Your search keyword '"Götze S"' showing total 5 results

1. Combined Methylome and Transcriptome Analysis During Rat Hepatic Stellate Cell Activation.

Author

Schumacher EC, Götze S, Kordes C, Benes V, and Häussinger D

Subjects

Animals, Cell Differentiation genetics, Epigenesis, Genetic genetics, Gene Expression genetics, Gene Expression Profiling methods, Mesenchymal Stem Cells physiology, Promoter Regions, Genetic genetics, Rats, Rats, Wistar, DNA Methylation genetics, Hepatic Stellate Cells physiology, Liver physiology, Transcriptome genetics

Abstract

Hepatic stellate cells (HSCs) are mesenchymal stem cells (MSCs) of the liver. They are unique among MSCs, since HSCs remain in a quiescent, retinoid-storing state in the normal liver but become activated after liver injury and contribute to tissue repair. The epigenetic mechanisms accompanying the transition of HSCs from a quiescent to an activated state are in the focus of the present study. We investigated the methylome and transcriptome during this process and observed profound changes. While the promoter methylation correlated negatively with gene expression, the gene-body methylation revealed no clear correlation. Most genes with altered expression were associated with cell differentiation. Among them, Wilms tumor 1 (Wt1) and Deltex4 (Dtx4) genes were identified as epigenetically regulated. Since HSCs were reported to derive from multipotent Wt1-positive cells and many differentially expressed genes were associated with cell differentiation during their activation, epigenetic alterations are presumably required to enable HSC development.

Published

2017

2. The Role of Embryonic Stem Cell-expressed RAS (ERAS) in the Maintenance of Quiescent Hepatic Stellate Cells.

Author

Nakhaei-Rad S, Nakhaeizadeh H, Götze S, Kordes C, Sawitza I, Hoffmann MJ, Franke M, Schulz WA, Scheller J, Piekorz RP, Häussinger D, and Ahmadian MR

Subjects

Animals, Apoptosis Regulatory Proteins genetics, Apoptosis Regulatory Proteins metabolism, Forkhead Transcription Factors genetics, Forkhead Transcription Factors metabolism, Hepatic Stellate Cells cytology, Male, Mechanistic Target of Rapamycin Complex 2, Multiprotein Complexes genetics, Multiprotein Complexes metabolism, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Oncogene Protein p21(ras) genetics, Proto-Oncogene Proteins c-akt genetics, Proto-Oncogene Proteins c-akt metabolism, Rats, Rats, Wistar, TOR Serine-Threonine Kinases genetics, TOR Serine-Threonine Kinases metabolism, YAP-Signaling Proteins, DNA Methylation physiology, Hepatic Stellate Cells enzymology, MAP Kinase Signaling System physiology, Oncogene Protein p21(ras) biosynthesis, Promoter Regions, Genetic physiology

Abstract

Hepatic stellate cells (HSCs) were recently identified as liver-resident mesenchymal stem cells. HSCs are activated after liver injury and involved in pivotal processes, such as liver development, immunoregulation, regeneration, and also fibrogenesis. To date, several studies have reported candidate pathways that regulate the plasticity of HSCs during physiological and pathophysiological processes. Here we analyzed the expression changes and activity of the RAS family GTPases and thereby investigated the signaling networks of quiescent HSCs versus activated HSCs. For the first time, we report that embryonic stem cell-expressed RAS (ERAS) is specifically expressed in quiescent HSCs and down-regulated during HSC activation via promoter DNA methylation. Notably, in quiescent HSCs, the high level of ERAS protein correlates with the activation of AKT, STAT3, mTORC2, and HIPPO signaling pathways and inactivation of FOXO1 and YAP. Our data strongly indicate that in quiescent HSCs, ERAS targets AKT via two distinct pathways driven by PI3Kα/δ and mTORC2, whereas in activated HSCs, RAS signaling shifts to RAF-MEK-ERK. Thus, in contrast to the reported role of ERAS in tumor cells associated with cell proliferation, our findings indicate that ERAS is important to maintain quiescence in HSCs., (© 2016 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2016

3. Epigenetic Changes during Hepatic Stellate Cell Activation.

Author

Götze S, Schumacher EC, Kordes C, and Häussinger D

Subjects

Animals, Cells, Cultured, DNA Methylation drug effects, Dideoxynucleosides pharmacology, Epigenesis, Genetic drug effects, Genome-Wide Association Study, Hepatic Stellate Cells cytology, Liver cytology, Male, Mesenchymal Stem Cells cytology, Mimosine pharmacology, Rats, Rats, Wistar, DNA Methylation physiology, Epigenesis, Genetic physiology, Hepatic Stellate Cells metabolism, Liver metabolism, Mesenchymal Stem Cells metabolism

Abstract

Background and Aims: Hepatic stellate cells (HSC), which can participate in liver regeneration and fibrogenesis, have recently been identified as liver-resident mesenchymal stem cells. During their activation HSC adopt a myofibroblast-like phenotype accompanied by profound changes in the gene expression profile. DNA methylation changes at single genes have been reported during HSC activation and may participate in the regulation of this process, but comprehensive DNA methylation analyses are still missing. The aim of the present study was to elucidate the role of DNA methylation during in vitro activation of HSC., Methods and Results: The analysis of DNA methylation changes by antibody-based assays revealed a strong decrease in the global DNA methylation level during culture-induced activation of HSC. To identify genes which may be regulated by DNA methylation, we performed a genome-wide Methyl-MiniSeq EpiQuest sequencing comparing quiescent and early culture-activated HSC. Approximately 400 differentially methylated regions with a methylation change of at least 20% were identified, showing either hypo- or hypermethylation during activation. Further analysis of selected genes for DNA methylation and expression were performed revealing a good correlation between DNA methylation changes and gene expression. Furthermore, global DNA demethylation during HSC activation was investigated by 5-bromo-2-deoxyuridine assay and L-mimosine treatment showing that demethylation was independent of DNA synthesis and thereby excluding a passive DNA demethylation mechanism., Conclusions: In summary, in vitro activation of HSC initiated strong DNA methylation changes, which were associated with gene regulation. These results indicate that epigenetic mechanisms are important for the control of early HSC activation. Furthermore, the data show that global DNA demethylation during activation is based on an active DNA demethylation mechanism.

