Your search keyword '"Kamil Mikulášek"' showing total 21 results

1. SP3 Protocol for Proteomic Plant Sample Preparation Prior LC-MS/MS

Author

Kamil Mikulášek, Hana Konečná, David Potěšil, Renata Holánková, Jan Havliš, and Zbyněk Zdráhal

Subjects

bottom-up, protein cleanup, Arabidopsis thaliana, sodium dodecyl sulfate removal, single-pot solid-phase-enhanced sample preparation, carboxylated magnetic beads, Plant culture, SB1-1110

Abstract

Quantitative protein extraction from biological samples, as well as contaminants removal before LC-MS/MS, is fundamental for the successful bottom-up proteomic analysis. Four sample preparation methods, including the filter-aided sample preparation (FASP), two single-pot solid-phase-enhanced sample preparations (SP3) on carboxylated or HILIC paramagnetic beads, and protein suspension trapping method (S-Trap) were evaluated for SDS removal and protein digestion from Arabidopsis thaliana (AT) lysate. Finally, the optimized carboxylated SP3 workflow was benchmarked closely against the routine FASP. Ultimately, LC-MS/MS analyses revealed that regarding the number of identifications, number of missed cleavages, proteome coverage, repeatability, reduction of handling time, and cost per assay, the SP3 on carboxylated magnetic particles proved to be the best alternative for SDS and other contaminants removal from plant sample lysate. A robust and efficient 2-h SP3 protocol for a wide range of protein input is presented, benefiting from no need to adjust the amount of beads, binding and rinsing conditions, or digestion parameters.

Published

2021

2. Filter-Aided Sample Preparation Procedure for Mass Spectrometric Analysis of Plant Histones

Author

Dominika Ledvinová, Kamil Mikulášek, Hana Kuchaříková, Sylva Brabencová, Miloslava Fojtová, Zbyněk Zdráhal, and Gabriela Lochmanová

Subjects

histone derivatization, filter-aided sample preparation, post-translational modifications, epigenetics, mass spectrometry, Arabidopsis thaliana, Plant culture, SB1-1110

Abstract

Characterization of histone post-translational modifications (PTMs) is still challenging, and robust histone sample preparation is essential for convincing evaluation of PTMs by mass spectrometry. An effective protocol for extracting plant histone proteins must also avoid excessive co-extraction of the numerous potential interfering compounds, including those related to secondary metabolism. Currently, the co-existence of histone marks is addressed mostly by shotgun proteomic analysis following chemical derivatization of histone lysine residues. Here, we report a straightforward approach for plant histone sample preparation for mass spectrometry, based on filter-aided sample preparation coupled with histone propionylation. The approach offers savings in sample handling and preparation time, enables removal of interfering compounds from the sample, and does not require either precipitation or dialysis of histone extract. We show the comparison of two protocol variants for derivatization of histone proteins, in-solution propionylation in the vial and propionylation on the filter unit. For both protocols, we obtained identical abundances of post-translationally modified histone peptides. Although shorter time is required for histone protein labeling on the filter unit, in-solution derivatization slightly outweighed filter-based variant by lower data variability. Nevertheless, both protocol variants appear to be efficient and convenient approach for preparation of plant histones for mass spectrometric analysis.

Published

2018

3. Content of 4(5)-methylimidazole, caffeine and chlorogenic acid in commercial coffee brands

Author

Thi Thanh Dieu Phan, Miroslava Bittová, Kamil Mikulášek, Stanislav Kráčmar, Vlastimil Kubáň, Pavel Valášek, and Blanka Svobodová

Subjects

coffee, spectrophotometric methods, HPLC, caffeine extractability, Nutrition. Foods and food supply, TX341-641

Abstract

Content of 4(5)-methylimidazole (4-MeI), caffeine and chlorogenic acid in commercial coffee brands were determined using high-performance liquid chromatography (HPLC) with UV DAD and MS detectors. Positive ion ESI mass spectra of the 4-MeI standard yielded intense signals corresponding to [M+H]+ (83.0604) and [2M+H]+ ions (165.1115). Also, adducts of 4-MeI with acetonitrile from mobile were detected - [M+ACN]+ ions (124.0849). The LOD of 2.5 ng mL-1 and LOQ of 8.4 ng.mL-1 were calculated according to the following formulas: LOD = 3.SD/S, and LOQ = 10.SD/S, where S is the slope of the calibration curve and SD is the standard deviation of the noise. The caffeine content was compared to the results of the standard addition, 1st derivative and liquid-liquid extraction spectrophotometry. 4-MeI was in tens µg g-1 in the Vietnamese coffees while in units µg.g-1 in all Czech and Brazilian coffees (-1 and -1, respectively). The results for caffeine were within the documented range (0.31 - 2.20%) in all coffee samples. The lower content of caffeine and chlorogenic acid was observed in Vietnamese coffees. All the methods used for determination of caffeine in the Czech and Brazilian coffees gave acceptable precision and accuracy. However, there were significant differences in the results in Vietnamese coffees. The caffeine extractability (100 °C, 3 min brewing) almost reached 100% in Czech and Brazilian coffees, while it was less than 90% in Vietnamese coffees. The Czech and Brazilian coffees tend to produce more caffeine in brews than the Vietnamese coffee because of the different composition of blends and the particle size degree.

