were examined for the adherence to cultured ruminal epithelium cells. Four strains (47/3, 59/2, 4/1 and 46/2) were able to attach to the cultured epithelial cells. However, S. bovis 47/3 strain attached to the target cells in significantly greater numbers than the other strains. Strain 44/9 did not adhere to cells of ruminal epithelium. The adherent bacteria were observed on the surface of differentiated (mainly keratinized) cells of ruminal epithelium primoculture only. The different effect of F4, F5 and F6 bacteriophages was ascertained on S. bovis bacteria adhering to rumen epithelial primoculture. A significant decrease in the number of adherent bacteria was shown after cultivation of strains 47/3 and 4/1 with F6 bacteriophage and of 47/3 strain with F4 phage. The F5 bacteriophage had no significant effect on these bacteria.

Published
1991
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37. Isolation and characterization of two rumen Streptococcus bovis bacteriophages.

Author

Styriak I, Kmet V, and Spanova A

Subjects
Animals, Bacteriophages classification, Bacteriophages growth & development, Bacteriophages ultrastructure, Cattle, DNA, Viral analysis, Microscopy, Electron, Restriction Mapping, Streptococcus, Bacteriophages isolation & purification, Rumen microbiology
Abstract

A method for the isolation of Streptococcus bovis bacteriophages from ruminal fluid of calves is described. Thirty to 2 x 10(3) phages per ml infecting Streptococcus bovis strains 4/1 and 47/3 were isolated directly from ruminal fluid. Two bacteriophages were characterized on the basis of plaque morphology, host ranges, electron microscopic morphology and DNA restriction endonuclease digestion patterns. The F1 and F3 phages formed clear plaques of different sizes. The plaque size of the F1 phage was about 1-1.5 mm in diameter, while the plaques of the F3 phage were larger (1.5-2.5 mm in diameter). Both phages are placed in group B of Bradley's scheme and have different host ranges. The first isolation of Streptococcus bovis phage DNA is reported. Restriction analysis of their DNAs showed that phages F1 and F3 had different numbers of cleavage sites in their genomes and that they were not identical.

Published
1989

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