Your search keyword '"Katerina Galuskova"' showing total 8 results

1. Supplementary Figures S1-3, Tables S1-3 from HIC1 Tumor Suppressor Loss Potentiates TLR2/NF-κB Signaling and Promotes Tissue Damage–Associated Tumorigenesis

Author

Vladimir Korinek, Hynek Strnad, Katerina Galuskova, Eva Sloncova, Jitka Stancikova, Adela Hlavata, Monika Horazna, Nikol Baloghova, Dominique Leprince, Marion Dubuissez, Jan Dobes, Jolana Tureckova, Martina Vojtechova, Bohumil Fafilek, Vendula Pospichalova, and Lucie Janeckova

Abstract

Supplementary Figures S1-3, Tables S1-3. Supplementary Figure S1. Heatmaps depicting gene expression in Hic1flox/flox MEFs treated with 4- OHT when compared to MEFs treated with vehicle (ethanol) only. Genes (299 in total) displaying significantly (q < 0.05) changed expression in at least one of the indicated time points are listed. The position of Hic1 and six genes whose expression was changed more than twice (|log FC| > 1) in at least two time points is highlighted. Supplementary Figure S2. Loss of Hic1 results in increased counts of goblet and enteroendocrine cells. A,B, goblet (A) and enteroendocrine (B) cell distribution in the indicated segments of the small intestine. Specimens obtained from four Hic1flox/flox and four Hic1flox/flox Villin-Cre+ mice were stained using Periodic acid Schiff (PAS) and an anti-chromogranin A antibody to visualize goblet and enteroendocrine cells, respectively. Stained cells (indicated by black arrowheads in the histology images on the right) were in several different fields indicated by numbers on the X axis. C, no changes in enterocytes were noted in the Hic1-deficient small intestine. Left, qRT-PCR analysis of enterocytespecific markers hairy and enhancer of split-1 (Hes1) and sucrase-isomaltase (SI). The expression level of the respective gene in wt mice (upon normalization to Ubb) was arbitrarily set to 1. Right, staining of brush border enzyme alkaline phosphatase (AP) produced by differentiated enterocytes in the small intestine. Scale bar: 0.15 mm; error bars: SDs. Supplementary Figure S3. DSS-induced transcriptional response in the colon of Hic1flox/flox and Hic1flox/flox Villin-Cre+ mice six and nine days after DSS withdrawal. Epithelial lining of the colon obtained from four animals of each genotype was analyzed using qRT-PCR. The results were normalized to the Ubiquitin B (Ubb) housekeeping gene; the relative expression of another housekeeping gene, β-actin, is also shown. The expression level of the corresponding gene in mice without DSS treatment was arbitrarily set to 1. Error bars: SDs. Supplementary Table S1 Primers used for qRT-PCR analysis Supplementary Table S2. List of genes differentially expressed in Hic1flox/flox MEFs treated with 4- OHT for 48, 72, and 120 hours when compared to control MEFs treated (for the given time periods) with vehicle. Selection criterion: q < 0.05. Of note, none of the genes passed the selection criterion for the 24-hour time point. Supplementary Table S3. The most different 'Gene Ontology Biological Processes' (GO BPs) and WikiPathways categories in expression profiles of Hic1flox/flox MEFs 72 hours after addition of 4-OHT when compared to MEFs treated with vehicle only. In total, 268 gene probes passed the significance criterion (q-value < 0.05). Corresponding annotated genes (listed in Supplementary Table S2) were analyzed using the GO BP and WikiPathways 2015 Enricher datasets. The results were sorted according to the p-value; GO BPs and WikiPathways with p < 0.05 are listed.

Published

2023

2. Data from HIC1 Tumor Suppressor Loss Potentiates TLR2/NF-κB Signaling and Promotes Tissue Damage–Associated Tumorigenesis

Author

Vladimir Korinek, Hynek Strnad, Katerina Galuskova, Eva Sloncova, Jitka Stancikova, Adela Hlavata, Monika Horazna, Nikol Baloghova, Dominique Leprince, Marion Dubuissez, Jan Dobes, Jolana Tureckova, Martina Vojtechova, Bohumil Fafilek, Vendula Pospichalova, and Lucie Janeckova

