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8. Secreted microvesicular miR-31 inhibits osteogenic differentiation of mesenchymal stem cells

Author

Weilner, S, Schraml, E, Wieser, M, Messner, P, Schneider, K, Wassermann, K, Micutkova, L, Fortschegger, K, Maier, AB, Westendorp, R, Resch, H, Wolbank, S, Redl, H, Jansen-Durr, P, Pietschmann, P, Grillari-Voglauer, R, Grillari, J, Weilner, S, Schraml, E, Wieser, M, Messner, P, Schneider, K, Wassermann, K, Micutkova, L, Fortschegger, K, Maier, AB, Westendorp, R, Resch, H, Wolbank, S, Redl, H, Jansen-Durr, P, Pietschmann, P, Grillari-Voglauer, R, and Grillari, J

Abstract

Damage to cells and tissues is one of the driving forces of aging and age-related diseases. Various repair systems are in place to counteract this functional decline. In particular, the property of adult stem cells to self-renew and differentiate is essential for tissue homeostasis and regeneration. However, their functionality declines with age (Rando, 2006). One organ that is notably affected by the reduced differentiation capacity of stem cells with age is the skeleton. Here, we found that circulating microvesicles impact on the osteogenic differentiation capacity of mesenchymal stem cells in a donor-age-dependent way. While searching for factors mediating the inhibitory effect of elderly derived microvesicles on osteogenesis, we identified miR-31 as a crucial component. We demonstrated that miR-31 is present at elevated levels in the plasma of elderly and of osteoporosis patients. As a potential source of its secretion, we identified senescent endothelial cells, which are known to increase during aging in vivo (Erusalimsky, 2009). Endothelial miR-31 is secreted within senescent cell-derived microvesicles and taken up by mesenchymal stem cells where it inhibits osteogenic differentiation by knocking down its target Frizzled-3. Therefore, we suggest that microvesicular miR-31 in the plasma of elderly might play a role in the pathogenesis of age-related impaired bone formation and that miR-31 might be a valuable plasma-based biomarker for aging and for a systemic environment that does not favor cell-based therapies whenever osteogenesis is a limiting factor.

Published
2016

9. Existence of cardiac PNMT mRNA in adult rats: elevation by stress in a glucocorticoid-dependent manner

Author

KRIZANOVA, O., MICUTKOVA, L., JELOKOVA, J., FILIPENKO, M., SABBAN, E., and KVETNANSKY, R.

Subjects
Corticosteroids -- Physiological aspects, Adrenalectomy -- Physiological aspects, Epinephrine -- Physiological aspects, Noradrenaline -- Physiological aspects, Gene expression -- Research, Biological sciences
Abstract

Phenylethanolamine N-methyltransferase (PNMT) is the enzyme that synthesizes epinephrine from norepinephrine. The aim of this study was to determine potential PNMT gene expression in the cardiac atria and ventricles of adult rats and to examine whether the gene expression of this enzyme is affected by immobilization stress. PNMT mRNA levels were detected in all four parts of the heart, with the highest level in the left atrium. Both Southern blot and sequencing verified the specificity of PNMT detected by RT-PCR. Single immobilization for 2 h increased gene expression of PNMT in both atria and ventricles. In atria, this effect was clearly modulated by glucocorticoids, because either adrenalectomy or hypophysectomy prevented the increase in PNMT mRNA levels in response to immobilization stimulus. This study establishes, for the first time, that PNMT gene expression occurs in cardiac atria and also, to a small extent, in ventricles of adult rats. Immobilization stress increases gene expression in atria and ventricles. This increase requires an intact hypothalamus-pituitary-adrenocortical axis, indicating the involvement of glucocorticoids. effect of glucocorticoids; adrenalectomy; hypophysectomy; phenylethanolamine N-methyltransferase

Published
2001

10. Role of endonuclease G in senescence-associated cell death of human endothelial cells

Author

Micutkova, L., Neuhaus, M., Jansen-Dürr, P., Koziel, R., and Diener, T.