Published

2015

4. Development of a Comprehensive Toxicity Pathway Model for 17α-Ethinylestradiol in Early Life Stage Fathead Minnows (Pimephales promelas)

Author

Bradley Park, Zbyněk Zdráhal, Natacha S. Hogan, Doug Crump, Kamil Mikulášek, Connor Burbridge, Jianguo Xia, Marek Pipal, Derek Green, David J. Schneider, David Potěšil, Niladri Basu, Alper James G. Alcaraz, Kerstin Bluhm, Markus Hecker, Markus Brinkmann, Taylor Lane, and Othman Soufan

Subjects

biology, medicine.drug_class, Physiology, Histology, General Chemistry, 010501 environmental sciences, 01 natural sciences, Early life, Transcriptome, Vitellogenin, Estrogen, Toxicity, biology.protein, medicine, Environmental Chemistry, Pimephales promelas, Development of the gonads, 0105 earth and related environmental sciences

Abstract

There is increasing pressure to develop alternative ecotoxicological risk assessment approaches that do not rely on expensive, time-consuming, and ethically questionable live animal testing. This study aimed to develop a comprehensive early life stage toxicity pathway model for the exposure of fish to estrogenic chemicals that is rooted in mechanistic toxicology. Embryo-larval fathead minnows (FHM; Pimephales promelas) were exposed to graded concentrations of 17α-ethinylestradiol (water control, 0.01% DMSO, 4, 20, and 100 ng/L) for 32 days. Fish were assessed for transcriptomic and proteomic responses at 4 days post-hatch (dph), and for histological and apical end points at 28 dph. Molecular analyses revealed core responses that were indicative of observed apical outcomes, including biological processes resulting in overproduction of vitellogenin and impairment of visual development. Histological observations indicated accumulation of proteinaceous fluid in liver and kidney tissues, energy depletion, and delayed or suppressed gonad development. Additionally, fish in the 100 ng/L treatment group were smaller than controls. Integration of omics data improved the interpretation of perturbations in early life stage FHM, providing evidence of conservation of toxicity pathways across levels of biological organization. Overall, the mechanism-based embryo-larval FHM model showed promise as a replacement for standard adult live animal tests.

Published

2021

5. Assessing the Toxicity of 17α-Ethinylestradiol in Rainbow Trout Using a 4-Day Transcriptomics Benchmark Dose (BMD) Embryo Assay

Author

Bradley Park, Jessica Ewald, Doug Crump, David J. Schneider, David Potěšil, Markus Hecker, Jianguo Xia, Connor Burbridge, Niladri Basu, Kamran Shekh, Alper James G. Alcaraz, Zbyněk Zdráhal, and Kamil Mikulášek

Subjects

Percentile, medicine.drug_class, 010501 environmental sciences, Biology, Ethinyl Estradiol, 01 natural sciences, Transcriptome, Andrology, 03 medical and health sciences, medicine, Environmental Chemistry, Animals, 030304 developmental biology, 0105 earth and related environmental sciences, 0303 health sciences, Embryo, Estrogens, General Chemistry, 17α ethinylestradiol, Benchmarking, Estrogen, Oncorhynchus mykiss, Toxicity, Estrogenic Effects, Rainbow trout, Water Pollutants, Chemical

Abstract

There is an urgent demand for more efficient and ethical approaches in ecological risk assessment. Using 17α-ethinylestradiol (EE2) as a model compound, this study established an embryo benchmark dose (BMD) assay for rainbow trout (RBT; Oncorhynchus mykiss) to derive transcriptomic points-of-departure (tPODs) as an alternative to live-animal tests. Embryos were exposed to graded concentrations of EE2 (measured: 0, 1.13, 1.57, 6.22, 16.3, 55.1, and 169 ng/L) from hatch to 4 and up to 60 days post-hatch (dph) to assess molecular and apical responses, respectively. Whole proteome analyses of alevins did not show clear estrogenic effects. In contrast, transcriptomics revealed responses that were in agreement with apical effects, including excessive accumulation of intravascular and hepatic proteinaceous fluid and significant increases in mortality at 55.1 and 169 ng/L EE2 at later time points. Transcriptomic BMD analysis estimated the median of the 20th lowest geneBMD to be 0.18 ng/L, the most sensitive tPOD. Other estimates (0.78, 3.64, and 1.63 ng/L for the 10th percentile geneBMD, first peak geneBMD distribution, and median geneBMD of the most sensitive over-represented pathway, respectively) were within the same order of magnitude as empirically derived apical PODs for EE2 in the literature. This 4-day alternative RBT embryonic assay was effective in deriving tPODs that are protective of chronic effects of EE2.

Published

2021

6. Death Receptor 5 (TNFRSF10B) Is Upregulated and TRAIL Resistance Is Reversed in Hypoxia and Normoxia in Colorectal Cancer Cell Lines after Treatment with Skyrin, the Active Metabolite of Hypericum spp

Author

Zbyněk Zdráhal, Rastislav Jendželovský, Peter Fedoročko, Kamil Mikulášek, Marián Babinčák, Ján Košuth, Martin Majerník, and Jana Vargová

Subjects

Cancer Research, Death receptor 5, Reversion, colorectal cancer, TRAIL, lcsh:RC254-282, Article, 03 medical and health sciences, 0302 clinical medicine, proteomics, Downregulation and upregulation, medicine, Active metabolite, 030304 developmental biology, 0303 health sciences, Chemistry, hypoxia, Hypericum, Hypoxia (medical), lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, skyrin, TRAIL resistance, 3. Good health, Oncology, Mechanism of action, Cell culture, Apoptosis, 030220 oncology & carcinogenesis, Cancer research, Tumor necrosis factor alpha, medicine.symptom

Abstract

Simple Summary Hypoxic conditions are common in solid tumors and are very often connected with the poor prognosis of cancer patients. The lack of oxygen often causes the failure of therapy due to multiple mechanisms increasing cancer survival. Skyrin (SKR) is a secondary plant metabolite from the genus Hypericum spp., with a potential anticancer effects but still unknown mechanism of action. Based on our comprehensive analysis of SKR action, SKR shows significant efficiency against cancer, but not healthy cells, induces apoptosis, and upregulates Death receptor 5 in cancer cells in normoxic, as well as hypoxic conditions. SKR reverses TRAIL resistance even in TRAIL-resistant cancer cell lines in hypoxia. To sum up, SKR can be possibly used as a natural antitumor drug per se or as an adjuvant to TRAIL treatment in hypoxic and therapy-resistant tumors. Abstract Skyrin (SKR) is a plant bisanthraquinone secondary metabolite from the Hypericum genus with potential use in anticancer therapy. However, its effect and mechanism of action are still unknown. The negative effect of SKR on HCT 116 and HT-29 cancer cell lines in hypoxic and normoxic conditions was observed. HCT 116 cells were more responsive to SKR treatment as demonstrated by decreased metabolic activity, cellularity and accumulation of cells in the G1 phase. Moreover, an increasing number of apoptotic cells was observed after treatment with SKR. Based on the LC-MS comparative proteomic data from hypoxia and normoxia (data are available via ProteomeXchange with the identifier PXD019995), SKR significantly upregulated Death receptor 5 (DR5), which was confirmed by real-time qualitative PCR (RT-qPCR). Furthermore, multiple changes in the Tumor necrosis factor-related apoptosis-inducing ligand (TRAIL)-activated cascade were observed. Moreover, the reversion of TRAIL resistance was observed in HCT 116, HT-29 and SW620 cell lines, even in hypoxia, which was linked to the upregulation of DR5. In conclusion, our results propose the use of SKR as a prospective anticancer drug, particularly as an adjuvant to TRAIL-targeting treatment to reverse TRAIL resistance in hypoxia.