Abstract

Hypermethylated in cancer 1 (HIC1) represents a prototypic tumor suppressor gene frequently inactivated by DNA methylation in many types of solid tumors. The gene encodes a sequence-specific transcriptional repressor controlling expression of several genes involved in cell cycle or stress control. In this study, a Hic1 allele was conditionally deleted, using a Cre/loxP system, to identify genes influenced by the loss of Hic1. One of the transcripts upregulated upon Hic1 ablation is the toll-like receptor 2 (TLR2). Tlr2 expression levels increased in Hic1-deficient mouse embryonic fibroblasts (MEF) and cultured intestinal organoids or in human cells upon HIC1 knockdown. In addition, HIC1 associated with the TLR2 gene regulatory elements, as detected by chromatin immunoprecipitation, indicating that Tlr2 indeed represents a direct Hic1 target. The Tlr2 receptor senses “danger” signals of microbial or endogenous origin to trigger multiple signaling pathways, including NF-κB signaling. Interestingly, Hic1 deficiency promoted NF-κB pathway activity not only in cells stimulated with Tlr2 ligand, but also in cells treated with NF-κB activators that stimulate different surface receptors. In the intestine, Hic1 is mainly expressed in differentiated epithelial cells and its ablation leads to increased Tlr2 production. Finally, in a chemical-induced mouse model of carcinogenesis, Hic1 absence resulted in larger Tlr2-positive colonic tumors that showed increased proportion of proliferating cells.Implications: The tumor-suppressive function of Hic1 in colon is related to its inhibitory action on proproliferative signaling mediated by the Tlr2 receptor present on tumor cells. Mol Cancer Res; 13(7); 1139–48. ©2015 AACR.

Published

2023

3. Astrocyte-like subpopulation of NG2 glia in the adult mouse cortex exhibits characteristics of neural progenitor cells and is capable of forming neuron-like cells after ischemic injury

Author

Lucie Janeckova, Tomas Knotek, Jan Kriska, Zuzana Hermanova, Denisa Kirdajova, Jan Kubovciak, Linda Berkova, Jana Tureckova, Sara Camacho Garcia, Katerina Galuskova, Michal Kolar, Miroslava Anderova, and Vladimir Korinek

Abstract

Glia cells expressing neuron-glial antigen 2 (NG2) play a critical role as oligodendrocyte precursor cells (OPCs) in the healthy brain; however, their differentiation potential after ischemic injury remains an unresolved question. Here, we aimed to elucidate the heterogeneity and role of NG2 glia in the ischemic brain. We used transgenic mice to label NG2-expressing cells and their progeny with red fluorescent protein tdTomato in the healthy brains and those after focal cerebral ischemia (FCI). Based on single-cell RNA sequencing, the labeled glial cells were divided into five distinct subpopulations. The identity of these subpopulations was determined based on gene expression patterns. In addition, membrane properties were further analyzed using the patch-clamp technique. Three of the observed subpopulations represented OPCs, whereas the fourth group exhibited characteristics of cells destined for oligodendrocyte fate. The fifth subpopulation of NG2 glia carried astrocytic markers. Importantly, we detected features of neural progenitors in these cells. This subpopulation was present in both healthy and post-ischemic tissue; however, its gene expression changed after ischemia, with genes related to neurogenesis being more abundant. Neurogenic gene expression was monitored over time and complemented by immunohistochemical staining, which showed increased numbers of Purkinje cell protein 4-positive NG2 cells at the edge of the ischemic lesion 12 days after FCI, and NeuN-positive NG2 cells 28 days after injury, indicating the existence of neuron-like cells that develop from NG2 glia in the ischemic tissue. Our results provide further insight into the differentiation plasticity and neurogenic potential of NG2 glia after stroke.Main PointsDifferent subpopulations of NG2 glia in the healthy and ischemic adult cortex were identified based on their gene expression and membrane properties.Astrocyte-like NG2 glia exhibit neurogenic gene expression and are more abundant in post-ischemic tissue.Progeny of NG2-positive cells carrying neuronal marker NeuN was observed at the edge of the ischemic lesion.

Published

2023

4. <scp>W</scp> nt Signaling Inhibition Deprives Small Intestinal Stem Cells of Clonogenic Capacity

Author

Vladimir Korinek, Meritxell Alberich-Jorda, Michaela Krausova, Radislav Sedlacek, Monika Horazna, Miroslava Anderova, Bohumil Fafilek, Katerina Galuskova, Martina Vojtechova, Eva Sloncova, and Lucie Janeckova

Subjects

0301 basic medicine, Beta-catenin, Transcription, Genetic, Cellular differentiation, Wnt pathway, Mice, Transgenic, Biology, digestive system, gene targeting, Mice, 03 medical and health sciences, Transcription Factor 4, Endocrinology, Intestinal mucosa, Cre/loxP, Intestine, Small, Genetics, Animals, Intestinal Mucosa, Wnt Signaling Pathway, Research Articles, beta Catenin, TCF/LEF transcription factors, Cell Proliferation, Basic Helix-Loop-Helix Leucine Zipper Transcription Factors, Stem Cells, Wnt signaling pathway, LRP6, Cell Differentiation, LRP5, Cell Biology, Molecular biology, Intestinal epithelium, 030104 developmental biology, biology.protein, β‐catenin, gut, Stem cell, Cell Division, Research Article

