Your search keyword '"Ebrahim Razzazi-Fazeli"' showing total 104 results

1. Bos d 13, a novel heat‐stable beef allergen

Author

Patricia Román‐Carrasco, Christoph Klug, Wolfgang Hemmer, Margarete Focke‐Tejkl, Marianne Raith, Isabella Grosinger, Peter Stoll, Santiago Quirce, Marta Sanchez‐Jareño, Mónica Martínez‐Blanco, Elena Molina, Veronika Somoza, Barbara Lieder, Zana Marin, Katharina Nöbauer, Karin Hummel, Ebrahim Razzazi‐Fazeli, and Ines Swoboda

Subjects

Food Science, Biotechnology

Published

2023

2. The emerging pathogen Paecilomyces variotii ‐ a novel and important fungal allergen source

Author

Clara San Bartolome, Rosa Muñoz-Cano, Margarete Focke-Tejkl, Sandra Pfeiffer, Katja Sterflinger, Santiago Quirce, Marianne Raith, Katharina Nöbauer, Ines Swoboda, Ebrahim Razzazi-Fazeli, and Mariona Pascal

Subjects

biology, Immunology, Byssochlamys, Allergens, medicine.disease_cause, biology.organism_classification, Paecilomyces variotii, Microbiology, Emerging pathogen, Allergen, medicine, Humans, Immunology and Allergy, Paecilomyces

Published

2021

3. Diet and phytogenic supplementation substantially modulate the salivary proteome in dairy cows

Author

Ezequias Castillo-Lopez, Cátia Pacífico, Arife Sener-Aydemir, Karin Hummel, Katharina Nöbauer, Sara Ricci, Raul Rivera-Chacon, Nicole Reisinger, Ebrahim Razzazi-Fazeli, Qendrim Zebeli, and Susanne Kreuzer-Redmer

Subjects

Biophysics, Biochemistry

Abstract

Phytogenic compounds may influence salivation or salivary properties. However, their effects on the bovine salivary proteome have not been evaluated. We investigated changes in the bovine salivary proteome due to transition from forage to high-concentrate diet, with and without supplementation with a phytogenic feed additive. Eight non-lactating cows were fed forage, then transitioned to a 65% concentrate diet (DM basis) over a week. Cows were control (n = 4, CON) or supplemented with a phytogenic feed additive (n = 4, PHY). Proteomic analysis was conducted using liquid chromatography coupled with mass spectrometry. We identified 1233 proteins; 878 were bovine proteins, 189 corresponded to bacteria, and 166 were plant proteins. Between forage and high-concentrate, 139 proteins were differentially abundant (P 0.05), with 48 proteins having a log2FC difference |2|. The salivary proteome reflected shifts in processes involving nutrient utilization, body tissue accretion, and immune response. Between PHY and CON, 195 proteins were differently abundant (P 0.05), with 37 having a log2FC difference |2|; 86 proteins were increased by PHY, including proteins involved in smell recognition. Many differentially abundant proteins correlated (r |0.70|) with salivary bicarbonate, total mucins or pH. Results provide novel insights into the bovine salivary proteome using a non-invasive approach, and the association of specific proteins with major salivary properties influencing rumen homeostasis. SIGNIFICANCE: Phytogenic compounds may stimulate salivation due to their olfactory properties, but their effects on the salivary proteome have not been investigated. We investigated the effect of high-concentrate diets and supplementation with a phytogenic additive on the salivary proteome of cows. We show that analysis of cows' saliva can be a non-invasive approach to detect effects occurring not only in the gut, but also systemically including indications for gut health and immune response. Thus, results provide unique insights into the bovine salivary proteome, and will have a crucial contribution to further understand animal response in terms of nutrient utilization and immune activity due to the change from forage to a high-energy diet. Additionally, our findings reveal changes due to supplementation with a phytogenic feed additive with regard to health and olfactory stimulation. Furthermore, findings suggest an association between salivary proteins and other components like bicarbonate content.

Published

2022

4. Identification of Ulocladium chartarum as an important indoor allergen source

Author

Katja Sterflinger, Katharina Nöbauer, Margarete Focke-Tejkl, Ebrahim Razzazi-Fazeli, Mariona Pascal, Clara San Bartolome, Peter Sandler, Marianne Raith, Santiago Quirce, Rosa Muñoz-Cano, Ines Swoboda, and Sandra Pfeiffer

Subjects

Immunology, Alternaria, Allergens, Biology, Mould allergy, medicine.disease_cause, Microbiology, Allergen, Air Pollution, Indoor, Hypersensitivity, medicine, Humans, Immunology and Allergy, Identification (biology), Ulocladium chartarum

Published

2021

5. Elucidation of putative binding partners for the protein encoded by ORF149 of cyprinid herpesvirus 3 in goldfish ( Carassius auratus )

Author

Sven Bergmann, Simon Menanteau–Ledouble, Mansour El-Matbouli, Michael Gotesman, and Ebrahim Razzazi-Fazeli

Subjects

Short Communication, Veterinary (miscellaneous), Cyprinid herpesvirus 3, ved/biology.organism_classification_rank.species, Short Communications, Plasma protein binding, Aquatic Science, Mitochondrion, LC‐MS/MS, Fish Diseases, Viral Proteins, Goldfish, antibody, protein purification, Protein purification, Lc ms ms, Carassius auratus, Animals, Cytoskeleton, Herpesviridae, biology, ved/biology, Herpesviridae Infections, mitochondria, Biochemistry, biology.protein, Antibody, cytoskeletal, Protein Binding

Published

2020

6. Author Correction: Shotgun proteomics reveals putative polyesterases in the secretome of the rock-inhabiting fungus Knufia chersonesos

Author

Georg M. Guebitz, Felice Quartinello, Doris Ribitsch, Katja Sterflinger, Ebrahim Razzazi-Fazeli, Katharina Nöbauer, and Donatella Tesei

Subjects

Geologic Sediments, Multidisciplinary, biology, Proteome, Protein Conformation, Hydrolysis, Polyesters, lcsh:R, Esterases, lcsh:Medicine, Fungus, Computational biology, biology.organism_classification, Fungal Proteins, Ascomycota, lcsh:Q, lcsh:Science, Shotgun proteomics, Author Correction

Abstract

Knufia chersonesos is an ascomycotal representative of black fungi, a morphological group of polyextremotolerant melanotic fungi, whose ability to resort to recalcitrant carbon sources makes it an interesting candidate for degradation purposes. A secretome screening towards polyesterases was carried out for the fungus and its non-melanized mutant, grown in presence of the synthetic copolyester Polybutylene adipate terephthalate (PBAT) as additional or sole carbon source, and resulted in the identification of 37 esterolytic and lipolytic enzymes across the established cultivation conditions. Quantitative proteomics allowed to unveil 9 proteins being constitutively expressed at all conditions and 7 which were instead detected as up-regulated by PBAT exposure. Protein functional analysis and structure prediction indicated similarity of these enzymes to microbial polyesterases of known biotechnological use such as MHETase from Ideonella sakaiensis and CalA from Candida albicans. For both strains, PBAT hydrolysis was recorded at all cultivation conditions and primarily the corresponding monomers were released, which suggests degradation to the polymer's smallest building block. The work presented here aims to demonstrate how investigations of the secretome can provide new insights into the eco-physiology of polymer degrading fungi and ultimately aid the identification of novel enzymes with potential application in polymer processing, recycling and degradation.

Published

2020

7. Effects of Yersinia ruckeri invasion on the proteome of the Chinook salmon cell line CHSE-214

Author

Mansour El-Matbouli, Ebrahim Razzazi-Fazeli, Simon Menanteau-Ledouble, and Katharina Nöbauer

Subjects

0301 basic medicine, Fish Proteins, Yersinia ruckeri, Embryo, Nonmammalian, Integrin beta Chains, Proteome, Yersinia Infections, Cellular microbiology, lcsh:Medicine, Biology, Article, Bacterial Adhesion, Microbiology, Cell Line, Applied microbiology, 03 medical and health sciences, Fish Diseases, 0302 clinical medicine, Salmon, Animals, HSP90 Heat-Shock Proteins, lcsh:Science, Pathogen, Multidisciplinary, Cell adhesion molecule, Intracellular parasite, Gene Expression Profiling, lcsh:R, Embryo, Molecular Sequence Annotation, HSP40 Heat-Shock Proteins, biology.organism_classification, 030104 developmental biology, Gene Ontology, Gene Expression Regulation, Cell culture, 030220 oncology & carcinogenesis, Host-Pathogen Interactions, lcsh:Q, Pathogens

Abstract

Yersinia ruckeri is an important bacterial pathogen of fish, in particular salmonids, it has been associated with systemic infections worldwide and, like many enteric bacteria, it is a facultative intracellular pathogen. However, the effect of Y. ruckeri’s interactions with the host at the cellular level have received little investigation. In the present study, a culture of Chinook Salmon Embryo (CHSE) cell line was exposed to Y. ruckeri. Afterwards, the proteins were investigated and identified by mass spectrometry and compared to the content of unexposed cultures. The results of this comparison showed that 4.7% of the identified proteins were found at significantly altered concentrations following infection. Interestingly, infection with Y. ruckeri was associated with significant changes in the concentration of surface adhesion proteins, including a significantly decreased presence of β-integrins. These surface adhesion molecules are known to be the target for several adhesion molecules of Yersiniaceae. The concentration of several anti-apoptotic regulators (HSP90 and two DNAj molecules) appeared similarly downregulated. Taken together, these findings suggest that Y. ruckeri affects the proteome of infected cells in a notable manner and our results shed some light on the interaction between this important bacterial pathogen and its host.

Published

2020

8. ECM Characterization Reveals a Massive Activation of Acute Phase Response during FSGS

Author

Christoph Aufricht, Christoph Kornauth, Klaus Kratochwill, Sigurd Krieger, Nicole Huttary, Helga Schachner, Christoph A. Gebeshuber, Ebrahim Razzazi Fazeli, André Oszwald, Gábor Szénási, Eva Nora Bukosza, Karin Hummel, Katharina Nöbauer, and Péter Hamar

Subjects

0301 basic medicine, Candidate gene, 030232 urology & nephrology, Fibrinogen, urologic and male genital diseases, lcsh:Chemistry, Mice, 0302 clinical medicine, Focal segmental glomerulosclerosis, sclerosis, lcsh:QH301-705.5, Spectroscopy, Mice, Inbred BALB C, Glomerulosclerosis, Focal Segmental, Glomerular basement membrane, General Medicine, female genital diseases and pregnancy complications, Computer Science Applications, Extracellular Matrix, medicine.anatomical_structure, Proteome, Slit diaphragm, medicine.drug, Mice, Transgenic, Biology, Catalysis, Article, Inorganic Chemistry, 03 medical and health sciences, acute phase response, medicine, Animals, Protease Inhibitors, Physical and Theoretical Chemistry, Molecular Biology, complement system, ECM, urogenital system, Organic Chemistry, Complement System Proteins, medicine.disease, Complement system, Disease Models, Animal, MicroRNAs, FSGS, 030104 developmental biology, lcsh:Biology (General), lcsh:QD1-999, Gene Expression Regulation, Cancer research, Homeostasis

Abstract

The glomerular basement membrane (GBM) and extra-cellular matrix (ECM) are essential to maintain a functional interaction between the glomerular podocytes and the fenestrated endothelial cells in the formation of the slit diaphragm for the filtration of blood. Dysregulation of ECM homeostasis can cause Focal segmental glomerulosclerosis (FSGS). Despite this central role, alterations in ECM composition during FSGS have not been analyzed in detail yet. Here, we characterized the ECM proteome changes in miR-193a-overexpressing mice, which suffer from FSGS due to suppression of Wilms’ tumor 1 (WT1). By mass spectrometry we identified a massive activation of the acute phase response, especially the complement and fibrinogen pathways. Several protease inhibitors (ITIH1, SERPINA1, SERPINA3) were also strongly increased. Complementary analysis of RNA expression data from both miR-193a mice and human FSGS patients identified additional candidate genes also mainly involved in the acute phase response. In total, we identified more than 60 dysregulated, ECM-associated genes with potential relevance for FSGS progression. Our comprehensive analysis of a murine FSGS model and translational comparison with human data offers novel targets for FSGS therapy.