Subjects
HUVEC EndoG Senescence Apoptosis,Biological Sciences
Abstract

Mitotic cells in culture show a limited replicative potential and after extended subculturing undergo a terminal growth arrest termed cellular senescence. When cells reach the senescent phenotype, this is accompanied by a significant change in the cellular phenotype and massive changes in gene expression, including the upregulation of secreted factors. In human fibroblasts, senescent cells also acquire resistance to apoptosis. In contrary, in human endothelial cells, both replicative and stress-induced premature senescence is accompanied by increased cell death; however mechanisms of cell death are poorly explored. In this communication, we addressed the role of endonuclease G (EndoG), a mitochondrial mediator of caspase-independent cell death, in senescence-associated cell death of human endothelial cells. Using immunofluorescence microscopy, we found, that EndoG is localized in the mitochondria in young cells, but relocalizes to the nucleus upon senescence. When EndoG gene expression was downregulated by lentiviral shRNA vectors, we found a significant reduction in the replicative life span and a corresponding increase in cell death. We also observed a slight shift in the cell death phenotype from necrosis to apoptosis. Together these observations suggest an important role of EndoG in the senescence program of human endothelial cells.

Published
2011

11. Analysis of the cellular uptake and nuclear delivery of insulin-like growth factor binding protein-3 in human osteosarcoma cells

Author

Laich, A., Matscheski, A., Mück, C., Ferrando-May, E., Pircher, H., Ebner, H.L., Micutkova, L., Huber, L.A., Hermann, M., Offerdinger, M., Hess, M.W., Jansen-Dürr, P., and Zwerschke, W..

Subjects
IGFBP-3 Endocytosis Trafficking Nuclear_Transport Importin,Biological Sciences, hormones, hormone substitutes, and hormone antagonists
Abstract

Insulin-like growth factor (IGF) binding protein-3 (IGFBP-3) is an important regulator of cell proliferation and survival, which plays an important role in a variety of epithelial cancers, including prostate cancer, cervical cancer and breast cancer. IGFBP-3 was described as a tumor suppressor in the prostate and identified as a functional cellular target for the E7 oncoprotein of human papillomaviruses. IGFBP-3 interacts with IGF-I outside the cell; however, IGF-independent actions of IGFBP-3 were also described which are mediated by intracellular IGFBP-3, including nuclear IGFBP-3. The mechanisms by which extracellular proteins can reach the nucleus are still largely unknown. We show here that the addition of IGFBP-3 to living cells results in the rapid appearance of nuclear IGFBP-3 by confocal microscopy of IGFBP-3 uptake in live cells, supported by electron microscopy and cell fractionation studies. IGFBP-3 is internalized through a dynamin-dependent pathway, traffics through endocytic compartments and is finally delivered into the nucleus. We observed docking of IGFBP-3 containing structures to the nuclear envelope and found IGFBP-3 containing dot-like structures to permeate the nuclear envelope. In summary, our findings establish the pathway by which this tumor suppressor protein is delivered from extracellular space to the nucleus.

Published
2010

12. miR-17, miR-19b, miR-20a and miR-106a are down-regulated in human aging

Author

Strasser, A., Trost, A., Grubeck-Loebenstein, B., Mück, C., Papak, C., Schreiner, C., Herndler-Brandstetter, D., Tschachler, E., Laschober, G., Lepperdinger, G., Kühnel, H., Grillari, J., Bauer, J.W., Fortschegger, K., Eckhard, L., Micutkova, L., Breitenbach, M., Hackl, M., Mildner, M., Rinnerthaler, M., Scheideler, M., Wieser, M., Sampson, N., Berger, P., Jansen-Dürr, P., Grillari-Voglauer, R., Brunner, S., and Trajanoski, Z.

Subjects
Biological Sciences
Abstract

Aging is a multifactorial process where deterioration of body functions is driven by stochastic damage while counteracted by distinct genetically encoded repair systems. In order to better understand the genetic component of aging, many studies have addressed the gene and protein expression profiles of various aging model systems engaging different organisms from yeast to human. The recently identified small non-coding miRNAs are potent post-transcriptional regulators that can modify the expression of up to several hundred target genes per single miRNA, similar to transcription factors. Increasing evidence shows that miRNAs contribute to the regulation of most if not all important physiological processes, including aging. However, so far the contribution of miRNAs to age-related and senescence-related changes in gene expression remains elusive. To address this question, we have selected 4 replicative cell aging models including endothelial cells, replicated CD8+ 13 T cells, renal proximal tubular epithelial cells, and skin fibroblasts. Further included were three organismal aging models including foreskin, mesenchymal stem cells and CD8+ 16 T cell populations from old and young donors. Using LNA-based miRNA microarrays we identified four commonly regulated miRNAs, miR-17 down-regulated in all 7, miR-19b and miR-20a, down-regulated in 6 models and miR-106a down19 regulated in 5 models. Decrease in these miRNAs correlated with increased transcript levels of some established target genes, especially the cdk inhibitor p21/CDKN1A. These results establish miRNAs as novel markers of cell aging in humans.

