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Dive into the research topics where Hana Kotasová is active.

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Featured researches published by Hana Kotasová.


Free Radical Research | 2011

ABC transporters affect the detection of intracellular oxidants by fluorescent probes

Jiřina Procházková; Lukáš Kubala; Hana Kotasová; Iva Gudernova; Zuzana Šrámková; Michaela Pekarova; Balázs Sarkadi; Jiří Pacherník

Abstract Intracellular production of reactive oxygen species (ROS) plays an important role in the control of cell physiology. For the assessment of intracellular ROS production, a plethora of fluorescent probes is commonly used. Interestingly, chemical structures of these probes imply they could be substrates of plasma membrane efflux pumps, called ABC transporters. This study tested whether the determination of intracellular ROS production and mitochondrial membrane potential by selected fluorescent probes is modulated by the expression and activity of ABC transporters. The sub-clones of the HL-60 cell line over-expressing MDR1, MRP1 and BCRP transporters were employed. ROS production measured by luminol- and L-012-enhaced chemiluminescence and cytochrome c reduction assay showed similar levels of ROS production in all the employed cell lines. It was proved that dihydrorhodamine 123, dihexiloxocarbocyanine iodide, hydroethidine, tetrachloro-tetraethylbenzimidazolocarbo-cyanine iodide and tetramethylrhodamine ethyl ester perchlorate are substrates for MDR1; dichlorodihydrofluoresceine, hydroethidine and tetramethylrhodamine ethyl ester perchlorate are substrates for MRP1; dichlorodihydrofluoresceine, dihydrorhodamine 123, hydroethidine and tetrachloro-tetraethylbenzimidazolocarbo-cyanine iodide are substrates for BCRP. Thus, the determination of intracellular ROS and mitochondrial potential by the selected probes is significantly altered by ABC transporter activities. The activity of these transporters must be considered when employing fluorescent probes for the assessment of ROS production or mitochondrial membrane potential.


Journal of Cellular Biochemistry | 2012

Phosphoinositide 3‐kinase inhibition enables retinoic acid‐induced neurogenesis in monolayer culture of embryonic stem cells

Hana Kotasová; Iva Vesela; Jan Kučera; Zbyněk Houdek; Jiřina Procházková; Milena Kralickova; Jiří Pacherník

Retinoic acid (RA) is able to induce the differentiation of embryonic stem cells into neuronal lineages. The mechanism of this effect is unknown but it has been evidenced to be dependent on the formation of floating spheroids called embryoid bodies. Results presented here show that the inhibition of phosphoinositide 3‐kinase signaling pre‐determines mouse embryonic stem cells to RA induced neurogenesis in monolayer culture with no need of embryoid bodies formation. J. Cell. Biochem. 113: 563–570, 2012.


Cellular and Molecular Neurobiology | 2014

Interaction of Notch and gp130 Signaling in the Maintenance of Neural Stem and Progenitor Cells

Hana Kotasová; Jiřina Procházková; Jiří Pacherník

Notch and gp130 signaling are involved in the regulation of multiple cellular processes across various tissues during animal ontogenesis. In the developing nervous system, both signaling pathways intervene at many stages to determine cell fate—from the first neural lineage commitment and generation of neuronal precursors, to the terminal specification of cells as neurons and glia. In most cases, the effects of Notch and gp130 signaling in these processes are similar. The aim of the current review was to summarize the knowledge regarding the roles of Notch and gp130 signaling in the maintenance of neural stem and progenitor cells during animal ontogenesis, from early embryo to adult. Recent data show a direct crosstalk between these signaling pathways that seems to be specific for a particular type of neural progenitors.