Published

2020

9. Pharmacokinetics of harpagoside in horses after intragastric administration of a Devil's claw (Harpagophytum procumbens) extract

Author

Karin Hummel, S Axmann, Katharina Nöbauer, Ebrahim Razzazi-Fazeli, and Karin Zitterl-Eglseer

Subjects

Male, 040301 veterinary sciences, Cmax, Anti-Inflammatory Agents, Harpagophytum, 0403 veterinary science, 03 medical and health sciences, Random Allocation, 0302 clinical medicine, Devil's claw, Pharmacokinetics, Intragastric administration, Harpagophytum procumbens, Scientific Papers, Medicine, Animals, Glycosides, Horses, Intubation, Gastrointestinal, Pyrans, Pharmacology, harpagoside, Harpagoside, Cross-Over Studies, General Veterinary, biology, Traditional medicine, business.industry, Plant Extracts, Horse, 04 agricultural and veterinary sciences, biology.organism_classification, horse, Original Article, Female, business, pharmacokinetics, 030217 neurology & neurosurgery, Devil's Claw

Abstract

Devil's claw is used for the treatment of inflammatory symptoms and degenerative disorders in horses since many years, but without the substantive pharmacokinetic data. The pharmacokinetic parameters of harpagoside, the main active constituent of Harpagophytum procumbens DC ex Meisn., were evaluated in equine plasma after administration of Harpagophytum extract FB 8858 in an open, single‐dose, two‐treatment, two‐period, randomized cross‐over design. Six horses received a single dose of Harpagophytum extract, corresponding to 5 mg/kg BM harpagoside, and after 7 days washout period, 10 mg/kg BM harpagoside via nasogastric tube. Plasma samples at certain time points (before and 0–24 hr after administration) were collected, cleaned up by solid‐phase extraction, and harpagoside concentrations were determined by LC‐MS/MS using apigenin‐7‐glucoside as internal standard. Plasma concentration‐time data and relevant parameters were described by noncompartmental model through PKSolver software. Harpagoside could be detected up to 9 hr after administration. C max was found at 25.59 and 55.46 ng/ml, t 1/2 at 2.53 and 2.32 hr, respectively, and t max at 1 hr in both trials. AUC 0–inf was 70.46 and 117.85 ng hr ml−1, respectively. A proportional relationship between dose, C max and AUC was observed. Distribution (V z/F) was 259.04 and 283.83 L/kg and clearance (CL/F) 70.96 and 84.86 L hr−1 kg−1, respectively. Treatment of horses with Harpagophytum extract did not cause any clinically detectable side effects.

Published

2018

10. Alterations in haemolymph proteome of Mytilus galloprovincialis mussel after an induced injury

Author

Sarah Schlosser, José J. Cerón, Asta Tvarijonaviciute, Ebrahim Razzazi-Fazeli, Damián Escribano, Diego Romero, Lorena Franco-Martínez, Katharina Nöbauer, and Silvia Martínez-Subiela

Subjects

0301 basic medicine, Proteome, Trolox equivalent antioxidant capacity, 010501 environmental sciences, Aquatic Science, Biology, medicine.disease_cause, 01 natural sciences, Superoxide dismutase, 03 medical and health sciences, Hemolymph, Heat shock protein, Myosin, medicine, Animals, Environmental Chemistry, Acute-Phase Reaction, 0105 earth and related environmental sciences, Mytilus, General Medicine, biology.organism_classification, Tropomyosin, Immunity, Innate, High-Throughput Screening Assays, Oxidative Stress, 030104 developmental biology, Biochemistry, biology.protein, Creatine kinase, Biomarkers, Oxidative stress

Abstract

A proteomic and biochemical approach was performed to assess the effects of an induced muscle injury on the haemolymph of bivalve molluscs. For this purpose, Mytilus galloprovincialis were exposed to puncture of adductor muscle for three consecutive days, and their haemolymph proteome was then compared to healthy animals using 2-dimensional electrophoresis (2-DE) to identify proteins that differed significantly in abundance. Those proteins were then subjected to tandem mass spectrometry and 6 proteins, namely myosin, tropomyosin, CuZn superoxide dismutase (SOD), triosephosphate isomerase, EP protein and small heat shock protein were identified. SOD and tropomyosin changes were verified by spectrophotometric measurements and western blotting, respectively. As some of the proteins identified are related to muscular damage and oxidative stress, other biomarkers associated with these processes that can be evaluated by automatic biochemical assays were measured including troponin, creatine kinase (CK), and aspartate aminotransferase (AST) for muscle damage, and SOD, trolox equivalent antioxidant capacity (TEAC) and esterase activity (EA) for oxidative stress. Significantly higher concentrations of troponin, CK, AST, and TEAC were observed in mussels after puncture, being also possible biomarkers of non-specific induced damage.

Published

2018

11. Toxicity of DDT to the hooded oyster Saccostrea cucullata: Mortality, histopathology and molecular mechanisms as revealed by a proteomic approach

Author

Karin Hummel, Katharina Nöbauer, Jisnuson Svasti, Daranee Chokchaichamnankit, Supatta Chueycham, Sutin Kingtong, Ebrahim Razzazi-Fazeli, Omid Hekmat, and Chantragan Srisomsap

Subjects

Proteomics, Oyster, Proteome, Health, Toxicology and Mutagenesis, Histopathology, Connective tissue, Context (language use), DTT exposure, Toxicology, Environmental pollution, DDT, Microbiology, Hooded oyster, Tandem Mass Spectrometry, biology.animal, medicine, Animals, GE1-350, biology, Public Health, Environmental and Occupational Health, General Medicine, biology.organism_classification, Ostreidae, Pollution, Environmental sciences, medicine.anatomical_structure, TD172-193.5, Molecular Response, Toxicity, Water Pollutants, Chemical, Chromatography, Liquid

Abstract

Dichlorodiphenyltrichloroethane (DDT), a persistent organochlorine pesticide, has been linked to adverse biological effects in organisms. However, there is limited knowledge about its toxic effects on marine organisms and the underlying molecular mechanisms. This study investigated the toxic effects of DDT in the hooded oyster Saccostrea cucullata. The oysters were exposed to DDT at concentrations of 0, 10, 50, 100, 500, 1000 and 2000 µg/L for 96 h and the LC50 (96 h) was 891.25 µg/L. Two sublethal concentrations (10 and 100 µg/L) were used to investigate the histopathological effects and the proteome response. Histopathological results showed that DDT caused the alteration of mantle tissue. This included the induction of mucocytes in the epithelium and the inflammatory effect in the connective tissue indicated by the enlargement of blood sinus and hemocyte aggregation within the sinus. Proteomic results showed that, amongst approximately 500 protein spots that were detected across 2DE gels, 51 protein spots were differentially expressed (P 1.2). Of these, 29 protein spots were identified by LC-MS/MS. These included 23 up-regulated, 5 down-regulated and 1 fluctuating spots. Thus, we observed that stress response and cytoskeletal proteins are the central targets of DDT action. Furthermore, DDT alters the expression of proteins involved in energy metabolism, calcium homeostasis and other proteins of unknown function. Additionally, proteomic results clearly elucidated the molecular response of the histopathological changes which were driven by the alteration of cytoskeletal proteins. Our results improve the current knowledge of toxicity of the DDT to histology and molecular response of oyster proteome to DDT exposure. In addition, histopathological changes will be beneficial for the development of an appropriate guideline for health assessment of this species in ecotoxicological context.

Published

2021

12. Devil’s claw (Harpagophytum procumbens) – Pharmacokinetics of harpagoside in horses

Author

Katharina Nöbauer, S Axmann, Ebrahim Razzazi-Fazeli, Karin Hummel, and Karin Zitterl-Eglseer

Subjects

Harpagoside, Devil's claw, Pharmacokinetics, Traditional medicine, Harpagophytum procumbens, Chemistry

Published

2019

13. Pharmacokinetic Study of Bioactive Glycopeptide from Strongylocentrotus droebachiensis After Intranasal Administration to Rats Using Biomarker Approach

Author

Valery G. Makarov, V. M. Kosman, Ebrahim Razzazi-Fazeli, Johannes Novak, Alexander N. Shikov, Olga N. Pozharitskaya, and Natalia M. Faustova

Subjects

Male, kidney, strongylocentrotus droebachiensis, Cmax, Strongylocentrotus droebachiensis, Biological Availability, Pharmaceutical Science, Spleen, Pharmacology, liver, 01 natural sciences, Article, 03 medical and health sciences, chemistry.chemical_compound, Pharmacokinetics, Lactate dehydrogenase, Drug Discovery, medicine, Animals, Tissue Distribution, Pharmacology, Toxicology and Pharmaceutics (miscellaneous), lcsh:QH301-705.5, Administration, Intranasal, plasma, Strongylocentrotus, 030304 developmental biology, 0303 health sciences, Kidney, Glycopeptides, Area under the curve, nose mucosa, Glycopeptide, 0104 chemical sciences, rats, 010404 medicinal & biomolecular chemistry, medicine.anatomical_structure, chemistry, lcsh:Biology (General), Area Under Curve, Injections, Intravenous, striated muscle, Nasal administration, spleen, Biomarkers

Abstract

A glycopeptide fraction (GPF) from internal organs of green sea urchins (Strongylocentrotus droebachiensis M&uuml, ller, Strongylocentrotidae) has been reported to be an effective bronchitis treatment. In this study, we evaluated the pharmacokinetic and tissue distribution of GPF, following single and repeated intranasal (i/n) administration over the course of seven days in rats. The method measuring lactate dehydrogenase as biomarker was used to analyse the plasma and tissue concentrations of GPF. GPF appears in the plasma 15 min after single i/n administration (100 &micro, g/kg) and reaches its maximum at 45 min. The area under the curve (AUC)0&ndash, 24 and Cmax were similar using both i/n and intravenous administration, while mean residence time (MRT) and T1/2 after i/n administration were significantly higher compared with intravenous (i/v) administration. The absolute bioavailability of GPF after i/n administration was 89%. The values of tissue availability (ft) provided evidence about the highest concentration of GPF in the nose mucosa (ft = 34.9), followed by spleen (ft = 4.1), adrenal glands (ft = 3.8), striated muscle (ft = 1.8), kidneys (ft = 0.5), and liver (ft = 0.3). After repeated dose administration, GPF exhibited significantly higher AUC0&ndash, 24 and MRT, indicating its accumulation in the plasma.