Published

2021

7. Development of a Comprehensive Toxicity Pathway Model for 17α-Ethinylestradiol in Early Life Stage Fathead Minnows (

Author

Alper James G, Alcaraz, David, Potěšil, Kamil, Mikulášek, Derek, Green, Bradley, Park, Connor, Burbridge, Kerstin, Bluhm, Othman, Soufan, Taylor, Lane, Marek, Pipal, Markus, Brinkmann, Jianguo, Xia, Zbyněk, Zdráhal, David, Schneider, Doug, Crump, Niladri, Basu, Natacha, Hogan, and Markus, Hecker

Subjects

Proteomics, Vitellogenins, Sex Differentiation, Cyprinidae, Animals, Ethinyl Estradiol, Water Pollutants, Chemical

Abstract

There is increasing pressure to develop alternative ecotoxicological risk assessment approaches that do not rely on expensive, time-consuming, and ethically questionable live animal testing. This study aimed to develop a comprehensive early life stage toxicity pathway model for the exposure of fish to estrogenic chemicals that is rooted in mechanistic toxicology. Embryo-larval fathead minnows (FHM

Published

2021

8. A Model of Aerobic and Anaerobic Metabolism of Hydrogen in the Extremophile Acidithiobacillus ferrooxidans

Author

Sabrina Hedrich, Martin Mandl, Oldrich Janiczek, D. Barrie Johnson, Jan Lochman, Pavel Bouchal, Kamil Mikulášek, Jiri Kucera, and Eva Pakostova

Subjects

Microbiology (medical), Ubiquinol, Cytochrome, Acidithiobacillus, lcsh:QR1-502, Microbiology, lcsh:Microbiology, 03 medical and health sciences, chemistry.chemical_compound, Rusticyanin, Electrochemical gradient, extremophiles, Original Research, 030304 developmental biology, 0303 health sciences, Oxidase test, biology, 030306 microbiology, Chemistry, Cytochrome c, hydrogen metabolism, multi-omics, oxygen reduction, 13. Climate action, Coenzyme Q – cytochrome c reductase, biology.protein, Biophysics, ferric iron reduction, Cytochrome aa3

Abstract

Hydrogen can serve as an electron donor for chemolithotrophic acidophiles, especially in the deep terrestrial subsurface and geothermal ecosystems. Nevertheless, the current knowledge of hydrogen utilization by mesophilic acidophiles is minimal. A multi-omics analysis was applied on Acidithiobacillus ferrooxidans growing on hydrogen, and a respiratory model was proposed. In the model, [NiFe] hydrogenases oxidize hydrogen to two protons and two electrons. The electrons are used to reduce membrane-soluble ubiquinone to ubiquinol. Genetically associated iron-sulfur proteins mediate electron relay from the hydrogenases to the ubiquinone pool. Under aerobic conditions, reduced ubiquinol transfers electrons to either cytochrome aa3 oxidase via cytochrome bc1 complex and cytochrome c4 or the alternate directly to cytochrome bd oxidase, resulting in proton efflux and reduction of oxygen. Under anaerobic conditions, reduced ubiquinol transfers electrons to outer membrane cytochrome c (ferrireductase) via cytochrome bc1 complex and a cascade of electron transporters (cytochrome c4, cytochrome c552, rusticyanin, and high potential iron-sulfur protein), resulting in proton efflux and reduction of ferric iron. The proton gradient generated by hydrogen oxidation maintains the membrane potential and allows the generation of ATP and NADH. These results further clarify the role of extremophiles in biogeochemical processes and their impact on the composition of the deep terrestrial subsurface.

Published

2020

9. The oligomeric states of elicitins affect the hypersensitive response and resistance in tobacco

Author

Martina Zapletalová, Annick Chiltz, Zbyněk Zdráhal, Marek Petřivalský, Kamil Mikulášek, Nathalie Leborgne-Castel, Martin Solanský, Jan Lochman, Department of Biochemistry, Faculty of Science, Masaryk University, Kotlářská 2, 61137 Brno, Czech Republic, Central European Institute of Technology, Masaryk University, Kamenice 5, 625 00 Brno, Czech Republic, Department of Biochemistry, 3Department of Botany, Faculty of Science, Palacký University, Šlechtitelů 27, 78371 Olomouc, Czech Republic, Agroécologie [Dijon], and Université de Bourgogne (UB)-AgroSup Dijon - Institut National Supérieur des Sciences Agronomiques, de l'Alimentation et de l'Environnement-Université Bourgogne Franche-Comté [COMUE] (UBFC)-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE)

Subjects

0106 biological sciences, Hypersensitive response, hypersensitive response, Physiology, Nicotiana tabacum, [SDV]Life Sciences [q-bio], oligomeric structure, Plant Science, 01 natural sciences, Cell wall, resistance, 03 medical and health sciences, Transduction (genetics), Tobacco, elicitin response, Amino Acid Sequence, signalling, 030304 developmental biology, Plant Diseases, 0303 health sciences, biology, Chemistry, Pattern recognition receptor, Elicitin, phytophthora, biology.organism_classification, Cell biology, suppressor of bir1-1 (SOBIR1), Oomycetes, cell wall, Phytophthora, Solanaceae, elicitin b-CRY, 010606 plant biology & botany