Published
2009

13. Gene expression of catecholamine synthesizing enzymes in A5 cell group and modulation of tyrosine hydroxylase mRNA by immobilization stress

Author

Micutkova L, Kiss A, Filipenko M, Rychkova N, Krizanova O, Miklós Palkovits, and Kvetnansky R

Subjects
Male, Neurons, Restraint, Physical, Time Factors, Tyrosine 3-Monooxygenase, Reverse Transcriptase Polymerase Chain Reaction, Phenylethanolamine N-Methyltransferase, Brain, Gene Expression, Dopamine beta-Hydroxylase, Rats, Rats, Sprague-Dawley, Norepinephrine, Stress, Physiological, Animals, RNA, Messenger
Abstract

The A5 group of noradrenergic neurons plays a key role in autonomic mechanisms like cardiovascular regulation, nociception and respiration. The aim of this work was to detect the gene expression of catecholamine synthesizing enzymes in A5 brain nuclei.The gene expression of. tyrosine hydroxylase (TH), dopamine-beta-hydroxylase (DBH) and phenylethanolamine N-methyl-transferase (PNMT) in A5 brain nuclei was estimated. We also investigated various time intervals after the end of the single two-hour immobilization, as well as the effect of short-term repeated immobilization (120 min daily for 7 days) on tyrosine hydroxylase gene expression, the rate-limiting enzymes in catecholamines biosynthesis, in the A5 cell group. For all experiments, reverse transcription with subsequent polymerase chain reaction (RT-PCR) was used.As expected, we detected a clear signal for TH and DBH mRNA but no signal for PNMT mRNA. Both, single and repeated immobilization stress exposure increased significantly the gene expression of TH in A5 area. Maximal elevation in TH mRNA levels occurred after single immobilization for two hours and subsequent decapitation 24 hours later.In this study we detected for the first time the presence of DBH mRNA in micro dissected A5 cell group. We also showed how the gene expression of tyrosine hydroxylase changed with the function of time after the single immobilization exposure. Thus, TH mRNA in A5 cell group is modulated by immobilization stress in a time-dependent manner.

Published
2002

16. Cas-CLOVER-mediated knockout of STAT1: A novel approach to engineer packaging HEK-293 cell lines used for rAAV production.

Author

Andorfer P, Kahlig CI, Pakusic D, Pachlinger R, John C, Schrenk I, Eisenhut P, Lengler J, Innthaler B, Micutkova L, Kraus B, Brizzee C, Crawford J, and Hernandez Bort JA

Subjects
Humans, HEK293 Cells, Genetic Vectors genetics, RNA, Guide, CRISPR-Cas Systems genetics, Dependovirus genetics, STAT1 Transcription Factor genetics, STAT1 Transcription Factor metabolism, CRISPR-Cas Systems genetics, Gene Editing methods, Gene Knockout Techniques methods
Abstract

In addressing the limitations of CRISPR-Cas9, including off-target effects and high licensing fees for commercial use, Cas-CLOVER, a dimeric gene editing tool activated by two guide RNAs, was recently developed. This study focused on implementing and evaluating Cas-CLOVER in HEK-293 cells used for recombinant adeno-associated virus (rAAV) production by targeting the signal transducer and activator of transcription 1 (STAT1) locus, which is crucial for cell growth regulation and might influence rAAV production yields. Cas-CLOVER demonstrated impressive efficiency in gene editing, achieving over 90% knockout (KO) success. Thirteen selected HEK-293 STAT1 KO sub-clones were subjected to extensive analytical characterization to assess their genomic stability, crucial for maintaining cell integrity and functionality. Additionally, rAAV9 productivity, Rep protein pattern profile, and potency, among others, were assessed. Clones showed significant variation in capsid and vector genome titers, with capsid titer reductions ranging from 15% to 98% and vector genome titers from 16% to 55%. Interestingly, the Cas-CLOVER-mediated STAT1 KO bulk cell population showed a better ratio of full to empty capsids. Our study also established a comprehensive analytical workflow to detect and evaluate the gene KOs generated by this innovative tool, providing a solid groundwork for future research in precise gene editing technologies., (© 2024 The Author(s). Biotechnology Journal published by Wiley‐VCH GmbH.)