Published

2019

14. Author Correction: Regulation of volatile and non-volatile pheromone attractants depends upon male social status

Author

Ken Luzynski, Dustin J. Penn, V. M. Enk, I Ortner, Ebrahim Razzazi-Fazeli, J Kwak, and Michaela Thoß

Subjects

Male, 0303 health sciences, Volatile Organic Compounds, Multidisciplinary, Reproduction, lcsh:R, lcsh:Medicine, Biology, Pheromones, Animal Communication, 03 medical and health sciences, Mice, 0302 clinical medicine, ComputingMethodologies_DOCUMENTANDTEXTPROCESSING, Pheromone, Animals, lcsh:Q, Female, lcsh:Science, Author Correction, Social Behavior, 030217 neurology & neurosurgery, 030304 developmental biology, Demography, Social status

Abstract

We investigated the regulation of chemical signals of house mice living in seminatural social conditions. We found that male mice more than doubled the excretion of major urinary proteins (MUPs) after they acquired a territory and become socially dominant. MUPs bind and stabilize the release of volatile pheromone ligands, and some MUPs exhibit pheromonal properties themselves. We conducted olfactory assays and found that female mice were more attracted to the scent of dominant than subordinate males when they were in estrus. Yet, when male status was controlled, females were not attracted to urine with high MUP concentration, despite being comparable to levels of dominant males. To determine which compounds influence female attraction, we conducted additional analyses and found that dominant males differentially upregulated the excretion of particular MUPs, including the pheromone MUP20 (darcin), and a volatile pheromone that influences female reproductive physiology and behavior. Our findings show that once male house mice become territorial and socially dominant, they upregulate the amount and types of excreted MUPs, which increases the intensities of volatiles and the attractiveness of their urinary scent to sexually receptive females.

Published

2019

15. Separation of HIV‐1 gag virus‐like particles from vesicular particles impurities by hydroxyl‐functionalized monoliths

Author

Eva Berger, Alois Jungbauer, Katharina Nöbauer, Miriam Klausberger, Ebrahim Razzazi-Fazeli, Daniel Burgstaller, Andres Tover, Petra Steppert, and Petra Kramberger

Subjects

Proteomics, 0301 basic medicine, Ammonium sulfate, Gene Products, gag, Filtration and Separation, Fraction (chemistry), Chemistry Techniques, Analytical, Analytical Chemistry, law.invention, 03 medical and health sciences, chemistry.chemical_compound, law, Humans, Vaccines, Virus-Like Particle, Monolith, Cells, Cultured, Filtration, geography, Downstream processing, Chromatography, geography.geographical_feature_category, Hydroxyl Radical, Elution, Chemistry, 030104 developmental biology, Mixed-mode chromatography, Membrane, HIV-1, Hydrophobic and Hydrophilic Interactions

Abstract

The downstream processing of enveloped virus-like particles is very challenging because of the biophysical and structural similarity between correctly assembled particles and contaminating vesicular particles present in the feedstock. We used hydroxyl-functionalized polymethacrylate monoliths, providing hydrophobic and electrostatic binding contributions, for the purification of HIV-1 gag virus-like particles. The clarified culture supernatant was conditioned with ammonium sulfate and after membrane filtration loaded onto a 1 mL monolith. The binding capacity was 2 × 1012 /mL monolith and was only limited by the pressure drop. By applying either a linear or a step gradient elution, to decrease the ammonium sulfate concentration, the majority of double-stranded DNA (88-90%) and host cell protein impurities (39-61%) could be removed while the particles could be separated into two fractions. Proteomic analysis and evaluation of the p24 concentration showed that one fraction contained majority of the HIV-1 gag and the other fraction was less contaminated with proteins originated from intracellular compartments. We were able to process up to 92 bed volumes of conditioned loading material within 3 h and eluted in average 7.3 × 1011 particles per particle fraction, which is equivalent to 730 vaccination doses of 1 × 109 particles.

Published

2017

16. Exploring the oviductal fluid proteome by a lectin-based affinity approach

Author

Gottfried Brem, Urban Besenfelder, Hans Yu, Konstantin A. Artemenko, Ebrahim Razzazi-Fazeli, Judith Reiser, Jonas Bergquist, and Corina Mayrhofer

Subjects

Male, 0301 basic medicine, Spectrometry, Mass, Electrospray Ionization, Proteome, Wheat Germ Agglutinins, Peptide, Biochemistry, Workflow, 03 medical and health sciences, Concanavalin A, Animals, Molecular Biology, Fallopian Tubes, Glycoproteins, chemistry.chemical_classification, biology, Reproducibility of Results, Lectin, Molecular biology, Wheat germ agglutinin, Body Fluids, Staining, 030104 developmental biology, Enzyme, chemistry, biology.protein, Female, Rabbits, Glycoprotein

Abstract

The analysis of glycoproteins in body fluids represents a central task in the study of vital processes. Herein, we assessed the combined use of Concanavalin A and Wheat Germ Agglutinin as ligands to fractionate and enrich glycoproteins from oviductal fluid (OF), which is a source of molecules involved in fertilization. First, the selectivity was corroborated by a gel-based approach using glycoprotein staining and enzymatic deglycosylation. Nanoliquid chromatography-tandem mass spectrometry (nLC-ESI-MS/MS) further allowed the reliable identification of 134 nonbound as well as 130 lectin-bound OF proteins. Enrichment analysis revealed that 77% of the annotated proteins in the lectin-bound fraction were known glycoproteins (p-value [FDR] = 1.45E-31). The low variance of the number of peptide spectrum matches for each protein within replicates indicated a consistent reproducibility of the whole workflow (median CV 17.3% for technical replicates and 20.7% for biological replicates). Taken together, this study highlights the applicability of a lectin-based workflow for the comprehensive analysis of OF proteins and gives for the first time an insight into the broad glycoprotein content of OF.

Published

2016

17. Growth promotion in pigs by oxytetracycline coincides with down regulation of serum inflammatory parameters and of hibernation-associated protein HP-27

Author

Ebrahim Razzazi-Fazeli, Theo Niewold, Karin Hummel, Damián Escribano, Ingrid Miller, Flemming Jessen, and Laura Soler

Subjects

0301 basic medicine, Hibernation, medicine.medical_specialty, medicine.drug_class, media_common.quotation_subject, Clinical Biochemistry, Antibiotics, Inflammation, Oxytetracycline, Biology, Biochemistry, Analytical Chemistry, 03 medical and health sciences, Internal medicine, medicine, media_common, 0402 animal and dairy science, Acute-phase protein, Appetite, Lipid metabolism, 04 agricultural and veterinary sciences, 040201 dairy & animal science, Blood proteins, 3. Good health, 030104 developmental biology, Endocrinology, medicine.symptom, medicine.drug

Abstract

The growth promoting effect of supplementing animal feed with antibiotics like tetracycline has traditionally been attributed to their antibiotic character. However, more evidence has been accumulated on their direct anti-inflammatory effect during the last two decades. Here we used a pig model to explore the systemic molecular effect of feed supplementation with sub therapeutic levels of oxytetracycline (OTC) by analysis of serum proteome changes. Results showed that OTC promoted growth, coinciding with a significant down regulation of different serum proteins related to inflammation, oxidation and lipid metabolism, confirming the anti-inflammatory mechanism of OTC. Interestingly, apart from the classic acute phase reactants also down regulation was seen of a hibernation associated plasma protein (HP-27), which is to our knowledge the first description in pigs. Although the exact function in non-hibernators is unclear, down regulation of HP-27 could be consistent with increased appetite, which is possibly linked to the anti-inflammatory action of OTC. Given that pigs are good models for human medicine due to their genetic and physiologic resemblance, the present results might also be used for rational intervention in human diseases in which inflammation plays an important role such as obesity, type 2 diabetes and cardiovascular diseases.

Published

2016

18. Identification of Rabbit Oviductal Fluid Proteins Involved in Pre-Fertilization Processes by Quantitative Proteomics

Author

Gottfried Brem, Urban Besenfelder, Hans Yu, Florian R. L. Meyer, Corina Mayrhofer, Claus Vogl, Judith Reiser, Ebrahim Razzazi-Fazeli, Lena Hackenbroch, and Katharina Nöbauer

Subjects

Male, Proteomics, Bodily Secretions, Glycosylation, Quantitative proteomics, Insemination, Biochemistry, 03 medical and health sciences, Western blot, Tandem Mass Spectrometry, medicine, Animals, Molecular Biology, Chromatography, High Pressure Liquid, Fallopian Tubes, 030304 developmental biology, chemistry.chemical_classification, 0303 health sciences, biology, medicine.diagnostic_test, 030302 biochemistry & molecular biology, Lectin, Proteins, Cell biology, chemistry, Fertilization, Peptidase regulator activity, Proteome, biology.protein, Oviduct, Female, Rabbits, Glycoprotein

Abstract

Oviductal fluid (ODF) proteins modulate and support reproductive processes in the oviduct. In the present study, proteins involved in the biological events that precede fertilization have been identified in the rabbit ODF proteome, isolated from the ampulla and isthmus of the oviduct at different time points within 8 h after intrauterine insemination. A workflow is used that integrates lectin affinity capture with stable-isotope dimethyl labeling prior to nanoLC-MS/MS analysis. In total, over 400 ODF proteins, including 214 lectin enriched glycoproteins, are identified and quantified. Selected data are validated by Western blot analysis. Spatiotemporal alterations in the abundance of ODF proteins in response to insemination are detected by global analysis. A subset of 63 potentially biologically relevant ODF proteins is identified, including extracellular matrix components, chaperones, oxidoreductases, and immunity proteins. Functional enrichment analysis reveals an altered peptidase regulator activity upon insemination. In addition to protein identification and abundance changes, N-glycopeptide analysis further identifies 281 glycosites on 199 proteins. Taken together, these results show, for the first time, the evolving oviductal milieu early upon insemination. The identified proteins are likely those that modulate in vitro processes, including spermatozoa function.

Published

2018

19. Proteome Profiles of Head Kidney and Spleen of Rainbow Trout (Oncorhynchus Mykiss)

Author

Gokhlesh, Kumar, Karin, Hummel, Ebrahim, Razzazi-Fazeli, and Mansour, El-Matbouli

Subjects

Fish Proteins, lymphoid organs, endocrine system, animal structures, Proteome, urogenital system, animal diseases, trout proteomics, Head Kidney, Article, Tandem Mass Spectrometry, Oncorhynchus mykiss, salmonids, Animals, Spleen

Abstract

The head kidney and spleen are major lymphoid organs of the teleost fish. The authors identify proteome profiles of head kidney and spleen of rainbow trout (Oncorhynchus mykiss) using a shotgun proteomic approach. Gene ontology annotation of proteins is predicted using bioinformatic tools. This study represents detailed proteome profiles of head kidney and spleen of rainbow trout, with a total of 3241 and 2542 proteins identified, respectively. It is found that lymphoid organs are equipped with a variety of functional proteins related to defense, receptor, signal transduction, antioxidant, cytoskeleton, transport, binding, and metabolic processes. The identified proteome profiles will serve as a template for understanding lymphoid organ functions in salmonids and will increase the amount of spectra information of rainbow trout proteins in the public data repository PRIDE. This data can be accessed via ProteomeXchange with identifiers PXD008473 and PXD008478.