Published

2015

4. Frequent promoter hypermethylation of Wnt pathway inhibitor genes in malignant astrocytic gliomas.

Author

Götze S, Wolter M, Reifenberger G, Müller O, and Sievers S

Subjects

Adaptor Proteins, Signal Transducing, Calcium-Binding Proteins, Carrier Proteins genetics, Cell Line, Tumor, DNA Mutational Analysis, DNA, Neoplasm genetics, DNA, Neoplasm isolation & purification, Exons, Eye Proteins genetics, Glioblastoma genetics, Glioblastoma secondary, Glioma genetics, Glioma pathology, Humans, Intercellular Signaling Peptides and Proteins genetics, Membrane Proteins genetics, Mutation, Polymerase Chain Reaction, Proto-Oncogene Proteins genetics, beta Catenin genetics, Astrocytoma genetics, DNA Methylation genetics, Promoter Regions, Genetic, Wnt Proteins genetics

Abstract

Aberrant activation of wingless (Wnt) signaling is involved in the pathogenesis of various cancers. Recent studies suggested a role of Wnt signaling in gliomas, the most common primary brain tumors. We investigated 70 gliomas of different malignancy grades for promoter hypermethylation in 8 genes encoding members of the secreted frizzled-related protein (SFRP1, SFRP2, SFRP4, SFRP5), dickkopf (DKK1, DKK3) and naked (NKD1, NKD2) families of Wnt pathway inhibitors. All tumors were additionally analyzed for mutations in exon 3 of the beta-catenin gene (CTNNB1). While none of the tumors carried CTNNB1 mutations, we found frequent promoter hypermethylation of Wnt pathway inhibitor genes, with at least one of these genes being hypermethylated in 6 of 16 diffuse astrocytomas (38%), 4 of 14 anaplastic astrocytomas (29%), 7 of 10 secondary glioblastomas (70%) and 23 of 30 primary glioblastomas (77%). Glioblastomas often demonstrated hypermethylation of 2 or more analyzed genes. Hypermethylation of SFRP1, SFRP2 and NKD2 each occurred in more than 40% of the primary glioblastomas, while DKK1 hypermethylation was found in 50% of secondary glioblastomas. Treatment of SFRP1-, SFRP5-, DKK1-, DKK3-, NKD1- and NKD2-hypermethylated U87-MG glioblastoma cells with 5-aza-2'-deoxycytidine and trichostatin A resulted in increased expression of each gene. Furthermore, SFRP1-hypermethylated gliomas showed significantly lower expression of the respective transcripts when compared with unmethylated tumors. Taken together, our results suggest an important role of epigenetic silencing of Wnt pathway inhibitor genes in astrocytic gliomas, in particular, in glioblastomas, with distinct patterns of hypermethylated genes distinguishing primary from secondary glioblastomas.

Published

2010

5. ECRG4 is a candidate tumor suppressor gene frequently hypermethylated in colorectal carcinoma and glioma.

Author

Götze S, Feldhaus V, Traska T, Wolter M, Reifenberger G, Tannapfel A, Kuhnen C, Martin D, Müller O, and Sievers S

Subjects

Cell Line, Tumor, Cell Proliferation, Colorectal Neoplasms pathology, Gene Expression Regulation, Neoplastic, Humans, Promoter Regions, Genetic, Tumor Suppressor Proteins, Colorectal Neoplasms genetics, Colorectal Neoplasms metabolism, DNA Methylation, Genes, Tumor Suppressor, Glioma genetics, Glioma metabolism, Neoplasm Proteins genetics

Abstract

Background: Cancer cells display widespread changes in DNA methylation that may lead to genetic instability by global hypomethylation and aberrant silencing of tumor suppressor genes by focal hypermethylation. In turn, altered DNA methylation patterns have been used to identify putative tumor suppressor genes., Methods: In a methylation screening approach, we identified ECRG4 as a differentially methylated gene. We analyzed different cancer cells for ECRG4 promoter methylation by COBRA and bisulfite sequencing. Gene expression analysis was carried out by semi-quantitative RT-PCR. The ECRG4 coding region was cloned and transfected into colorectal carcinoma cells. Cell growth was assessed by MTT and BrdU assays. ECRG4 localization was analyzed by fluorescence microscopy and Western blotting after transfection of an ECRG4-eGFP fusion gene., Results: We found a high frequency of ECRG4 promoter methylation in various cancer cell lines. Remarkably, aberrant methylation of ECRG4 was also found in primary human tumor tissues, including samples from colorectal carcinoma and from malignant gliomas. ECRG4 hypermethylation associated strongly with transcriptional silencing and its expression could be re-activated in vitro by demethylating treatment with 5-aza-2'-deoxycytidine. Overexpression of ECRG4 in colorectal carcinoma cells led to a significant decrease in cell growth. In transfected cells, ECRG4 protein was detectable within the Golgi secretion machinery as well as in the culture medium., Conclusions: ECRG4 is silenced via promoter hypermethylation in different types of human cancer cells. Its gene product may act as inhibitor of cell proliferation in colorectal carcinoma cells and may play a role as extracellular signaling molecule.

Published

2009