Abstract

Summary The Wnt pathway plays a crucial role in self‐renewal and differentiation of cells in the adult gut. In the present study, we revealed the functional consequences of inhibition of canonical Wnt signaling in the intestinal epithelium. The study was based on generation of a novel transgenic mouse strain enabling inducible expression of an N‐terminally truncated variant of nuclear Wnt effector T cell factor 4 (TCF4). The TCF4 variant acting as a dominant negative (dn) version of wild‐type (wt) TCF4 protein decreased transcription of β‐catenin‐TCF4‐responsive genes. Interestingly, suppression of Wnt/β‐catenin signaling affected asymmetric division of intestinal stem cells (ISCs) rather than proliferation. ISCs expressing the transgene underwent several rounds of division but lost their clonogenic potential and migrated out of the crypt. Expression profiling of crypt cells revealed that besides ISC‐specific markers, the dnTCF4 production downregulated expression levels of epithelial genes produced in other crypt cells including markers of Paneth cells. Additionally, in Apc conditional knockout mice, dnTCF activation efficiently suppressed growth of Apc‐deficient tumors. In summary, the generated mouse strain represents a convenient tool to study cell‐autonomous inhibition of β‐catenin‐Tcf‐mediated transcription. genesis 54:101–114, 2016. © 2016 The Authors genesis Published by Wiley Periodicals, Inc.

Published

2016

5. Unique Gene Expression Signatures in the Intestinal Mucosa and Organoids Derived from Germ-Free and Monoassociated Mice

Author

Monika Stastna, Klara Kostovcikova, Nikol Baloghova, Hynek Strnad, Jolana Tureckova, Lucie Janeckova, Helena Tlaskalova-Hogenova, Katerina Galuskova, Jiri Svec, Michal Kolar, Eva Sloncova, Jitka Stancikova, Vladimir Korinek, and Tomas Hudcovic

Subjects

Colon, Adipose tissue, Biology, Catalysis, Article, Inorganic Chemistry, lcsh:Chemistry, Intestinal mucosa, ANGPTL4, Gene expression, Organoid, medicine, Escherichia coli, Animals, Germ-Free Life, Physical and Theoretical Chemistry, Intestinal Mucosa, Onecut2, Molecular Biology, lcsh:QH301-705.5, Immunity, Mucosal, Spectroscopy, Enricher tool, Mice, Inbred BALB C, Gene Expression Profiling, Microbiota, Organic Chemistry, Lipid metabolism, General Medicine, Molecular biology, Small intestine, Computer Science Applications, Gene expression profiling, Organoids, medicine.anatomical_structure, lcsh:Biology (General), lcsh:QD1-999, Gene Expression Regulation, expression profiling, Immune System, monoassociation, Biomarkers

Abstract

Commensal microbiota contribute to gut homeostasis by inducing transcription of mucosal genes. Analysis of the impact of various microbiota on intestinal tissue provides an important insight into the function of this organ. We used cDNA microarrays to determine the gene expression signature of mucosa isolated from the small intestine and colon of germ-free (GF) mice and animals monoassociated with two E. coli strains. The results were compared to the expression data obtained in conventionally reared (CR) mice. In addition, we analyzed gene expression in colon organoids derived from CR, GF, and monoassociated animals. The analysis revealed that the complete absence of intestinal microbiota mainly affected the mucosal immune system, which was not restored upon monoassociation. The most important expression changes observed in the colon mucosa indicated alterations in adipose tissue and lipid metabolism. In the comparison of differentially expressed genes in the mucosa or organoids obtained from GF and CR mice, only six genes were common for both types of samples. The results show that the increased expression of the angiopoietin-like 4 (Angptl4) gene encoding a secreted regulator of lipid metabolism indicates the GF status.

Published

2019

6. Wnt Effector TCF4 Is Dispensable for Wnt Signaling in Human Cancer Cells

Author

Eva Sloncova, Vladimir Korinek, Lucie Janeckova, Vitezslav Kriz, Katerina Galuskova, Dusan Hrckulak, Martina Vojtechova, Lucie Lanikova, Monika Horazna, and Olga Babosova

Subjects

0301 basic medicine, lcsh:QH426-470, colorectal cancer, Tumor initiation, Biology, medicine.disease_cause, Article, 03 medical and health sciences, Coactivator, Genetics, medicine, Transcription factor, Genetics (clinical), organoids, conditional gene inactivation, Wnt signaling pathway, TCF4, Intestinal epithelium, Wnt signaling, 3. Good health, Cell biology, TCF7L2, lcsh:Genetics, tumorigenesis, 030104 developmental biology, gut, Carcinogenesis, epithelium