Published

2018

20. Proteome analysis reveals a role of rainbow trout lymphoid organs during Yersinia ruckeri infection process

Author

Gokhlesh Kumar, Karin Hummel, Katharina Noebauer, Timothy J. Welch, Ebrahim Razzazi-Fazeli, and Mansour El-Matbouli

Subjects

Yersinia ruckeri, Proteome, Yersinia Infections, urogenital system, animal diseases, lcsh:R, lcsh:Medicine, Head Kidney, Fish Diseases, Oncorhynchus mykiss, Animals, lcsh:Q, lcsh:Science, Author Correction, Spleen

Abstract

Yersinia ruckeri is the causative agent of enteric redmouth disease in salmonids. Head kidney and spleen are major lymphoid organs of the teleost fish where antigen presentation and immune defense against microbes take place. We investigated proteome alteration in head kidney and spleen of the rainbow trout following Y. ruckeri strains infection. Organs were analyzed after 3, 9 and 28 days post exposure with a shotgun proteomic approach. GO annotation and protein-protein interaction were predicted using bioinformatic tools. Thirty four proteins from head kidney and 85 proteins from spleen were found to be differentially expressed in rainbow trout during the Y. ruckeri infection process. These included lysosomal, antioxidant, metalloproteinase, cytoskeleton, tetraspanin, cathepsin B and c-type lectin receptor proteins. The findings of this study regarding the immune response at the protein level offer new insight into the systemic response to Y. ruckeri infection in rainbow trout. This proteomic data facilitate a better understanding of host-pathogen interactions and response of fish against Y. ruckeri biotype 1 and 2 strains. Protein-protein interaction analysis predicts carbon metabolism, ribosome and phagosome pathways in spleen of infected fish, which might be useful in understanding biological processes and further studies in the direction of pathways.

Published

2018

21. Concentration and pattern changes of porcine serum apolipoprotein A-I in four different infectious diseases

Author

Karin Hummel, Anna Bassols, Ingrid Miller, Anna Marco-Ramell, and Ebrahim Razzazi-Fazeli

Subjects

Salmonella, biology, Apolipoprotein B, Clinical Biochemistry, biology.organism_classification, Proteomics, medicine.disease_cause, Biochemistry, Molecular biology, Analytical Chemistry, Porcine circovirus, Blood serum, Infectious disease (medical specialty), biology.protein, medicine, lipids (amino acids, peptides, and proteins), Protein precursor, Escherichia coli

Abstract

Apolipoprotein A-I (Apo A-I) is a major protein in lipid/lipoprotein metabolism and decreased serum levels have been observed in many species in response to inflammatory and infectious challenges. Little is known about the porcine homologue, therefore in this work we have characterized it through biochemical and proteomic techniques. In 2DE, porcine serum Apo A-I is found as three spots, the two more acidic ones corresponding to the mature protein, the more basic spot to the protein precursor. Despite high sequence coverage in LC-MS/MS, we did not find a sequence or PTM difference between the two mature protein species. Besides this biochemical characterization, we measured overall levels and relative species abundance of serum Apo A-I in four different viral and bacterial porcine infectious diseases. Lower overall amounts of Apo A-I were observed in Salmonella typhimurium and Escherichia coli infections. In the 2DE protein pattern, an increase of the protein precursor together with a lower level of mature protein species were detected in the porcine circovirus type 2-systemic disease and S. typhimurium infection. These results reveal that both the porcine serum Apo A-I concentration and the species pattern are influenced by the nature of the infectious disease.

Published

2015

22. Semen modulated secretory activity of oviductal epithelial cells is linked to cellular proteostasis network remodeling: Proteomic insights into the early phase of interaction in the oviduct in vivo

Author

Ebrahim Razzazi-Fazeli, Gottfried Brem, Hans Yu, Urban Besenfelder, Konstantin A. Artemenko, Daniela Milovanovic, Corina Mayrhofer, Birgit Steinberger, Ursula Reichart, and Theodor Brodmann

Subjects

0301 basic medicine, Male, Proteomics, Cell signaling, Time Factors, Cellular adaptation, Proteome, Biophysics, Cellular homeostasis, Oviducts, Biology, Biochemistry, Insemination, 03 medical and health sciences, 0302 clinical medicine, Semen, medicine, OVGP1, Animals, Humans, Secretion, Epithelial Cells, Phosphoproteins, Epithelium, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Proteostasis, Secretory protein, 030220 oncology & carcinogenesis, Female, Rabbits

Abstract

The oviductal epithelium is crucial for the integrity of the female organ. Previously we got evidence that the surface proteome of oviductal epithelial cells (Oecs) is promptly altered in response to insemination and thus suggested that this early phase plays a notable regulatory role in maintaining cellular function. This study further aimed to assess the effect of semen on the cellular and molecular mechanisms in rabbit Oecs. A quantitative gel-based proteomic approach was applied to analyze changes at three time points (0 h, 1 h, 2 h) after intrauterine insemination (IUI) compared to time matched controls. Within two hours the abundance of 22 protein species was evidently altered in the intracellular fraction. Functional analysis revealed that the proteins were primarily involved in proteostasis as well as metabolic processes. The analysis of phosphoproteins specified a role of mitogen-activated protein kinase (MAPK) signaling molecules. Concurrently, semen increased oviduct-specific glycoprotein (OVGP1) secretion. A correlation between OVGP1 abundance and microtubule-associated proteins 1A/1B–light chain 3 lipidation was observed. The localization and changes in abundance of selected proteins were corroborated by antibody-based methods. These results clearly show that the early phase of interaction acts as a trigger for cellular adaptation to meet an altered demand in the female organ. Significance The oviductal epithelium and its secreted proteins exert a pivotal role in reproductive processes, including the final maturation of male gametes. Thereby, the regulation and subsequently the functionality of the oviductal epithelial cell layer are important factors for the establishment of the appropriate milieu in the female reproductive tract. Notably, male gametes themselves have been shown to be an extrinsic modulatory factor of the oviductal epithelium. Accordingly a comprehensive knowledge about the underlying cellular and molecular mechanisms in the epithelial cells is of interest, also with regard to in vitro purposes. So far, the role of the early phase of interaction in the female organ has not been considered in detail. To get a further insight into the underlying cellular and molecular mechanisms, herein we analyzed the effect of semen on oviductal epithelial cells (Oecs) on the intracellular proteome level within the first two hours after insemination. The present study revealed a directed response of Oecs in vivo and disclosed intracellular pathways that are affected by the interplay between semen and the female reproductive tract. The prompt adaptation of the secretory activity and remodeling of the oviductal epithelium was accompanied by the concerted alterations of protein species that are primarily involved in the maintenance of cellular homeostasis. Besides emphasizing the importance of the early interaction phase for subsequent reproductive processes, the gained knowledge might further be implemented for in vitro applications as well.

Published

2017

23. In between — Proteomics of dog biological fluids

Author

Andrea Preßlmayer-Hartler, Elisabetta Gianazza, Ingrid Miller, R Wait, Cristina Sensi, Ivano Eberini, Ebrahim Razzazi-Fazeli, and Karin Hummel

Subjects

Proteomics, Silver Staining, business.industry, Temperature, Biophysics, Blood Proteins, Computational biology, Allergens, Hydrogen-Ion Concentration, Urine, Biochemistry, Body Fluids, Toxicology studies, Proteinuria, Dogs, Animal model, Polysaccharides, Models, Animal, Biological fluids, Animals, Medicine, Electrophoresis, Gel, Two-Dimensional, Animal species, business

Abstract

Dogs are relevant to biomedical research in connection both to veterinary medicine for their role as pets and to basic investigations for their use as animal models in pathology, pharmacology and toxicology studies. Proteomic analysis of biological fluids is less advanced for dogs than for other animal species but a wealth of information has already been gathered, which we summarize in this review. As a remarkable feature, we also assemble here for due reference a number of 2-DE serum/plasma or urine patterns in health and disease; some of them correspond to unpublished data from the University of Veterinary Medicine Vienna.

Published

2014

24. Global Proteomics of the Extremophile Black Fungus Cryomyces antarcticus Using 2D-Electrophoresis

Author

Kristina Zakharova, Ebrahim Razzazi-Fazeli, Katharina Noebauer, Katja Sterflinger, and Gorji Marzban

Subjects

Cryomyces antarcticus, Two-dimensional gel electrophoresis, ved/biology, fungi, ved/biology.organism_classification_rank.species, Fungus, Biology, biology.organism_classification, Proteomics, medicine.drug_formulation_ingredient, Evolutionary biology, Proteome, Botany, medicine, Extremophile, Model organism, Organism

Abstract

The microcolonial black fungus Cryomyces antarcticus is an extremophile organism growing on and in rock in the Antarctic desert. Ecological plasticity and stress tolerance make it a perfect model organism for astrobiology. 2D-gel electrophoresis and MALDI-TOF/TOF mass spectrometry were performed to explore the protein repertoire, which allows the fungus to survive in the harsh environment. Only a limited number of proteins could be identified by using sequence homologies in public databases. Due to the rather low identification rate by sequence homology, this study reveals that a major part of the proteome of C. antarcticus varies significantly from other fungal species.

Published

2014

25. Aflatoxins in selected Thai commodities

Author

M. Hollmann, Josef Böhm, Ebrahim Razzazi-Fazeli, Natthasit Tansakul, and Sasithorn Limsuwan

Subjects

2. Zero hunger, Aflatoxin, Arachis, 010401 analytical chemistry, Public Health, Environmental and Occupational Health, Food Contamination, Oryza, 04 agricultural and veterinary sciences, Contamination, Thailand, Toxicology, 040401 food science, 01 natural sciences, High-performance liquid chromatography, 0104 chemical sciences, 0404 agricultural biotechnology, Certified reference materials, Aflatoxins, Food, Food science, Capsicum, Food Analysis, Food Science, Mathematics

Abstract

Aflatoxin (AF) B1, B2, G1 and G2 were determined in 120 samples of selected Thai commodities including unpolished rice, unpolished glutinous rice, chilli powder, whole dried chilli pods and raw peanut. The mean concentrations of the total AFs for analysed samples were 0.16, 25.43, 14.18, 6.62 and 1.43 µg kg(-1) with positive incidences of 4%, 20%, 97%, 37% and 30%, respectively. Quantitative analysis was performed using HPLC equipped with post-column derivatisation and fluorescence detection. Sample clean-up was carried out using immunoaffinity columns for selective enrichment of AFs. The method was validated by using certified reference material, which showed recoveries over 85%. The limit of detections (LODs) and limit of quantifications (LOQs) were in a range between 0.01-0.11 µg kg(-1) and 0.03-0.38 µg kg(-1), respectively. The results clearly demonstrated that AFs were detectable in different matrices. Chilli powder was found to have the highest level of AFs contamination followed by chilli pods, peanut and rice, respectively. However, among the selected commodities, unpolished rice contained only trace levels of AFB1 and AFB2. With regard to the fact that AFs are a natural contaminant in commodities, this report calls to attention the regular monitoring and effective control of food commodities to prevent health hazards.

Published

2013

26. Contamination of therapeutic human immunoglobulin preparations with apolipoprotein H (β2-glycoprotein I)

Author

Karin Hummel, Gerhard Beck, Dieter Pullirsch, Ebrahim Razzazi-Fazeli, Friedrich Lackner, Ingrid Miller, Stephanie Eichmeir, Alexandra Seifner, and Manfred Gemeiner

Subjects

chemistry.chemical_classification, biology, medicine.diagnostic_test, Chemistry, Clinical Biochemistry, Albumin, Contamination, Biochemistry, Molecular biology, Analytical Chemistry, Polyclonal antibodies, In vivo, Transferrin, Immunoassay, biology.protein, medicine, Antibody, Apolipoprotein H

Abstract

Polyclonal immunoglobulin (Ig) concentrates are important biological medicinal products and the assurance of their quality and safety is crucial. In our present approach we used proteomic methods to check the purity of commercial Ig products of different origin. The experimental setup included nonreducing 2DE or DIGE combined with MALDI-TOF and the thrombin generation assay, a routine safety test for pharmaceutical Ig preparations, and was complemented by a specific immunoassay. 2DE patterns displayed contaminations with trace amounts of human apolipoprotein H (Apo-H), transferrin, albumin, and its fragments. In contrast to the latter, Apo-H is a protein that is active in the coagulation cascade, and thus a potential involvement in thromboembolic events in vivo cannot be excluded. It was found by 2DE and MALDI-TOF to be a contaminant of several Ig preparations. Spiking experiments of Ig preparations with pure Apo-H demonstrated an Apo-H concentration dependent increase in thrombin generation assay values. Traces of Apo-H are possibly also contributing to unwanted side effects, as already known for factor XIa. The significance of Apo-H contaminations for these side effects might be verified by detailed analyses of pharmacovigilance data.