Abstract

Successful plant defence against microbial pathogens is based on early recognition and fast activation of inducible responses. Key mechanisms include detection of microbe-associated molecular patterns by membrane-localized pattern recognition receptors that induce a basal resistance response. A well-described model of such responses to pathogens involves the interactions between Solanaceae plants and proteinaceous elicitors secreted by oomycetes, called elicitins. It has been hypothesized that the formation of oligomeric structures by elicitins could be involved in their recognition and activation of defensive transduction cascades. In this study, we tested this hypothesis using several approaches, and we observed differences in tobacco plant responses induced by the elicitin β-cryptogein (β-CRY) and its homodimer, β-CRYDIM. We also found that the C-terminal domain of elicitins of other ELI (true-elicitin) clades plays a significant role in stabilization of their oligomeric structure and restraint in the cell wall. In addition, covalently cross-linking β-CRYDIM impaired the formation of signalling complexes, thereby reducing its capacity to elicit the hypersensitive response and resistance in the host plant, with no significant changes in pathogenesis-related protein expression. By revealing the details of the effects of β-CRY dimerization on recognition and defence responses in tobacco, our results shed light on the poorly understood role of elicitins’ oligomeric structures in the interactions between oomycetes and plants.

Published

2020

10. Tick-borne Encephalitis Virus Vaccines Contain Non-structural Protein 1 (NS1) Antigen and May Elicit NS1-Specific Antibody Responses in Vaccinated Individuals

Author

Zbyněk Zdráhal, Juraj Petrik, Dana Teislerova, Martin Palus, Jan Haviernik, Aleš Chrdle, Petra Formanová, Osmany Larralde, Daniel Ruzek, Jana Elsterová, Kamil Mikulášek, Jiri Salat, and Ludek Eyer

Subjects

biology, viruses, Tick-borne encephalitis, Structural protein, Ns1 antigen, biochemical phenomena, metabolism, and nutrition, medicine.disease, biology.organism_classification, Virology, virology, Vaccination, Specific antibody, Flavivirus, Tick-borne encephalitis virus, medicine

Abstract

Vaccination against tick-borne encephalitis (TBE) is based on the use of formalin-inactivated, culture-derived whole-virus vaccines. Immune response following vaccination is primarily directed to the viral envelope (E) protein, the major viral surface antigen. In Europe, two TBE vaccines are available in adult and pediatric formulations, FSME-IMMUN® (Pfizer) and Encepur® (GlaxoSmithKline). Herein, we analyzed the content of these vaccines using mass spectrometry (MS). The MS analysis revealed that the Encepur vaccine contains not only proteins of the whole virus particle, but also viral non-structural protein 1 (NS1). MS analysis of the FSME-IMMUN vaccine failed due to the high content of human serum albumin used as a stabilizer in the vaccine. However, the presence of NS1 in FSME-IMMUN was confirmed by immunization of mice with six doses of this vaccine, which led to a robust anti-NS1 antibody response. NS1-specific western blot analysis detected anti-NS1 antibodies also in sera of humans who received multiple doses of either of these two vaccines; however, most vaccinees who received ≤3 doses were negative for NS1-specific antibodies. The contribution of NS1-specific antibodies to protection against TBE was demonstrated by immunization of mice with purified NS1 antigen, which led to a significant (p < 0.01) prolongation of the mean survival time after lethal virus challenge. This indicates that stimulation of anti-NS1 immunity by the TBE vaccines may increase their protective effect.

Published

2020

11. Tick-Borne Encephalitis Virus Vaccines Contain Non-Structural Protein 1 Antigen and may Elicit NS1-Specific Antibody Responses in Vaccinated Individuals

Author

Osmany Larralde, Juraj Petrik, Dana Teislerova, Zbynek Zdrahal, Kamil Mikulášek, Martin Palus, Daniel Ruzek, Petra Formanová, Jan Haviernik, Aleš Chrdle, Jiri Salat, Ludek Eyer, and Jana Elsterová

Subjects

0301 basic medicine, viruses, Immunology, ns1, lcsh:Medicine, chemical and pharmacologic phenomena, Article, 03 medical and health sciences, 0302 clinical medicine, Antigen, flavivirus, Immunity, vaccine, Drug Discovery, medicine, Pharmacology (medical), 030212 general & internal medicine, Pharmacology, biology, business.industry, tick-borne encephalitis, lcsh:R, Tick-borne encephalitis, biochemical phenomena, metabolism, and nutrition, medicine.disease, biology.organism_classification, vaccination, Virology, 3. Good health, Vaccination, Tick-borne encephalitis virus, Flavivirus, 030104 developmental biology, Infectious Diseases, Immunization, biology.protein, Antibody, business

Abstract

Vaccination against tick-borne encephalitis (TBE) is based on the use of formalin-inactivated, culture-derived whole-virus vaccines. Immune response following vaccination is primarily directed to the viral envelope (E) protein, the major viral surface antigen. In Europe, two TBE vaccines are available in adult and pediatric formulations, namely FSME-IMMUN&reg, (Pfizer) and Encepur&reg, (GlaxoSmithKline). Herein, we analyzed the content of these vaccines using mass spectrometry (MS). The MS analysis revealed that the Encepur vaccine contains not only proteins of the whole virus particle, but also viral non-structural protein 1 (NS1). MS analysis of the FSME-IMMUN vaccine failed due to the high content of human serum albumin used as a stabilizer in the vaccine. However, the presence of NS1 in FSME-IMMUN was confirmed by immunization of mice with six doses of this vaccine, which led to a robust anti-NS1 antibody response. NS1-specific Western blot analysis also detected anti-NS1 antibodies in sera of humans who received multiple doses of either of these two vaccines, however, most vaccinees who received &le, 3 doses were negative for NS1-specific antibodies. The contribution of NS1-specific antibodies to protection against TBE was demonstrated by immunization of mice with purified NS1 antigen, which led to a significant (p &lt, 0.01) prolongation of the mean survival time after lethal virus challenge. This indicates that stimulation of anti-NS1 immunity by the TBE vaccines may increase their protective effect.