PLOS ONE | 2017

The acceleration of cardiomyogenesis in embryonic stem cells in vitro by serum depletion does not increase the number of developed cardiomyocytes

Katarzyna Anna Radaszkiewicz; Dominika Sýkorová; Lucia Binó; Jana Kudová; Markéta Bébarová; Jiřina Procházková; Hana Kotasová; Lukáš Kubala; Jiří Pacherník

The differentiation of pluripotent embryonic stem (ES) cells into various lineages in vitro represents an important tool for studying the mechanisms underlying mammalian embryogenesis. It is a key technique in studies evaluating the molecular mechanisms of cardiomyogenesis and heart development and also in embryotoxicology. Herein, modest modifications of the basic protocol for ES cell differentiation into cardiomyocytes were evaluated in order to increase the yield and differentiation status of developed cardiomyocytes. Primarily, the data show that ES cell cultivation in the form of non-adherent embryoid bodies (EBs) for 5 days compared to 8 days significantly improved cardiomyogenic differentiation. This is illustrated by the appearance of beating foci in the adherent EBs layer at earlier phases of differentiation from day 10 up to day 16 and by the significantly higher expression of genes characteristic of cardiomyogenic differentiation (sarcomeric alpha actinin, myosin heavy chain alpha and beta, myosin light chain 2 and 7, and transcriptional factor Nkx2.5) in EBs cultivated under non-adherent conditions for 5 days. The ratio of cardiomyocytes per other cells was also potentiated in EBs cultivated in non-adherent conditions for only 5 days followed by cultivation in adherent serum-free culture conditions. Nevertheless, the alteration in the percentage of beating foci among these two tested cultivation conditions vanished at later phases and also did not affect the total number of cardiomyocytes determined as myosin heavy chain positive cells at the end of the differentiation process on day 20. Thus, although these modifications of the conditions of ES cells differentiation may intensify cardiomyocyte differentiation, the final count of cardiomyocytes might not change. Thus, serum depletion was identified as a key factor that intensified cardiomyogenesis. Further, the treatment of EBs with N-acetylcysteine, a reactive oxygen species scavenger, did not affect the observed increase in cardiomyogenesis under serum depleted conditions. Interestingly, a mild induction of the ventricular-like phenotype of cardiomyocytes was observed in 5-day-old EBs compared to 8-day-old EBs. Overall, these findings bring crucial information on the mechanisms of ES cells differentiation into cardiomyocytes and on the establishment of efficient protocols for the cardiomyogenic differentiation of ES cells. Further, the importance of determining the absolute number of formed cardiomyocyte-like cells per seeded pluripotent cells in contrast to the simple quantification of the ratios of cells is highlighted.


Folia Biologica | 2008

Densities and Morphology of Two Co-existing Lizard Species (Lacerta agilis and Zootoca vivipara) in Extensively Used Farmland in Poland*

Iva Veselá; Hana Kotasová; Štěpánka Jankovská; Jiřina Procházková; Jiří Pacherník


Archive | 2012

The role of hypoxia in expression of MDR-associated ABCtransporters in embryonic stem cells

Martina Kohutková Lánová; Jan Kučera; Hana Kotasová; Jiřina Medalová; Jiří Pacherník


Archive | 2012

Úloha hypoxie v regulaci exprese ABC-transportérů asociovaných s MDR u (embryonálních) kmenových buněk

Martina Kohutková Lánová; Jan Kučera; Hana Kotasová; Jiřina Medalová; Jiří Pacherník


Archive | 2011

Localization of the STAT3 binding site in the MDR1 enhanceosom

Zuzana Šrámková; Jiřina Procházková; Hana Kotasová; Kateřina Tmejová; Iva Gudernova; Jiří Pacherník


Archive | 2011

Commonly used ROS-sensitive fluorescent probes are substrates of ABC transporters

Jiřina Medalová; Lukáš Kubala; Hana Kotasová; Iva Gudernova; Zuzana Šrámková; Michaela Pekarova; Balázs Sarkadi; Jiří Pacherník


Archive | 2010

ABC transporters in mES cells - possible role of p38 MAPK

Jiřina Procházková; Hana Kotasová; Kateřina Štefková; Martina Kohutková Lánová; Jiří Pacherník

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Jiřina Procházková

Academy of Sciences of the Czech Republic

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Lukáš Kubala

Academy of Sciences of the Czech Republic

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Iva Vesela

University of Veterinary and Pharmaceutical Sciences Brno

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Michaela Pekarova

Academy of Sciences of the Czech Republic

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