Published

2013

27. A limited survey of aflatoxin B1 contamination in Indonesian palm kernel cake and copra meal sampled from batches

Author

Jürgen Zentek, Deni Pranowo, Ali Agus, Sri Wedhastri, Elisabeth Viktoria Reiter, Ebrahim Razzazi-Fazeli, and Nuryono

Subjects

Aflatoxin, Meal, Aflatoxin B1, business.industry, Animal feed, Maximum level, Enzyme-Linked Immunosorbent Assay, Food Contamination, Contamination, Toxicology, Animal Feed, Microbiology, Biotechnology, Animal science, Indonesia, Palm kernel, Humans, media_common.cataloged_instance, European union, Copra, business, media_common, Mathematics

Abstract

Samples from large (100–200 tons) batches of palm kernel cake (PKC, n = 20) and copra meal (CM, n = 13) were collected at production facilities of four Indonesian feed mill manufacturers and analysed for aflatoxin B1 (AFB1) by ELISA. Recoveries using spiked samples ranged from 86 to 113 %, with relative standard deviations of

Published

2013

28. Detection of potential markers for systemic disease in saliva of pigs by proteomics: A pilot study

Author

Ingrid Miller, Ebrahim Razzazi-Fazeli, José J. Cerón, Ana Gutiérrez, Manfred Gemeiner, Katharina Nöbauer, L. Soler, Department of Animal Medicine and Surgery, Universidad de Murcia, VetCore Facility for Research, University of Veterinary Medicine, Faculty of Biosciences Engineering, Biosystems Department, Livestock-Nutrition-Quality Division, Université Catholique de Louvain = Catholic University of Louvain (UCL), Department of Biomedical Sciences, and University of Guelph

Subjects

Male, Proteomics, pig, Saliva, Swine, 040301 veterinary sciences, [SDV]Life Sciences [q-bio], Sus scrofa, Immunology, Pilot Projects, Biology, Lipocalin, Serology, 0403 veterinary science, 03 medical and health sciences, Tandem Mass Spectrometry, Animals, Electrophoresis, Gel, Two-Dimensional, Salivary Proteins and Peptides, proteomic, 030304 developmental biology, Swine Diseases, Gel electrophoresis, saliva, 0303 health sciences, Haptoglobins, General Veterinary, Haptoglobin, Acute-phase protein, Albumin, disease status, 04 agricultural and veterinary sciences, Molecular biology, 3. Good health, C-Reactive Protein, Case-Control Studies, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, biology.protein, Biomarkers

Abstract

Animals with different health status have been studied in order to extend the knowledge about protein composition of porcine saliva samples and to discover potential salivary markers for systemic disease in porcine production. Clinical examination of animals was performed at farm level where 10 healthy pigs and 10 animals with evident clinical signs of disease were randomly selected. Saliva and blood samples were obtained and afterwards animals were humanely sacrificed to perform a complete necropsy. Levels of two acute phase proteins, haptoglobin and C-reactive protein, were used to identify possible active infections of the animals. Moreover, serological analysis, to the main porcine infectious diseases in the area, was performed. Salivary proteins were separated by two-dimensional gel electrophoresis followed by mass spectrometry for the identification of specific proteins. A total of 58 spots out of 75 were successfully identified by MS, which correspond to 20 unique proteins. Two different approaches were used to perform a statistical comparison of saliva protein patterns from healthy and diseased animals using the relative spot volume (% spot volume/total volume of all spot in the gel, approach "A") or taking also into account the total protein content of each saliva sample (μg of spot/mL of saliva, approach "B"). Both analyses showed three proteins in common that are differentially regulated between states. However, approach B was selected for biomarker searching since it gave an estimation of protein concentration and showed differential expression of proteins between both health states in a total of 10 proteins, which were up-regulated in disease. Mass spectrometric analysis identified those proteins as salivary lipocalin, lipocalin 1, double headed protease inhibitor protein, adenosine deaminase, haptoglobin, albumin fragments, S100-A8, S100-A9, S100-A12 and pancreatic alpha amylase. These proteins could be considered as potential salivary markers of disease.

Published

2013

29. Proteome Analyses of Jatropha curcas

Author

Margit Laimer, Ebrahim Razzazi-Fazeli, Fatemeh Maghuly, and Gorji Marzban

Subjects

0301 basic medicine, food and beverages, Computational biology, Biology, biology.organism_classification, Plant tissue, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, 030228 respiratory system, Proteome, Protein purification, Identification (biology), Jatropha curcas

Abstract

Plant proteomes are complex and therefore their analyses represent major technical challenges. In fact, proteome analyses depend on several crucial steps, such as the amount of proteins, extraction, separation, visualization, identification, quantification, and the interaction between proteins and other molecules in a plant tissue at a given time.

Published

2016

30. Diversity of major urinary proteins (MUPs) in wild house mice

Author

Michaela Thoß, Viktoria Enk, Hans Yu, Ingrid Miller, Kenneth C. Luzynski, Boglarka Balint, Steve Smith, Ebrahim Razzazi-Fazeli, and Dustin J. Penn

Subjects

Male, Heterozygote, Genome, Base Sequence, Gene Expression, Proteins, Animals, Wild, Sequence Analysis, DNA, Article, Mice, Multigene Family, Animals, Female, Alleles, Conserved Sequence, Microsatellite Repeats

Abstract

Major urinary proteins (MUPs) are often suggested to be highly polymorphic, and thereby provide unique chemical signatures used for individual and genetic kin recognition; however, studies on MUP variability have been lacking. We surveyed populations of wild house mice (Mus musculus musculus), and examined variation of MUP genes and proteins. We sequenced several Mup genes (9 to 11 loci) and unexpectedly found no inter-individual variation. We also found that microsatellite markers inside the MUP cluster show remarkably low levels of allelic diversity, and significantly lower than the diversity of markers flanking the cluster or other markers in the genome. We found low individual variation in the number and types of MUP proteins using a shotgun proteomic approach, even among mice with variable MUP electrophoretic profiles. We identified gel bands and spots using high-resolution mass spectrometry and discovered that gel-based methods do not separate MUP proteins, and therefore do not provide measures of MUP diversity, as generally assumed. The low diversity and high homology of Mup genes are likely maintained by purifying selection and gene conversion, and our results indicate that the type of selection on MUPs and their adaptive functions need to be re-evaluated.

Published

2016

31. Detection and first characterization of an uncommon haptoglobin in porcine saliva of pigs with rectal prolapse by using boronic acid sample enrichment

Author

Ebrahim Razzazi-Fazeli, Ingrid Miller, Katharina Nöbauer, Daniel Kolarich, Karin Hummel, and Ana Gutiérrez

Subjects

0301 basic medicine, pig, Male, Saliva, Pathology, medicine.medical_specialty, Swine, Blotting, Western, Biology, 01 natural sciences, SF1-1100, Mass Spectrometry, 03 medical and health sciences, proteomics, Western blot, medicine, Animals, Electrophoresis, Gel, Two-Dimensional, Salivary Proteins and Peptides, Gel electrophoresis, chemistry.chemical_classification, Swine Diseases, medicine.diagnostic_test, Haptoglobins, 010401 analytical chemistry, Haptoglobin, Acute-phase protein, Rectal Prolapse, medicine.disease, Molecular biology, Boronic Acids, 0104 chemical sciences, Animal culture, Rectal prolapse, 030104 developmental biology, Isoelectric point, chemistry, inflammation, biology.protein, Animal Science and Zoology, Electrophoresis, Polyacrylamide Gel, glyco-enrichment, Glycoprotein

Abstract

Salivary glycoprotein profiles, obtained after boronic acid enrichment, were studied for the first time in pigs in order to search for specific overall alterations related to acute inflammatory condition. Five healthy pigs and five pigs suffering from rectal prolapse were used, and the levels of acute phase proteins were measured to determine the degree of inflammation of the animals. The enriched glycoprotein profiles, achieved by two-dimensional gel electrophoresis (2DE) were statistically evaluated and spots that appeared differentially regulated between states were subjected to MS analysis for protein identification. Spots from three unique proteins were identified: carbonic anhydrase VI (CA VI), α-1-antichymotrypsin and haptoglobin (Hp). CA VI appeared as two adjacent horizontal spot trains in the glycoprotein profile of healthy animals in its regular isoelectric points (pI). One spot of α-1-antichymotrypsin was found in saliva from pigs with rectal prolapse in an unusual basic pI, and was considered as a breakdown product. Hp was identified as several spot trains in saliva from pigs with rectal prolapse in an unusual alkaline pI and was consequently further investigated. SDS-PAGE and 2DE of paired serum and saliva samples combined with Western blot analysis showed that the unusual Hp position observed in saliva samples was absent in serum. Furthermore, N-glycans from serum and saliva Hp glycopatterns were evaluated from SDS-PAGE Hp bands and showed that the serum N-glycan distribution in Hp β-chain was comparable in quantity and quality in both groups of animals. In saliva, no Hp β-chain derived N-glycans could unambiguously be identified from this sample set, thus needing further detailed investigations in the future.

Published

2016

32. Influence of different sample preparation strategies on the proteomic identification of stress biomarkers in porcine saliva

Author

José J. Cerón, Ana Gutiérrez, Fernando Tecles, Sarah Schlosser, and Ebrahim Razzazi-Fazeli

Subjects

0301 basic medicine, Male, Proteomics, Saliva, 040301 veterinary sciences, Swine, Lipocalin, 0403 veterinary science, 03 medical and health sciences, Stress, Physiological, Protein purification, Animals, Electrophoresis, Gel, Two-Dimensional, Hexapeptide libraries, Lipocalin 1, chemistry.chemical_classification, Gel electrophoresis, Swine Diseases, Pig, lcsh:Veterinary medicine, General Veterinary, Chemistry, 04 agricultural and veterinary sciences, General Medicine, Glycoprotein-enrichment, 030104 developmental biology, Prolactin-Inducible Protein, Biochemistry, lcsh:SF600-1100, Glycoprotein, Biomarkers, Research Article

Abstract

Background The influence of two different sample treatments comprising the enrichment of glycoproteins by boronic acid and dynamic range compression by hexapeptide libraries, on the detection of stress markers in saliva of pigs was evaluated in this study. For this purpose, saliva samples collected before and after the application of an acute stress model consisting of nasal restraining in pigs were processed without any treatment and with the two different treatments mentioned above. Protein separation by two-dimensional gel electrophoresis (2-DE) followed by identification of proteins using MALDI-TOF/TOF mass spectrometry (MS) was used as proteomic technique. Results The application of each of the two different sample treatment protocols allowed the identification of unique proteins that could be potential salivary acute stress markers in pigs: lipocalin 1, protein S100-A8 and immunoglobulin M by enrichment of glycoproteins; protein S100-A9, double headed protease inhibitor submandibular gland, and haemoglobin by dynamic range compression; and protein S100-A12 by both protocols. Salivary lipocalin, prolactin inducible protein, light chain of immunoglobulins, adenosine deaminase and carbonic anhydrase VI were identified as potential markers in untreated saliva as well as one of the other treatments. Conclusion The use of different procedures allowed the detection of different potential stress markers. Although from a practical point of view, the use of saliva without further treatment as well as the enrichment of glycoproteins are less expensive and easy to do procedures.