Published
2024
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17. Enhancement of rAAV titers via inhibition of the interferon signaling cascade in transfected HEK293 suspension cultures.

Author

Kahlig CI, Moser S, Micutkova L, Grillari J, Kraus B, and Hernandez Bort JA

Subjects
Humans, HEK293 Cells, Nitriles pharmacology, Pyrimidines pharmacology, Transfection, Pyrazoles pharmacology, Signal Transduction, Dependovirus genetics, Interferons metabolism, Interferons genetics
Abstract

The production of recombinant adeno-associated virus (rAAV) for gene therapy applications relies on the use of various host cell lines, with suspension-grown HEK293 cells being the preferred expression system due to their satisfactory rAAV yields in transient transfections. As the field of gene therapy continues to expand, there is a growing demand for efficient rAAV production, which has prompted efforts to optimize HEK293 cell line productivity through engineering. In contrast to other cell lines like CHO cells, the transcriptome of HEK293 cells during rAAV production has remained largely unexplored in terms of identifying molecular components that can enhance yields. In our previous research, we analyzed global regulatory pathways and mRNA expression patterns associated with increased rAAV production in HEK293 cells. Our data revealed substantial variations in the expression patterns between cell lines with low (LP) and high-production (HP) rates. Moving to a deeper layer for a more detailed analysis of inflammation-related transcriptome data, we detected an increased expression of interferon-related genes in low-producing cell lines. Following upon these results, we investigated the use of Ruxolitinib, an interferon pathway inhibitor, during the transient production of rAAV in HEK293 cells as potential media additive to boost rAAV titers. Indeed, we find a two-fold increase in rAAV titers compared to the control when the interferon pathways were inhibited. In essence, this work offers a rational design approach for optimization of HEK293 cell line productivity and potential engineering targets, ultimately paving the way for more cost-efficient and readily available gene therapies for patients., (© 2024 The Authors. Biotechnology Journal published by Wiley‐VCH GmbH.)

Published
2024
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18. Loss of the ribosomal RNA methyltransferase NSUN5 impairs global protein synthesis and normal growth.

Author

Heissenberger C, Liendl L, Nagelreiter F, Gonskikh Y, Yang G, Stelzer EM, Krammer TL, Micutkova L, Vogt S, Kreil DP, Sekot G, Siena E, Poser I, Harreither E, Linder A, Ehret V, Helbich TH, Grillari-Voglauer R, Jansen-Dürr P, Koš M, Polacek N, Grillari J, and Schosserer M

Subjects
Animals, Body Weight genetics, Cell Enlargement, Cell Proliferation genetics, Cells, Cultured, Child, Embryo, Mammalian, Female, Gene Deletion, HEK293 Cells, HeLa Cells, Humans, Infant, Male, Mice, Mice, Inbred C57BL, Mice, Knockout, Growth and Development genetics, Methyltransferases genetics, Muscle Proteins genetics, Protein Biosynthesis genetics
Abstract

Modifications of ribosomal RNA expand the nucleotide repertoire and thereby contribute to ribosome heterogeneity and translational regulation of gene expression. One particular m5C modification of 25S ribosomal RNA, which is introduced by Rcm1p, was previously shown to modulate stress responses and lifespan in yeast and other small organisms. Here, we report that NSUN5 is the functional orthologue of Rcm1p, introducing m5C3782 into human and m5C3438 into mouse 28S ribosomal RNA. Haploinsufficiency of the NSUN5 gene in fibroblasts from William Beuren syndrome patients causes partial loss of this modification. The N-terminal domain of NSUN5 is required for targeting to nucleoli, while two evolutionary highly conserved cysteines mediate catalysis. Phenotypic consequences of NSUN5 deficiency in mammalian cells include decreased proliferation and size, which can be attributed to a reduction in total protein synthesis by altered ribosomes. Strikingly, Nsun5 knockout in mice causes decreased body weight and lean mass without alterations in food intake, as well as a trend towards reduced protein synthesis in several tissues. Together, our findings emphasize the importance of single RNA modifications for ribosome function and normal cellular and organismal physiology., (© The Author(s) 2019. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published
2019
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19. Secreted microvesicular miR-31 inhibits osteogenic differentiation of mesenchymal stem cells.