Published

2020

12. Nuclear inclusions of pathogenic ataxin-1 induce oxidative stress and perturb the protein synthesis machinery

Author

Fotis Psomopoulos, Zoltán Ivics, Boris Tichy, Maria Lefaki, Zsuzsanna Izsvák, Maria Tsagiopoulou, Gregorio Alanis-Lobato, Šárka Pospíšilová, Jan Pribyl, Niki Chondrogianni, Georgia Kastrinaki, Tamás Raskó, Spyros Petrakis, Petr Skládal, Kamil Mikulášek, Alessandro Prigione, Manvendra K. Singh, Stamatia Laidou, Miguel A. Andrade-Navarro, Jan Oppelt, and Annika Zink

Subjects

0301 basic medicine, SCA1, Spinocerebellar ataxia type-1, Intranuclear Inclusion Bodies, Clinical Biochemistry, MSC, mesenchymal stem cell, Protein aggregation, Biochemistry, 0302 clinical medicine, Mutant protein, Protein biosynthesis, DE, differentially expressed genes, Nuclear protein, lcsh:QH301-705.5, FTIR, Fourier-transform infrared spectroscopy, Ataxin-1, lcsh:R5-920, biology, Chemistry, Nuclear Proteins, polyQ, polyglutamine, Ribosome, Cell biology, SB, Sleeping Beauty, Polyglutamine, Oxidative stress, Transposon, Sleeping beauty transposon, Protein network, Spinocerebellar ataxia, Protein folding, Cellular model, Function and Dysfunction of the Nervous System, lcsh:Medicine (General), Research Paper, iPSC, induced pluripotent stem cell, Ataxin 1, Nerve Tissue Proteins, PPI, protein-protein interaction, 03 medical and health sciences, ROS, reactive oxygen species, GSEA, Gene Set Enrichment Analysis, medicine, Humans, NPC, neural progenitor cell, Organic Chemistry, medicine.disease, AFM, atomic force microscopy, Oxidative Stress, 030104 developmental biology, lcsh:Biology (General), IIBs, intranuclear inclusion bodies, MS, mass spectrometry, Cardiovascular and Metabolic Diseases, biology.protein, 030217 neurology & neurosurgery

Abstract

Spinocerebellar ataxia type-1 (SCA1) is caused by an abnormally expanded polyglutamine (polyQ) tract in ataxin-1. These expansions are responsible for protein misfolding and self-assembly into intranuclear inclusion bodies (IIBs) that are somehow linked to neuronal death. However, owing to lack of a suitable cellular model, the downstream consequences of IIB formation are yet to be resolved. Here, we describe a nuclear protein aggregation model of pathogenic human ataxin-1 and characterize IIB effects. Using an inducible Sleeping Beauty transposon system, we overexpressed the ATXN1(Q82) gene in human mesenchymal stem cells that are resistant to the early cytotoxic effects caused by the expression of the mutant protein. We characterized the structure and the protein composition of insoluble polyQ IIBs which gradually occupy the nuclei and are responsible for the generation of reactive oxygen species. In response to their formation, our transcriptome analysis reveals a cerebellum-specific perturbed protein interaction network, primarily affecting protein synthesis. We propose that insoluble polyQ IIBs cause oxidative and nucleolar stress and affect the assembly of the ribosome by capturing or down-regulating essential components. The inducible cell system can be utilized to decipher the cellular consequences of polyQ protein aggregation. Our strategy provides a broadly applicable methodology for studying polyQ diseases.

Published

2020

13. Comparative analysis of transcriptomic points-of-departure (tPODs) and apical responses in embryo-larval fathead minnows exposed to fluoxetine

Author

Alper James G. Alcaraz, Shaina Baraniuk, Kamil Mikulášek, Bradley Park, Taylor Lane, Connor Burbridge, Jessica Ewald, David Potěšil, Jianguo Xia, Zbyněk Zdráhal, David Schneider, Doug Crump, Niladri Basu, Natacha Hogan, Markus Brinkmann, and Markus Hecker

Subjects

Fluoxetine, Larva, Health, Toxicology and Mutagenesis, Cyprinidae, Animals, General Medicine, Transcriptome, Toxicology, Pollution, Water Pollutants, Chemical

Abstract

Current approaches in chemical hazard assessment face significant challenges because they rely on live animal testing, which is time-consuming, expensive, and ethically questionable. These concerns serve as an impetus to develop new approach methodologies (NAMs) that do not rely on live animal tests. This study explored a molecular benchmark dose (BMD) approach using a 7-day embryo-larval fathead minnow (FHM) assay to derive transcriptomic points-of-departure (tPODs) to predict apical BMDs of fluoxetine (FLX), a highly prescribed and potent selective serotonin reuptake inhibitor frequently detected in surface waters. Fertilized FHM embryos were exposed to graded concentrations of FLX (confirmed at LOD, 0.19, 0.74, 3.38, 10.2, 47.5 μg/L) for 32 days. Subsets of fish were subjected to omics and locomotor analyses at 7 days post-fertilization (dpf) and to histological and biometric measurements at 32 dpf. Enrichment analyses of transcriptomics and proteomics data revealed significant perturbations in gene sets associated with serotonergic and axonal functions. BMD analysis resulted in tPOD values of 0.56 μg/L (median of the 20 most sensitive gene-level BMDs), 5.0 μg/L (tenth percentile of all gene-level BMDs), 7.51 μg/L (mode of the first peak of all gene-level BMDs), and 5.66 μg/L (pathway-level BMD). These tPODs were protective of locomotor and reduced body weight effects (LOEC of 10.2 μg/L) observed in this study and were reflective of chronic apical BMDs of FLX reported in the literature. Furthermore, the distribution of gene-level BMDs followed a bimodal pattern, revealing disruption of sensitive neurotoxic pathways at low concentrations and metabolic pathway perturbations at higher concentrations. This is one of the first studies to derive protective tPODs for FLX using a short-term embryo assay at a life stage not considered to be a live animal under current legislations.