Published

2016

33. ADSORPTION OF AFLATOXIN B1 IN CORN ON NATURAL ZEOLITE AND BENTONITE

Author

Ebrahim Razzazi-Fazeli, Deni Pranowo, Yunianto Yunianto, Sri Wedhastri, Y.M.S. Maryudhani, Nuryono Nuryono, and Ali Agus

Subjects

Chromatography, Chemistry, bentonite, Mixing (process engineering), aflatoxin, General Chemistry, Standard solution, High-performance liquid chromatography, corn, adsorption, zeolite, Adsorption, Bentonite, Particle size, Suspension (vehicle), Zeolite, QD1-999, Nuclear chemistry

Abstract

A study on adsorption of AFB1 in corn (kernel and grained) on natural zeolite and bentonite has been investigated. The first work was adsorption in a batch system of standard AFB1 solution on adsorbents. Some factors such as contact time, concentration of AFB1 and particle size of adsorbent were evaluated. The amount of AFB1 adsorbed was calculated based on the difference of AFB1 concentration before and after adsorption determined by high performance liquid chromatography (HPLC) method. Adsorption of AFB1 in corn sample was emphasized by mixing aqueous suspension of sample with adsorbent. Concentration of AFB1 in suspension was analyzed by enzyme-linked immuno-sorbent assay (ELISA) method. Result shows that adsorption of AFB1 on adsorbents of natural zeolite and bentonite is very fast. Within 15 min 99% of AFB1 (200 ng/mL) has been adsorbed by 25 mg of bentonite and 96% by zeolite. The particle size higher than 200 mesh did not give significant effect on the AFB1 adsorption capability. Effectiveness of zeolite in adsorbing AFB1 is lower than that of bentonite. Capability in reducing AFB1 contamination in corn samples (kernel and meal) for both adsorbents is lower than that in standard solution.

Published

2012

34. Exploring the Unique N-Glycome of the Opportunistic Human Pathogen Acanthamoeba

Author

Birgit Schiller, Katharina Paschinger, Georgia Makrypidi, Julia Walochnik, Ebrahim Razzazi-Fazeli, and Iain B. H. Wilson

Subjects

Glycan, Glycobiology and Extracellular Matrices, Virulence, Acanthamoeba, Human pathogen, Biochemistry, Mass Spectrometry, Fucose, Glycomics, chemistry.chemical_compound, Polysaccharides, parasitic diseases, Carbohydrate Conformation, Animals, Humans, Molecular Biology, Pathogen, biology, Cell Biology, biology.organism_classification, Glycome, eye diseases, chemistry, biology.protein

Abstract

Glycans play key roles in host-pathogen interactions; thus, knowing the N-glycomic repertoire of a pathogen can be helpful in deciphering its methods of establishing and sustaining a disease. Therefore, we sought to elucidate the glycomic potential of the facultative amoebal parasite Acanthamoeba. This is the first study of its asparagine-linked glycans, for which we applied biochemical tools and various approaches of mass spectrometry. An initial glycomic screen of eight strains from five genotypes of this human pathogen suggested, in addition to the common eukaryotic oligomannose structures, the presence of pentose and deoxyhexose residues on their N-glycans. A more detailed analysis was performed on the N-glycans of a genotype T11 strain (4RE); fractionation by HPLC and tandem mass spectrometric analyses indicated the presence of a novel mannosylfucosyl modification of the reducing terminal core as well as phosphorylation of mannose residues, methylation of hexose and various forms of pentosylation. The largest N-glycan in the 4RE strain contained two N-acetylhexosamine, thirteen hexose, one fucose, one methyl, and two pentose residues; however, in this and most other strains analyzed, glycans with compositions of Hex(8-9)HexNAc(2)Pnt(0-1) tended to dominate in terms of abundance. Although no correlation between pathogenicity and N-glycan structure can be proposed, highly unusual structures in this facultative parasite can be found which are potential virulence factors or therapeutic targets.

Published

2012

35. Galactosylated Fucose Epitopes in Nematodes

Author

Silvia Bleuler-Martinez, Anja Joachim, Ebrahim Razzazi-Fazeli, David F. Plaza, Markus Künzler, Iain B. H. Wilson, Shi Yan, Markus Aebi, Katharina Paschinger, Verena Jantsch, and Rudolf Geyer

Subjects

0303 health sciences, Glycan, biology, 030302 biochemistry & molecular biology, Mutant, Lectin, Cell Biology, biology.organism_classification, Biochemistry, Molecular biology, Fucose, Hexosaminidases, carbohydrates (lipids), Caenorhabditis, 03 medical and health sciences, chemistry.chemical_compound, chemistry, biology.protein, Molecular Biology, Ascaris suum, Caenorhabditis elegans, 030304 developmental biology

Abstract

The modification of α1,6-linked fucose residues attached to the proximal (reducing-terminal) core N-acetylglucosamine residue of N-glycans by β1,4-linked galactose (“GalFuc” epitope) is a feature of a number of invertebrate species including the model nematode Caenorhabditis elegans. A pre-requisite for both core α1,6-fucosylation and β1,4-galactosylation is the presence of a nonreducing terminal N-acetylglucosamine; however, this residue is normally absent from the final glycan structure in invertebrates due to the action of specific hexosaminidases. Previously, we have identified two hexosaminidases (HEX-2 and HEX-3) in C. elegans, which process N-glycans. In the present study, we have prepared a hex-2;hex-3 double mutant, which possesses a radically altered N-glycomic profile. Whereas in the double mutant core α1,3-fucosylation of the proximal N-acetylglucosamine was abolished, the degree of galactosylation of core α1,6-fucose increased, and a novel Galα1,2Fucα1,3 moiety attached to the distal core N-acetylglucosamine residue was detected. Both galactosylated fucose moieties were also found in two parasitic nematodes, Ascaris suum and Oesophagostomum dentatum. As core modifications of N-glycans are known targets for fungal nematotoxic lectins, the sensitivity of the C. elegans double hexosaminidase mutant was assessed. Although this mutant displayed hypersensitivity to the GalFuc-binding lectin CGL2 and the N-acetylglucosamine-binding lectin XCL, the mutant was resistant to CCL2, which binds core α1,3-fucose. Thus, the use of C. elegans mutants aids the identification of novel N-glycan modifications and the definition of in vivo specificities of nematotoxic lectins with potential as anthelmintic agents.

Published

2012

36. Limited survey of deoxynivalenol occurrence in maize kernels and maize-products collected from Indonesian retail market

Author

Nuryono Nuryono, Helmut K. Mayer, Ebrahim Razzazi-Fazeli, F. M. C. S. Setyabudi, and Sri Wedhastri

Subjects

Detection limit, Toxicology, Animal health, Relative standard deviation, Retail market, European commission, Repeatability, Contamination, High-performance liquid chromatography, Food Science, Biotechnology, Mathematics

Abstract

Fifty samples consisted of 24 maize kernels and 26 maize based-food products from retail market in Yogyakarta, Indonesia were analysed for deoxynivalenol (DON) using high performance liquid chromatography (HPLC) combined with ultraviolet detection after immunoaffinity column (IAC) clean-up process. Prior to use, performance of the analytical method was evaluated in term of recovery, repeatability, and detection limit. The recoveries of DON in spiked samples (50–360 μg DON/kg sample) were obtained in a range of 70.9–97.3% with relative standard deviation (RSD) for repeatability within a day less than 16%. Limit of detection based on the response ratio of signal to noise (3/1) was noted being 20 μg DON/kg sample. All analysed samples contained DON ranging between 47 and 348 μg/kg with median and means of 111.0 and 124.6 μg/kg, respectively. The contamination of DON in the studied samples may not be taken into account as hazard for human and animal health since the concentrations were lower than maximum limit of DON contamination in foodstuffs (500 μg/kg) established by European Commission (2006).

Published

2012

37. The levels of zearalenone and its metabolites in plasma, urine and faeces of horses fed with naturally, Fusarium toxin-contaminated oats

Author

Christine Aurich, Josef Böhm, Ebrahim Razzazi-Fazeli, P. Songsermsakul, and Jürgen Zentek

Subjects

Fusarium, Chromatography, biology, Metabolite, Glucuronidation, Horse, Urine, biology.organism_classification, chemistry.chemical_compound, Animal science, Food Animals, chemistry, Animal Science and Zoology, Zearalanone, Zearalenone, Feces

Abstract

Concentration profile of zearalenone (ZON) and its metabolites in plasma, urine and faeces samples of horses fed with Fusarium toxin-contaminated oats is described. In plasma, β-zearalenol (β-ZOL) was detected at high levels on day 10 of the study (3.21-6.24 μg/l). β-Zearalenol and α-zearalenol were the major metabolites in urine. Zearalenone, α-ZOL and β-ZOL were predominantly found in faeces. Zearalanone could also be detected in urine (1.34-5.79 μg/l) and faeces (1 μg/kg). The degree of glucuronidation was established in all sample types, approximately 100% in urine and plasma. Low per cent of glucuronidation (4-15%) was found in faeces samples. The results indicate the main conversion of ZON into β-ZOL in horse. This finding could explain why horse is not susceptible to ZON in comparison with swine which produce α-ZOL as a predominant metabolite.

Published

2011

38. The N-glycans of Trichomonas vaginalis contain variable core and antennal modifications

Author

Alba Hykollari, Ebrahim Razzazi-Fazeli, Katharina Paschinger, Pamela Greenwell, Iain B. H. Wilson, Julia Walochnik, and David Leitsch

Subjects

Glycan, Glycosylation, Glycoconjugate, Pentoses, Oligosaccharides, Biology, medicine.disease_cause, Biochemistry, Article, Microbiology, chemistry.chemical_compound, Polysaccharides, Trichomonas vaginalis, medicine, Parasite hosting, Chromatography, High Pressure Liquid, Galectin, chemistry.chemical_classification, Strain (chemistry), Host (biology), Amino Sugars, chemistry, Ethanolamines, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, biology.protein

Abstract

Trichomonad species are widespread unicellular flagellated parasites of vertebrates which interact with their hosts through carbohydrate-lectin interactions. In the past, some data have been accumulated regarding their lipo(phospho)glycans, a major glycoconjugate on their cell surfaces; on the other hand, other than biosynthetic aspects, few details about their N-linked oligosaccharides are known. In this study, we present both mass spectrometric and high-performance liquid chromatography data about the N-glycans of different strains of Trichomonas vaginalis, a parasite of the human reproductive tract. The major structure in all strains examined is a truncated oligomannose form (Man(5)GlcNAc(2)) with α1,2-mannose residues, compatible with a previous bioinformatic examination of the glycogenomic potential of T. vaginalis. In addition, dependent on the strain, N-glycans modified by pentose residues, phosphate or phosphoethanolamine and terminal N-acetyllactosamine (Galβ1,4GlcNAc) units were found. The modification of N-glycans by N-acetyllactosamine in at least some strains is shared with the lipo(phospho)glycan and may represent a further interaction partner for host galectins, thereby playing a role in binding of the parasite to host epithelia. On the other hand, the variation in glycosylation between strains may be the result of genetic diversity within this species.