Author

Weilner S, Schraml E, Wieser M, Messner P, Schneider K, Wassermann K, Micutkova L, Fortschegger K, Maier AB, Westendorp R, Resch H, Wolbank S, Redl H, Jansen-Dürr P, Pietschmann P, Grillari-Voglauer R, and Grillari J

Subjects
Adipose Tissue cytology, Aging blood, Cell-Derived Microparticles ultrastructure, Cellular Senescence, Endothelial Cells metabolism, Frizzled Receptors genetics, Frizzled Receptors metabolism, Gene Knockdown Techniques, Human Umbilical Vein Endothelial Cells metabolism, Humans, MicroRNAs genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Tetraspanin 30 metabolism, Cell Differentiation, Cell-Derived Microparticles metabolism, Mesenchymal Stem Cells cytology, Mesenchymal Stem Cells metabolism, MicroRNAs metabolism, Osteogenesis
Abstract

Damage to cells and tissues is one of the driving forces of aging and age-related diseases. Various repair systems are in place to counteract this functional decline. In particular, the property of adult stem cells to self-renew and differentiate is essential for tissue homeostasis and regeneration. However, their functionality declines with age (Rando, 2006). One organ that is notably affected by the reduced differentiation capacity of stem cells with age is the skeleton. Here, we found that circulating microvesicles impact on the osteogenic differentiation capacity of mesenchymal stem cells in a donor-age-dependent way. While searching for factors mediating the inhibitory effect of elderly derived microvesicles on osteogenesis, we identified miR-31 as a crucial component. We demonstrated that miR-31 is present at elevated levels in the plasma of elderly and of osteoporosis patients. As a potential source of its secretion, we identified senescent endothelial cells, which are known to increase during aging in vivo (Erusalimsky, 2009). Endothelial miR-31 is secreted within senescent cell-derived microvesicles and taken up by mesenchymal stem cells where it inhibits osteogenic differentiation by knocking down its target Frizzled-3. Therefore, we suggest that microvesicular miR-31 in the plasma of elderly might play a role in the pathogenesis of age-related impaired bone formation and that miR-31 might be a valuable plasma-based biomarker for aging and for a systemic environment that does not favor cell-based therapies whenever osteogenesis is a limiting factor., (© 2016 The Authors. Aging Cell published by the Anatomical Society and John Wiley & Sons Ltd.)

Published
2016
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20. Identification of microRNA-mRNA functional interactions in UVB-induced senescence of human diploid fibroblasts.

Author

Greussing R, Hackl M, Charoentong P, Pauck A, Monteforte R, Cavinato M, Hofer E, Scheideler M, Neuhaus M, Micutkova L, Mueck C, Trajanoski Z, Grillari J, and Jansen-Dürr P

Subjects
Cell Line, Tumor, Cellular Senescence radiation effects, Diploidy, Enhancer of Zeste Homolog 2 Protein, Fibroblasts radiation effects, Gene Regulatory Networks radiation effects, Humans, Polycomb Repressive Complex 2 metabolism, RNA Interference radiation effects, Transcriptome radiation effects, Ultraviolet Rays, Cellular Senescence genetics, Fibroblasts metabolism, MicroRNAs physiology, Polycomb Repressive Complex 2 genetics, RNA, Messenger genetics
Abstract

Background: Cellular senescence can be induced by a variety of extrinsic stimuli, and sustained exposure to sunlight is a key factor in photoaging of the skin. Accordingly, irradiation of skin fibroblasts by UVB light triggers cellular senescence, which is thought to contribute to extrinsic skin aging, although molecular mechanisms are incompletely understood. Here, we addressed molecular mechanisms underlying UVB induced senescence of human diploid fibroblasts., Results: We observed a parallel activation of the p53/p21(WAF1) and p16(INK4a)/pRb pathways. Using genome-wide transcriptome analysis, we identified a transcriptional signature of UVB-induced senescence that was conserved in three independent strains of human diploid fibroblasts (HDF) from skin. In parallel, a comprehensive screen for microRNAs regulated during UVB-induced senescence was performed which identified five microRNAs that are significantly regulated during the process. Bioinformatic analysis of miRNA-mRNA networks was performed to identify new functional mRNA targets with high confidence for miR-15a, miR-20a, miR-20b, miR-93, and miR-101. Already known targets of these miRNAs were identified in each case, validating the approach. Several new targets were identified for all of these miRNAs, with the potential to provide new insight in the process of UVB-induced senescence at a genome-wide level. Subsequent analysis was focused on miR-101 and its putative target gene Ezh2. We confirmed that Ezh2 is regulated by miR-101 in human fibroblasts, and found that both overexpression of miR-101 and downregulation of Ezh2 independently induce senescence in the absence of UVB irradiation. However, the downregulation of miR-101 was not sufficient to block the phenotype of UVB-induced senescence, suggesting that other UVB-induced processes induce the senescence response in a pathway redundant with upregulation of miR-101., Conclusion: We performed a comprehensive screen for UVB-regulated microRNAs in human diploid fibroblasts, and identified a network of miRNA-mRNA interactions mediating UVB-induced senescence. In addition, miR-101 and Ezh2 were identified as key players in UVB-induced senescence of HDF.