Published

2022

14. Sequence-dependent separation of trinucleotides by ion-interaction reversed-phase liquid chromatography—A structure-retention study assisted by soft-modelling and molecular dynamics

Author

Kamil Mikulášek, Miroslava Bittová, Petr Kulhánek, Kamil S. Jaroň, and Jan Havliš

Subjects

Guanine, Static Electricity, Oligonucleotides, Quantitative Structure-Activity Relationship, Molecular Dynamics Simulation, 010402 general chemistry, 01 natural sciences, Biochemistry, Analytical Chemistry, Nucleobase, Accessible surface area, Molecular dynamics, Phase (matter), Molecule, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, Chromatography, Chemistry, Component (thermodynamics), Adenine, 010401 analytical chemistry, Organic Chemistry, Solvation, Water, General Medicine, Reversed-phase chromatography, 0104 chemical sciences, Solvents, Neural Networks, Computer, Thymine

Abstract

We studied sequence-dependent retention properties of synthetic 5′-terminal phosphate absent trinucleotides containing adenine, guanine and thymine through reversed-phase liquid chromatography (RPLC) and QSRR modelling. We investigated the influence of separation conditions, namely mobile phase composition (ion interaction agent content, pH and organic constituent content), on sequence-dependent separation by means of ion-interaction RPLC (II-RPLC) using two types of models: experimental design–artificial neural networks (ED-ANN), and linear regression based on molecular dynamics data. The aim was to determine those properties of the above-mentioned analytes responsible for the retention dependence of the sequence. Our results show that there is a deterministic relation between sequence and II-RPLC retention properties of the studied trinucleotides. Further, we can conclude that the higher the content of ion-interaction agent in the mobile phase, the more prominent these properties are. We also show that if we approximate the polar component of solvation energy in QSRR by the electrostatic work in transferring molecules from vacuum to water, and the non-polar component by the solvent accessible surface area, these parameters best describe the retention properties of trinucleotides. There are some exceptions to this finding, namely sequences 5′-NAN-3′, 5′-ANN-3′, 5′-TGN-3′, 5′-NTA-3′and 5′-NGA-3′ (N stands for generic nucleotide). Their role is still unknown, but since linear regression including these specific constellations showed a higher observable variance coverage than the model with only the basic descriptors, we may assume that solvent-analyte interactions are responsible for the exceptional behaviour of 5′-NAN-3′ & 5′-ANN-3′ trinucleotides and some intramolecular interactions of neighbouring nucleobases for 5′-TGN-3′, 5′-NTA-3′and 5′-NGA-3′ trinucleotides.

Published

2016

15. Filter-Aided Sample Preparation Procedure for Mass Spectrometric Analysis of Plant Histones

Author

Hana Kuchaříková, Dominika Ledvinová, Gabriela Lochmanová, Sylva Brabencová, Zbyněk Zdráhal, Kamil Mikulášek, and Miloslava Fojtová

Subjects

0301 basic medicine, Arabidopsis thaliana, Lysine, histone derivatization, Plant Science, lcsh:Plant culture, Mass spectrometry, 03 medical and health sciences, chemistry.chemical_compound, filter-aided sample preparation, Methods, post-translational modifications, Sample preparation, lcsh:SB1-1110, Epigenetics, Derivatization, mass spectrometry, Chromatography, 030102 biochemistry & molecular biology, biology, epigenetics, Mass spectrometric, 030104 developmental biology, Histone, chemistry, Filter (video), biology.protein

Abstract

Characterization of histone post-translational modifications (PTMs) is still challenging, and robust histone sample preparation is essential for convincing evaluation of PTMs by mass spectrometry. An effective protocol for extracting plant histone proteins must also avoid excessive co-extraction of the numerous potential interfering compounds, including those related to secondary metabolism. Currently, the co-existence of histone marks is addressed mostly by shotgun proteomic analysis following chemical derivatization of histone lysine residues. Here, we report a straightforward approach for plant histone sample preparation for mass spectrometry, based on filter-aided sample preparation coupled with histone propionylation. The approach offers savings in sample handling and preparation time, enables removal of interfering compounds from the sample, and does not require either precipitation or dialysis of histone extract. We show the comparison of two protocol variants for derivatization of histone proteins, in-solution propionylation in the vial and propionylation on the filter unit. For both protocols, we obtained identical abundances of post-translationally modified histone peptides. Although shorter time is required for histone protein labeling on the filter unit, in-solution derivatization slightly outweighed filter-based variant by lower data variability. Nevertheless, both protocol variants appear to be efficient and convenient approach for preparation of plant histones for mass spectrometric analysis.

Published

2018

16. Staphylococcus petrasii diagnostics and its pathogenic potential enhanced by mobile genetic elements

Author

Vojtěch Kovařovic, Pavel Švec, Ivo Sedláček, Lenka Fišarová, Jiří Doškař, Ivana Mašlaňová, Veronika Vrbovská, Petr Petráš, Adéla Indráková, Ondrej Šedo, Roman Pantůček, Marta Šiborová, and Kamil Mikulášek

Subjects

Microbiology (medical), Genotype, Virulence Factors, Staphylococcus, Virulence, Microbial Sensitivity Tests, Biology, medicine.disease_cause, Ribotyping, Microbiology, Genome, 03 medical and health sciences, Plasmid, medicine, Humans, 030304 developmental biology, Genetics, Comparative genomics, 0303 health sciences, 030306 microbiology, Genomics, General Medicine, Bacterial Typing Techniques, Electrophoresis, Gel, Pulsed-Field, Interspersed Repetitive Sequences, Phenotype, Infectious Diseases, Staphylococcus aureus, Mobile genetic elements, Coagulase, Genome, Bacterial