Published

2011

39. Aflatoxin B1 in Affecting Broiler’s Performance, Immunity, and Gastrointestinal Tract: A Review of History and Contemporary Issues

Author

Ebrahim Razzazi-Fazeli, Josef Böhm, and Agha Waqar Yunus

Subjects

Aflatoxin, Aflatoxin B1, animal structures, Animal feed, Health, Toxicology and Mutagenesis, chicken, lcsh:Medicine, Review, Biology, Toxicology, Weight Gain, broiler, Lethal Dose 50, chemistry.chemical_compound, Eating, Immunity, hormesis, Animals, Aflatoxin B, Mycotoxin, Gastrointestinal tract, Immunity, Cellular, business.industry, lcsh:R, Broiler, technology, industry, and agriculture, food and beverages, aflatoxin, Organ Size, Animal Feed, Biotechnology, Immunity, Humoral, Gastrointestinal Tract, Aspergillus, chemistry, Organ Specificity, business, Chickens

Abstract

Aflatoxin B(1) is a common contaminant of poultry feeds in tropical and subtropical climates. Research during the last five decades has well established the negative effects of the mycotoxin on health of poultry. However, the last ten years of relevant data have accentuated the potential of low levels of aflatoxin B(1) to deteriorate broiler performance. In this regard, any attempt to establish a dose-effect relationship between aflatoxin B(1) level and broiler performance is also complicated due to differences in types of broilers and length of exposure to the mycotoxin in different studies. Contrary to the prevalent notion regarding literature saturation with respect to aflatoxicosis of chicken, many areas of aflatoxicosis still need to be explored. Literature regarding effects of the mycotoxin on the gastrointestinal tract in this regard is particular scanty and non-conclusive. In addition to these issues, the metabolism of aflatoxin B(1) and recently proposed hypotheses regarding biphasic effects of the mycotoxin in broilers are briefly discussed.

Published

2011

40. Presence of galactosylated core fucose on N-glycans in the planaria Dugesia japonica

Author

Iain B. H. Wilson, Katharina Paschinger, Ebrahim Razzazi-Fazeli, and Kiyoshi Furukawa

Subjects

Glycan, Stereochemistry, Oligosaccharides, Peptide, Methylation, Fucose, 03 medical and health sciences, Residue (chemistry), chemistry.chemical_compound, Polysaccharides, Tandem Mass Spectrometry, Exoglycosidase, Carbohydrate Conformation, Animals, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase, Chromatography, High Pressure Liquid, Spectroscopy, mass spectrometry, 030304 developmental biology, chemistry.chemical_classification, 0303 health sciences, biology, Chemistry, 030302 biochemistry & molecular biology, Galactose, Planarians, planaria, biology.organism_classification, Galβ1,4Fuc epitope, Planaria, carbohydrates (lipids), Biochemistry, N-glycan, biology.protein, Dugesia japonica, Carbohydrate conformation, methylhexose, Research Article

Abstract

Planarial species are of especial interest to biologists due to the phenomenon of pluripotency and, in comparison to other developmental processes, it can be hypothesised that glycan–lectin interactions may play a role. In order to examine the N-glycans of one of these organisms, Dugesia japonica, peptide:N-glycosidase A was employed and the released glycans were subject to pyridylamination, HPLC and mass spectrometric analysis. A range of oligomannosidic glycans was observed with a trimethylated Man5GlcNAc2 structure being the dominant species. Three glycans were also observed to contain deoxyhexose; in particular, a glycan with the composition Hex4HexNAc2Fuc1Me2 was revealed by exoglycosidase digestion, in combination with MS/MS, to contain a galactosylated core α1,6-fucose residue, whereas this core modification was found to be capped with a methylhexose residue in the case of a Hex5HexNAc2Fuc1Me3 structure. This is the first report of these types of structures in a platyhelminth and indicates that the ‘GalFuc’ modification of N-glycans is not just restricted to molluscs and nematodes. Copyright © 2011 John Wiley & Sons, Ltd.

Published

2011

41. Determination of ochratoxin A in grains by immuno-ultrafiltration and HPLC-fluorescence detection after postcolumn derivatisation in an electrochemical cell

Author

Jürgen Zentek, Won-Bo Shim, Duck-Hwa Chung, Margit Cichna-Markl, Ebrahim Razzazi-Fazeli, and Elisabeth Viktoria Reiter

Subjects

Ochratoxin A, Detection limit, Chromatography, Elution, Ultrafiltration, food and beverages, Ochratoxins, Biochemistry, High-performance liquid chromatography, Fluorescence, Analytical Chemistry, Matrix (chemical analysis), chemistry.chemical_compound, Certified reference materials, chemistry, Electrochemistry, Sample preparation, Edible Grain, Quantitative analysis (chemistry), Chromatography, High Pressure Liquid

Abstract

The paper presents a new sample clean-up method based on immuno-ultrafiltration for the analysis of ochratoxin A in cereals. In contrast to immunoaffinity chromatography, in immuno-ultrafiltration, the antibodies are used in non-immobilised form. Ochratoxin A was extracted with ACN/water (60/40, v/v), and the extract was loaded onto the ultrafiltration device. After a washing step with phosphate-buffered saline, containing 0.05% Tween 20, ochratoxin A was eluted with MeOH/acetic acid (99/1, v/v). The detection of ochratoxin A was carried out with high-performance liquid chromatography and a fluorescence detector coupled to an electrochemical cell (Coring cell). The electrochemical cell was used to eliminate matrix interferences by oxidising matrix compounds. The method was validated by repeatedly analysing spiked barley and rye samples as well as a certified wheat reference material. Recoveries and standard deviations (1 SD) were found to be 71 ± 9%, 77 ± 12% and 77 ± 8% in wheat, barley and rye, respectively. The limit of detection (S/N = 3) and limit of quantitation (S/N = 10) were determined to be 0.4 μg kg(-1) and 1 μg kg(-1). The analysis of the certified reference material resulted in ochratoxin A concentrations which were in the range assigned by the producer. Additionally, the effect of the electrochemical cell on other widely used clean-up techniques, namely the immunoaffinity clean-up and multifunctional columns (Mycosep #229), was evaluated. In all clean-up methods, an improvement of the chromatogram quality was registered.

Published

2011

42. Proteomic analysis of porcine saliva

Author

Ana Gutiérrez, Ingrid Miller, Karin Hummel, Katharina Nöbauer, Silvia Martínez-Subiela, Ebrahim Razzazi-Fazeli, Manfred Gemeiner, and José J. Cerón

Subjects

Male, Swine Diseases, Saliva, Proteome, General Veterinary, Swine, Protein composition, Biology, Molecular biology, Mass Spectrometry, Specific Pathogen-Free Organisms, Biochemistry, Two dimensional electrophoresis, Salivary Proteins, Animals, Diagnostic biomarker, Electrophoresis, Gel, Two-Dimensional, Electrophoresis, Polyacrylamide Gel, Animal Science and Zoology, Salivary Proteins and Peptides, Biomarkers

Abstract

Saliva contains a number of proteins that may be useful as biomarkers of health and disease and can be easily obtained from large numbers of animals in a non-invasive, stress-free way. The objective of this study was to explore the protein composition of porcine saliva from 10 specific pathogen free pigs using first one-dimensional SDS–PAGE and then two-dimensional electrophoresis and mass spectrometry. A reference proteome pattern for porcine saliva was established with the identification of 13 different, mainly saliva-specific, proteins. These reference data will facilitate the investigation of salivary proteins potentially altered in disease and could serve as novel diagnostic biomarkers.

Published

2011

43. Author Correction: Proteome analysis reveals a role of rainbow trout lymphoid organs during Yersinia ruckeri infection process

Author

Timothy J. Welch, Ebrahim Razzazi-Fazeli, Mansour El-Matbouli, Katharina Noebauer, Karin Hummel, and Gokhlesh Kumar

Subjects

Multidisciplinary, lcsh:R, lcsh:Medicine, 04 agricultural and veterinary sciences, Biology, biology.organism_classification, 040401 food science, Microbiology, 0404 agricultural biotechnology, Lymphatic system, Proteome, ComputingMethodologies_DOCUMENTANDTEXTPROCESSING, Rainbow trout, lcsh:Q, Yersinia ruckeri, lcsh:Science

Abstract

A correction to this article has been published and is linked from the HTML and PDF versions of this paper. The error has been fixed in the paper.

Published

2018

44. A New Allergen from Ragweed (Ambrosia artemisiifolia) with Homology to Art v 1 from Mugwort

Author

Martin Pabst, Johannes Stadlmann, Gabriele Gadermaier, Fatima Ferreira, Nicole Wopfner, Martin Himly, Renaud Léonard, Christian Radauer, Friedrich Altmann, Ebrahim Razzazi-Fazeli, Jens Ø. Duus, and Bent O. Petersen

Subjects

Ragweed, DNA, Complementary, Immunology, medicine.disease_cause, Galactans, Biochemistry, Mugwort, Allergen, Pollen, Botany, otorhinolaryngologic diseases, medicine, Humans, Ambrosia, Molecular Biology, Ambrosia artemisiifolia, Plant Proteins, Artemisia vulgaris, Sequence Homology, Amino Acid, biology, Rhinitis, Allergic, Seasonal, food and beverages, Cell Biology, Allergens, Antigens, Plant, Immunoglobulin E, biology.organism_classification, Protein Structure, Tertiary, Europe, Artemisia, North America

Abstract

Art v 1, the major pollen allergen of the composite plant mugwort (Artemisia vulgaris) has been identified recently as a thionin-like protein with a bulky arabinogalactan-protein moiety. A close relative of mugwort, ragweed (Ambrosia artemisiifolia) is an important allergen source in North America, and, since 1990, ragweed has become a growing health concern in Europe as well. Weed pollen-sensitized patients demonstrated IgE reactivity to a ragweed pollen protein of apparently 29-31 kDa. This reaction could be inhibited by the mugwort allergen Art v 1. The purified ragweed pollen protein consisted of a 57-amino acid-long defensin-like domain with high homology to Art v 1 and a C-terminal proline-rich domain. This part contained hydroxyproline-linked arabinogalactan chains with one galactose and 5 to 20 and more alpha-arabinofuranosyl residues with some beta-arabinoses in terminal positions as revealed by high field NMR. The ragweed protein contained only small amounts of the single hydroxyproline-linked beta-arabinosyl residues, which form an important IgE binding determinant in Art v 1. cDNA clones for this protein were obtained from ragweed flowers. Immunological characterization revealed that the recombinant ragweed protein reacted with30% of the weed pollen allergic patients. Therefore, this protein from ragweed pollen constitutes a novel important ragweed allergen and has been designated Amb a 4.

Published

2010

45. Aflatoxins in rice – A limited survey of products marketed in Austria

Author

Elisabeth Viktoria Reiter, Ebrahim Razzazi-Fazeli, Florian Vouk, and Josef Böhm

Subjects

chemistry.chemical_compound, Aflatoxin, Chemistry, media_common.cataloged_instance, Food science, European union, Contamination, Mycotoxin, Whole grains, Food Science, Biotechnology, media_common, Food contaminant

Abstract

Eighty-one rice samples were purchased from different markets in Vienna and were analysed for their aflatoxin content. The samples were extracted using methanol in water (80/20 v/v) followed by immunoaffinity clean up. The determination was carried out by HPLC–FLD coupled to a Kobracell. Different samples including basmati rice, whole grain rice, long grain rice, short grain rice as well as puffed rice were investigated. Moreover, conventionally and organically produced rice were compared. The results revealed that 24 out of 81 samples contained detectable amounts of aflatoxins. Aflatoxin B1 could be quantified in 15 samples and aflatoxin B2 in one sample. The contamination range was noted to be between 0.45 μg kg−1 and 9.86 μg kg−1 for aflatoxin B1 and 1.5 μg kg−1 for aflatoxin B2. Aflatoxins G1 and G2 were not detected in any sample. Three samples exceeded the maximum levels set in the European Union; having AFB1 concentrations of 2.16, 2.85 and 9.86 μg kg−1. In the three organic produced rice samples only traces of aflatoxins were found.