Abstract

T-cell factor 4 (TCF4), together with &beta, catenin coactivator, functions as the major transcriptional mediator of the canonical wingless/integrated (Wnt) signaling pathway in the intestinal epithelium. The pathway activity is essential for both intestinal homeostasis and tumorigenesis. To date, several mouse models and cellular systems have been used to analyze TCF4 function. However, some findings were conflicting, especially those that were related to the defects observed in the mouse gastrointestinal tract after Tcf4 gene deletion, or to a potential tumor suppressive role of the gene in intestinal cancer cells or tumors. Here, we present the results obtained using a newly generated conditional Tcf4 allele that allows inactivation of all potential Tcf4 isoforms in the mouse tissue or small intestinal and colon organoids. We also employed the clustered regularly interspaced short palindromic repeats (CRISPR)/Cas9 system to disrupt the TCF4 gene in human cells. We showed that in adult mice, epithelial expression of Tcf4 is indispensable for cell proliferation and tumor initiation. However, in human cells, the TCF4 role is redundant with the related T-cell factor 1 (TCF1) and lymphoid enhancer-binding factor 1 (LEF1) transcription factors.

Published

2018

7. HIC1 Tumor Suppressor Loss Potentiates TLR2/NF-κB Signaling and Promotes Tissue Damage–Associated Tumorigenesis

Author

Martina Vojtechova, Marion Dubuissez, Bohumil Fafilek, Nikol Baloghova, Jitka Stancikova, Lucie Janeckova, Dominique Leprince, Adela Hlavata, Jolana Tureckova, Vladimir Korinek, Vendula Pospichalova, Eva Sloncova, Hynek Strnad, Jan Dobeš, Katerina Galuskova, and Monika Horazna

Subjects

Cancer Research, Tumor suppressor gene, Carcinogenesis, Azoxymethane, Kruppel-Like Transcription Factors, Mice, Transgenic, Biology, medicine.disease_cause, Mice, Cell Line, Tumor, medicine, Animals, Humans, Receptor, Molecular Biology, Cell Proliferation, Gene knockdown, Tumor Suppressor Proteins, Dextran Sulfate, NF-kappa B, Epithelial Cells, Toll-Like Receptor 2, Up-Regulation, Intestines, Disease Models, Animal, TLR2, Oncology, Gene Knockdown Techniques, Colonic Neoplasms, DNA methylation, Cancer research, Signal transduction, Chromatin immunoprecipitation, Signal Transduction

Abstract

Hypermethylated in cancer 1 (HIC1) represents a prototypic tumor suppressor gene frequently inactivated by DNA methylation in many types of solid tumors. The gene encodes a sequence-specific transcriptional repressor controlling expression of several genes involved in cell cycle or stress control. In this study, a Hic1 allele was conditionally deleted, using a Cre/loxP system, to identify genes influenced by the loss of Hic1. One of the transcripts upregulated upon Hic1 ablation is the toll-like receptor 2 (TLR2). Tlr2 expression levels increased in Hic1-deficient mouse embryonic fibroblasts (MEF) and cultured intestinal organoids or in human cells upon HIC1 knockdown. In addition, HIC1 associated with the TLR2 gene regulatory elements, as detected by chromatin immunoprecipitation, indicating that Tlr2 indeed represents a direct Hic1 target. The Tlr2 receptor senses “danger” signals of microbial or endogenous origin to trigger multiple signaling pathways, including NF-κB signaling. Interestingly, Hic1 deficiency promoted NF-κB pathway activity not only in cells stimulated with Tlr2 ligand, but also in cells treated with NF-κB activators that stimulate different surface receptors. In the intestine, Hic1 is mainly expressed in differentiated epithelial cells and its ablation leads to increased Tlr2 production. Finally, in a chemical-induced mouse model of carcinogenesis, Hic1 absence resulted in larger Tlr2-positive colonic tumors that showed increased proportion of proliferating cells. Implications: The tumor-suppressive function of Hic1 in colon is related to its inhibitory action on proproliferative signaling mediated by the Tlr2 receptor present on tumor cells. Mol Cancer Res; 13(7); 1139–48. ©2015 AACR.

Published

2015

8. Author Correction: Msx1 loss suppresses formation of the ectopic crypts developed in the Apc-deficient small intestinal epithelium

Author

Vladimir Korinek, Martina Vojtechova, Katerina Galuskova, Michal Kolar, Jiri Svec, Dusan Hrckulak, Lucie Janeckova, Eva Sloncova, Hynek Strnad, Monika Horazna, and Olga Babosova

Subjects

Pathology, medicine.medical_specialty, Multidisciplinary, Small intestinal epithelium, lcsh:R, medicine, lcsh:Medicine, lcsh:Q, Biology, lcsh:Science

Abstract

An amendment to this paper has been published and can be accessed via a link at the top of the paper.

Published

2019