Abstract

Staphylococcus petrasii is recently described coagulase negative staphylococcal species and an opportunistic human pathogen, still often misidentified in clinical specimens. Four subspecies are distinguished in S. petrasii by polyphasic taxonomical analyses, however a comparative study has still not been done on the majority of isolates and their genome properties have not yet been thoroughly analysed. Here, we describe the phenotypic and genotypic characteristics of 65 isolates and the results of de novo sequencing, whole genome assembly and annotation of draft genomes of five strains. The strains were identified by MALDI-TOF mass spectrometry to the species level and the majority of the strains were identified to the subspecies level by fingerprinting methods, (GTG)5 repetitive PCR and ribotyping. Macrorestriction profiling by pulsed-field gel electrophoresis was confirmed to be a suitable strain typing method. Comparative genomics revealed the presence of new mobile genetic elements carrying antimicrobial resistance factors such as staphylococcal cassette chromosome (SCC) mec, transposones, phage-inducible genomic islands, and plasmids. Their mosaic structure and similarity across coagulase-negative staphylococci and Staphylococcus aureus suggest the possible exchange of these elements. Numerous putative virulence factors such as adhesins, autolysins, exoenzymes, capsule formation genes, immunomodulators, the phage-associated sasX gene, and SCC-associated spermidine N-acetyltransferase gene, pseudouridine and sorbitol utilization operons might explain clinical manifestations of S. petrasii isolates. The increasing recovery of S. petrasii isolates from human clinical material, the multi-drug resistance including methicillin resistance of S. petrasii subsp. jettensis strains, and virulence factors homologous to other pathogenic staphylococci demonstrate the importance of the species in human disease.

Published

2019

17. Content of 4(5)-methylimidazole, caffeine and chlorogenic acid in commercial coffee brands

Author

Pavel Valášek, Blanka Svobodová, Stanislav Kráčmar, Thi Thanh Dieu Phan, Vlastimil Kubáň, Kamil Mikulášek, and Miroslava Bittová

Subjects

Caffeine extractability, coffee, lcsh:TX341-641, Coffee, 01 natural sciences, High-performance liquid chromatography, chemistry.chemical_compound, 0404 agricultural biotechnology, Chlorogenic acid, Spectrophotometry, medicine, Food science, caffeine extractability, Chromatography, medicine.diagnostic_test, 010401 analytical chemistry, Extraction (chemistry), Spectrophotometric methods, 04 agricultural and veterinary sciences, spectrophotometric methods, 040401 food science, 0104 chemical sciences, chemistry, Standard addition, Composition (visual arts), HPLC, Caffeine, lcsh:Nutrition. Foods and food supply, Food Science

Abstract

Content of 4(5)-methylimidazole (4-MeI), caffeine and chlorogenic acid in commercial coffee brands were determined using high-performance liquid chromatography (HPLC) with UV DAD and MS detectors. Positive ion ESI mass spectra of the 4-MeI standard yielded intense signals corresponding to [M+H]+ (83.0604) and [2M+H]+ ions (165.1115). Also, adducts of 4-MeI with acetonitrile from mobile were detected - [M+ACN]+ ions (124.0849). The LOD of 2.5 ng mL-1 and LOQ of8.4 ng.mL-1 were calculated according to the following formulas: LOD = 3.SD/S, and LOQ = 10.SD/S, where S is the slope of the calibration curve and SD is the standard deviation of the noise. The caffeine content was compared to the results of the standard addition, 1st derivative and liquid-liquid extraction spectrophotometry. 4-MeI was in tens µg g-1 in the Vietnamese coffees while in units µg.g-1 in all Czech and Brazilian coffees (-1 and -1, respectively). The results for caffeine were within the documented range (0.31 - 2.20%) in all coffee samples. The lower content of caffeine and chlorogenic acid was observed in Vietnamese coffees. All the methods used for determination of caffeine in the Czech and Brazilian coffees gave acceptable precision and accuracy. However, there were significant differences in the results in Vietnamese coffees. The caffeine extractability (100 °C, 3 min brewing) almost reached 100% in Czech and Brazilian coffees, while it was less than 90% in Vietnamese coffees. The Czech and Brazilian coffees tend to produce more caffeine in brews than the Vietnamese coffee because of the different composition of blends and the particle size degree.&nbsp

Published

2015

18. Staphylococcus sciuri bacteriophages double-convert for staphylokinase and phospholipase, mediate interspecies plasmid transduction, and package mecA gene

Author

Veronika Vrbovská, Ivana Mašlaňová, Jiří Doškař, Kamil Mikulášek, Kamila Bendíčková, Michal Zeman, Marta Šiborová, Adéla Indráková, Zbyněk Zdráhal, Roman Pantůček, and Pavel Plevka

Subjects

0301 basic medicine, Gene Transfer, Horizontal, Staphylococcus, viruses, Virus Attachment, Virulence, Genome, Viral, Article, Host Specificity, Microbiology, Siphoviridae, 03 medical and health sciences, Transduction (genetics), Plasmid, Transduction, Genetic, Staphylococcus sciuri, Prophage, Genetics, Multidisciplinary, biology, SCCmec, Metalloendopeptidases, Genomics, biology.organism_classification, 030104 developmental biology, Genes, Bacterial, Phospholipases, Horizontal gene transfer, Staphylococcus Phages, Plasmids

Abstract

Staphylococcus sciuri is a bacterial pathogen associated with infections in animals and humans, and represents a reservoir for the mecA gene encoding methicillin-resistance in staphylococci. No S. sciuri siphophages were known. Here the identification and characterization of two temperate S. sciuri phages from the Siphoviridae family designated ϕ575 and ϕ879 are presented. The phages have icosahedral heads and flexible noncontractile tails that end with a tail spike. The genomes of the phages are 42,160 and 41,448 bp long and encode 58 and 55 ORFs, respectively, arranged in functional modules. Their head-tail morphogenesis modules are similar to those of Staphylococcus aureus ϕ13-like serogroup F phages, suggesting their common evolutionary origin. The genome of phage ϕ575 harbours genes for staphylokinase and phospholipase that might enhance the virulence of the bacterial hosts. In addition both of the phages package a homologue of the mecA gene, which is a requirement for its lateral transfer. Phage ϕ879 transduces tetracycline and aminoglycoside pSTS7-like resistance plasmids from its host to other S. sciuri strains and to S. aureus. Furthermore, both of the phages efficiently adsorb to numerous staphylococcal species, indicating that they may contribute to interspecies horizontal gene transfer.