Published

2010

46. Molecular Basis for Galactosylation of Core Fucose Residues in Invertebrates

Author

Alex Butschi, Markus Aebi, Ebrahim Razzazi-Fazeli, Markus Künzler, Alexander Titz, Michael O. Hengartner, Bernard Henrissat, Yao-Yun Fan, Iain B. H. Wilson, and Thierry Hennet

Subjects

Galactosyltransferase, Glycan, biology, Cell Biology, biology.organism_classification, Biochemistry, Fucose, Coprinopsis cinerea, chemistry.chemical_compound, chemistry, Glycosyltransferase, biology.protein, Molecular Biology, Gene, Caenorhabditis elegans, Galectin

Abstract

Galectin CGL2 from the ink cap mushroom Coprinopsis cinerea displays toxicity toward the model nematode Caenorhabditis elegans. A mutation in a putative glycosyltransferase-encoding gene resulted in a CGL2-resistant C. elegans strain characterized by N-glycans lacking the β1,4-galactoside linked to the α1,6-linked core fucose. Expression of the corresponding GALT-1 protein in insect cells was used to demonstrate a manganese-dependent galactosyltransferase activity. In vitro, the GALT-1 enzyme showed strong selectivity for acceptors with α1,6-linked N-glycan core fucosides and required Golgi- dependent modifications on the oligosaccharide antennae for optimal synthesis of the Gal-β1,4-fucose structure. Phylogenetic analysis of the GALT-1 protein sequence identified a novel glycosyltransferase family (GT92) with members widespread among eukarya but absent in mammals.

Published

2009

47. A limited survey of aflatoxin M1 in milk from Indonesia by ELISA

Author

Ebrahim Razzazi-Fazeli, Sri Wedhastri, Ali Agus, F.M.C. Sigit Setyabudi, Josef Böhm, Nuryono Nuryono, and Y. B. Maryudani

Subjects

Aflatoxin, Veterinary medicine, food and beverages, Pasteurization, Microbial contamination, Contamination, law.invention, Fresh milk, chemistry.chemical_compound, chemistry, law, media_common.cataloged_instance, Food science, European union, Mycotoxin, Food Science, Biotechnology, media_common, Food contaminant

Abstract

This paper presents a limited survey of aflatoxin M1 (AFM1) in Indonesian milk. AFM1 concentrations of 113 fresh milk samples, collected in 2006 from farms in five different areas of the Yogyakarta Province were analysed. The fresh milk samples were taken directly from dairy farms before pasteurisation. Enzyme-linked immunosorbent assay (ELISA) was used for the analysis of milk samples. Results show that in 48 samples (42.5%) the AFM1 concentrations were less than 5 ng/L and in 31 samples (27.4%) AFM1 was found between 5 and 10 ng/L. In 34 samples (30.1%) the concentrations were above 10 ng/L. None of contaminated samples exceeded the European Union regulation limits of 25 and 50 ng AFM1/L for infant and adult consumption, respectively. Since AFM1 is derived from aflatoxin B1 (AFB1) contained in cow feedstuffs, based on the contamination levels of AFM1 found in this study, the exposure of animals to AFB1 seems to be low.

Published

2009

48. Distribution and activity levels of matrix metalloproteinase 2 and 9 in canine and feline osteosarcoma

Author

Christiane, Gebhard, Andrea, Fuchs-Baumgartinger, Ebrahim, Razzazi-Fazeli, Ingrid, Miller, and Ingrid, Walter

Subjects

musculoskeletal diseases, Male, Osteosarcoma, Bone Neoplasms, Cat Diseases, Article, body regions, Gene Expression Regulation, Neoplastic, Dogs, Matrix Metalloproteinase 9, Cats, Animals, Matrix Metalloproteinase 2, Female, Dog Diseases, neoplasms

Abstract

Overexpression of matrix metalloproteinases (MMPs) has been associated with increased tumor aggressiveness and metastasis dissemination. We investigated whether the contrasting metastatic behavior of feline and canine osteosarcoma is related to levels and activities of MMP2 and MMP9. Zymography and immunohistochemistry were used to determine expression levels of MMP2 and MMP9 in canine and feline osteosarcoma. Using immunohistochemistry, increased MMP9 levels were identified in most canine osteosarcomas, whereas cat samples more often displayed moderate levels. High levels of pro-MMP9, pro-MMP2, and active MMP2 were detected by gelatin zymography in both species, with significantly higher values for active MMP2 in canine osteosarcoma. These findings indicate that MMP2 is probably involved in canine and feline osteosarcoma and their expression and activity could be associated with the different metastatic behavior of canine and feline osteosarcoma.La surexpression de métalloprotéases de matrice (MPMs) a été associée avec une augmentation de l’agressivité des tumeurs et de la dissémination métastasique. Nous avons cherché à savoir si le comportement métastasique contrastant d’ostéosarcomes félin et canin est relié aux quantités et à l’activité de MPM2 et MPM9. La zymographie et l’immunohistochimie ont été utilisées afin de déterminer les niveaux d’expression de MPM2 et de MPM9 dans des ostéosarcomes canins et félins. En utilisant l’immunohistochimie, des quantités augmentées de MPM9 ont été identifiées dans la plupart des ostéosarcomes canins, alors que les échantillons félins montraient plus souvent des quantités modérées. Des niveaux élevés de pro-MPM9, pro-MPM2, et de la MPM2 active ont été détectés par zymographie sur gélatine chez les deux espèces, avec des valeurs significativement plus élevées pour de la MPM2 active dans les ostéosarcomes canins. Ces données indiquent que MPM2 est probablement impliquée dans les ostéosarcomes canins et félins et que leur expression et activité pourraient être associé avec le comportement métastasique différent des ostéosarcomes canins et félins.(Traduit par Docteur Serge Messier).

Published

2016

49. Purification of HIV-1 gag virus-like particles and separation of other extracellular particles

Author

Tobias Amadeus Schneider, Daniel Burgstaller, Petra Kramberger, Miriam Klausberger, Ebrahim Razzazi-Fazeli, Alois Jungbauer, Patricia Pereira Aguilar, Andres Tover, Petra Steppert, Eva Berger, and Katharina Nöbauer

Subjects

0301 basic medicine, viruses, Clinical Biochemistry, Fraction (chemistry), CHO Cells, Biochemistry, Exosome, gag Gene Products, Human Immunodeficiency Virus, Host cell DNA, Analytical Chemistry, 03 medical and health sciences, chemistry.chemical_compound, Cricetulus, Microscopy, Electron, Transmission, Cricetinae, Extracellular, Centrifugation, Density Gradient, Animals, Humans, Vaccines, Virus-Like Particle, Monolith, Host cell protein, Differential centrifugation, Vaccines, Chromatography, geography, geography.geographical_feature_category, Downstream processing, Organic Chemistry, virus diseases, Extracellular particles, General Medicine, Microvesicles, Recombinant Proteins, 3. Good health, 030104 developmental biology, chemistry, HIV-1, Molecular Medicine, Nanoparticles, Density gradient centrifugation, DNA

Abstract

Enveloped virus-like particles (VLPs) are increasingly used as vaccines and immunotherapeutics. Frequently, very time consuming density gradient centrifugation techniques are used for purification of VLPs. However, the progress towards optimized large-scale VLP production increased the demand for fast, cost efficient and scale able purification processes. We developed a chromatographic procedure for purification of HIV-1 gag VLPs produced in CHO cells. The clarified and filtered cell culture supernatant was directly processed on an anion-exchange monolith. The majority of host cell impurities passed through the column, whereas the VLPs were eluted by a linear or step salt gradient; the major fraction of DNA was eluted prior to VLPs and particles in the range of 100⿿200nm in diameter could be separated into two fractions. The earlier eluted fraction was enriched with extracellular particles associated to exosomes or microvesicles, whereas the late eluting fractions contained the majority of most pure HIV-1 gag VLPs. DNA content in the exosome-containing fraction could not be reduced by Benzonase treatment which indicated that the DNA was encapsulated. Many exosome markers were identified by proteomic analysis in this fraction. We present a laboratory method that could serve as a basis for rapid downstream processing of enveloped VLPs. Up to 2000 doses, each containing 1ÿ109 particles, could be processed with a 1mL monolith within 47min. The method compared to density gradient centrifugation has a 220-fold improvement in productivity.

Published

2015

50. Exoproteome analysis reveals higher abundance of proteins linked to alkaline stress in persistent Listeria monocytogenes strains

Author

Andreas Zaiser, Luminita Ciolacu, Kathrin Rychli, Stephan Schmitz-Esser, Ebrahim Razzazi-Fazeli, Tom Grunert, Martin Wagner, and Monika Ehling-Schulz

Subjects

0301 basic medicine, Food Safety, Proteome, Food Handling, 030106 microbiology, Virulence, Biology, medicine.disease_cause, Microbiology, Foodborne Diseases, 03 medical and health sciences, Listeria monocytogenes, Bacterial Proteins, Stress, Physiological, Cell Line, Tumor, Gene expression, medicine, Food microbiology, Humans, Electrophoresis, Gel, Two-Dimensional, Listeriosis, N-acetylmuramoyl-L-alanine amidase, Phylogeny, Principal Component Analysis, Strain (chemistry), Membrane Proteins, General Medicine, N-Acetylmuramoyl-L-alanine Amidase, Membrane protein, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Food Microbiology, Caco-2 Cells, Food Science, Multilocus Sequence Typing

Abstract

The foodborne pathogen Listeria monocytogenes, responsible for listeriosis a rare but severe infection disease, can survive in the food processing environment for month or even years. So-called persistent L. monocytogenes strains greatly increase the risk of (re)contamination of food products, and are therefore a great challenge for food safety. However, our understanding of the mechanism underlying persistence is still fragmented. In this study we compared the exoproteome of three persistent strains with the reference strain EGDe under mild stress conditions using 2D differential gel electrophoresis. Principal component analysis including all differentially abundant protein spots showed that the exoproteome of strain EGDe (sequence type (ST) 35) is distinct from that of the persistent strain R479a (ST8) and the two closely related ST121 strains 4423 and 6179. Phylogenetic analyses based on multilocus ST genes showed similar grouping of the strains. Comparing the exoproteome of strain EGDe and the three persistent strains resulted in identification of 22 differentially expressed protein spots corresponding to 16 proteins. Six proteins were significantly increased in the persistent L. monocytogenes exoproteomes, among them proteins involved in alkaline stress response (e.g. the membrane anchored lipoprotein Lmo2637 and the NADPH dehydrogenase NamA). In parallel the persistent strains showed increased survival under alkaline stress, which is often provided during cleaning and disinfection in the food processing environments. In addition, gene expression of the proteins linked to stress response (Lmo2637, NamA, Fhs and QoxA) was higher in the persistent strain not only at 37 °C but also at 10 °C. Invasion efficiency of EGDe was higher in intestinal epithelial Caco2 and macrophage-like THP1 cells compared to the persistent strains. Concurrently we found higher expression of proteins involved in virulence in EGDe e.g. the actin-assembly-inducing protein ActA and the surface virulence associated protein SvpA. Furthermore proteins involved in cell wall modification, such as the lipoteichonic acid primase LtaP and the N-acetylmuramoyl-l-alanine amidase (Lmo2591) are more abundant in EGDe than in the persistent strains and could indirectly contribute to virulence. In conclusion this study provides information about a set of proteins that could potentially support survival of L. monocytogenes in abiotic niches in food processing environments. Based on these data, a more detailed analysis of the role of the identified proteins under stresses mimicking conditions in food producing environment is essential for further elucidate the mechanism of the phenomenon of persistence of L. monocytogenes.

Published

2015