Published

2017

19. A Model of Aerobic and Anaerobic Metabolism of Hydrogen in the Extremophile Acidithiobacillus ferrooxidans

Author

Jiri Kucera, Jan Lochman, Pavel Bouchal, Eva Pakostova, Kamil Mikulasek, Sabrina Hedrich, Oldrich Janiczek, Martin Mandl, and D. Barrie Johnson

Subjects

Acidithiobacillus, extremophiles, ferric iron reduction, hydrogen metabolism, multi-omics, oxygen reduction, Microbiology, QR1-502

Abstract

Hydrogen can serve as an electron donor for chemolithotrophic acidophiles, especially in the deep terrestrial subsurface and geothermal ecosystems. Nevertheless, the current knowledge of hydrogen utilization by mesophilic acidophiles is minimal. A multi-omics analysis was applied on Acidithiobacillus ferrooxidans growing on hydrogen, and a respiratory model was proposed. In the model, [NiFe] hydrogenases oxidize hydrogen to two protons and two electrons. The electrons are used to reduce membrane-soluble ubiquinone to ubiquinol. Genetically associated iron-sulfur proteins mediate electron relay from the hydrogenases to the ubiquinone pool. Under aerobic conditions, reduced ubiquinol transfers electrons to either cytochrome aa3 oxidase via cytochrome bc1 complex and cytochrome c4 or the alternate directly to cytochrome bd oxidase, resulting in proton efflux and reduction of oxygen. Under anaerobic conditions, reduced ubiquinol transfers electrons to outer membrane cytochrome c (ferrireductase) via cytochrome bc1 complex and a cascade of electron transporters (cytochrome c4, cytochrome c552, rusticyanin, and high potential iron-sulfur protein), resulting in proton efflux and reduction of ferric iron. The proton gradient generated by hydrogen oxidation maintains the membrane potential and allows the generation of ATP and NADH. These results further clarify the role of extremophiles in biogeochemical processes and their impact on the composition of the deep terrestrial subsurface.

Published

2020

20. Nuclear inclusions of pathogenic ataxin-1 induce oxidative stress and perturb the protein synthesis machinery

Author

Stamatia Laidou, Gregorio Alanis-Lobato, Jan Pribyl, Tamás Raskó, Boris Tichy, Kamil Mikulasek, Maria Tsagiopoulou, Jan Oppelt, Georgia Kastrinaki, Maria Lefaki, Manvendra Singh, Annika Zink, Niki Chondrogianni, Fotis Psomopoulos, Alessandro Prigione, Zoltán Ivics, Sarka Pospisilova, Petr Skladal, Zsuzsanna Izsvák, Miguel A. Andrade-Navarro, and Spyros Petrakis

Subjects

Ataxin-1, Polyglutamine, Sleeping beauty transposon, Oxidative stress, Protein network, Ribosome, Medicine (General), R5-920, Biology (General), QH301-705.5

Abstract

Spinocerebellar ataxia type-1 (SCA1) is caused by an abnormally expanded polyglutamine (polyQ) tract in ataxin-1. These expansions are responsible for protein misfolding and self-assembly into intranuclear inclusion bodies (IIBs) that are somehow linked to neuronal death. However, owing to lack of a suitable cellular model, the downstream consequences of IIB formation are yet to be resolved. Here, we describe a nuclear protein aggregation model of pathogenic human ataxin-1 and characterize IIB effects. Using an inducible Sleeping Beauty transposon system, we overexpressed the ATXN1(Q82) gene in human mesenchymal stem cells that are resistant to the early cytotoxic effects caused by the expression of the mutant protein. We characterized the structure and the protein composition of insoluble polyQ IIBs which gradually occupy the nuclei and are responsible for the generation of reactive oxygen species. In response to their formation, our transcriptome analysis reveals a cerebellum-specific perturbed protein interaction network, primarily affecting protein synthesis. We propose that insoluble polyQ IIBs cause oxidative and nucleolar stress and affect the assembly of the ribosome by capturing or down-regulating essential components. The inducible cell system can be utilized to decipher the cellular consequences of polyQ protein aggregation. Our strategy provides a broadly applicable methodology for studying polyQ diseases.

Published

2020

21. Tick-Borne Encephalitis Virus Vaccines Contain Non-Structural Protein 1 Antigen and may Elicit NS1-Specific Antibody Responses in Vaccinated Individuals

Author

Jiri Salat, Kamil Mikulasek, Osmany Larralde, Petra Pokorna Formanova, Ales Chrdle, Jan Haviernik, Jana Elsterova, Dana Teislerova, Martin Palus, Ludek Eyer, Zbynek Zdrahal, Juraj Petrik, and Daniel Ruzek

Subjects

tick-borne encephalitis, vaccination, ns1, vaccine, flavivirus, Medicine

Abstract

Vaccination against tick-borne encephalitis (TBE) is based on the use of formalin-inactivated, culture-derived whole-virus vaccines. Immune response following vaccination is primarily directed to the viral envelope (E) protein, the major viral surface antigen. In Europe, two TBE vaccines are available in adult and pediatric formulations, namely FSME-IMMUN® (Pfizer) and Encepur® (GlaxoSmithKline). Herein, we analyzed the content of these vaccines using mass spectrometry (MS). The MS analysis revealed that the Encepur vaccine contains not only proteins of the whole virus particle, but also viral non-structural protein 1 (NS1). MS analysis of the FSME-IMMUN vaccine failed due to the high content of human serum albumin used as a stabilizer in the vaccine. However, the presence of NS1 in FSME-IMMUN was confirmed by immunization of mice with six doses of this vaccine, which led to a robust anti-NS1 antibody response. NS1-specific Western blot analysis also detected anti-NS1 antibodies in sera of humans who received multiple doses of either of these two vaccines; however, most vaccinees who received ≤3 doses were negative for NS1-specific antibodies. The contribution of NS1-specific antibodies to protection against TBE was demonstrated by immunization of mice with purified NS1 antigen, which led to a significant (p < 0.01) prolongation of the mean survival time after lethal virus challenge. This indicates that stimulation of anti-NS1 immunity by the TBE vaccines may increase their protective effect.

Published

2020