Published
2013
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21. Analysis of the cellular uptake and nuclear delivery of insulin-like growth factor binding protein-3 in human osteosarcoma cells.

Author

Micutkova L, Hermann M, Offterdinger M, Hess MW, Matscheski A, Pircher H, Mück C, Ebner HL, Laich A, Ferrando-May E, Zwerschke W, Huber LA, and Jansen-Dürr P

Subjects
Cell Fractionation methods, Cytoplasm metabolism, Endocytosis physiology, Humans, Insulin-Like Growth Factor Binding Protein 3 pharmacokinetics, Microscopy, Confocal methods, Microscopy, Electron methods, Protein Binding, Recombinant Proteins pharmacokinetics, Tumor Cells, Cultured, Bone Neoplasms metabolism, Cell Nucleus metabolism, Insulin-Like Growth Factor Binding Protein 3 metabolism, Osteosarcoma metabolism, Protein Transport physiology
Abstract

Insulin-like growth factor (IGF) binding protein-3 (IGFBP-3) regulates cell proliferation and survival by extracellular interaction and inactivation of the growth factor IGF-I. Beyond that, IGF-independent actions mediated by intracellular IGFBP-3 including nuclear-IGFBP-3, have also been described. We here show, using both confocal and electron microscopy and cell fractionation, that the extracellular addition of IGFBP-3 to living cells results in rapid uptake and nuclear delivery of IGFBP-3, by yet partly unknown mechanisms. IGFBP-3 is internalized through a dynamin-dependent pathway, traffics through endocytic compartments and is finally delivered into the nucleus. We observed docking of IGFBP-3 containing structures to the nuclear envelope and found IGFBP-3 containing dot-like structures to permeate the nuclear envelope. In summary, our findings establish the pathway by which this tumor suppressor protein is delivered from extracellular space to the nucleus., (Copyright © 2011 UICC.)

Published
2012
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22. Purification and characterization of native human insulin-like growth factor binding protein-6.

Author

Taferner A, Micutkova L, Hermann M, Jansen-Dürr P, and Pircher H

Abstract

Insulin-like growth factor binding proteins (IGFBPs) are key regulators of insulin-like growth factor (IGF) mediated signal transduction and thereby can profoundly influence cellular phenotypes and cell fate. Whereas IGFBPs are extracellular proteins, intracellular activities were described for several IGFBP family members, such as IGFBP-3, which can be reinternalized by endocytosis and reaches the nucleus through routes that remain to be fully established. Within the family of IGFBPs, IGFBP-6 is unique for its specific binding to IGF-II. IGFBP-6 was described to possess additional IGF-independent activities, which have in part been attributed to its translocation to the nucleus; however, cellular uptake of IGFBP-6 was not described. To further explore IGFBP-6 functions, we developed a new method for the purification of native human IGFBP-6 from cell culture supernatants, involving a four-step affinity purification procedure, which yields highly enriched IGFBP-6. Whereas protein purified in this way retained the capacity to interact with IGF-II and modulate IGF-dependent signal transduction, our data suggest that, unlike IGFBP-3, human IGFBP-6 is not readily internalized by human tumor cells. To summarize, this work describes a novel and efficient method for the purification of native human insulin-like growth factor binding protein 6 (IGFBP-6) from human cell culture supernatants, applying a four-step chromatography procedure. Intactness of purified IGFBP-6 was confirmed by IGF ligand Western blot and ability to modulate IGF-dependent signal transduction. Cellular uptake studies were performed to further characterize the purified protein, showing no short-term uptake of IGFBP-6, in contrast to IGFBP-3.

Published
2011
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23. Insulin-like growth factor binding protein-6 delays replicative senescence of human fibroblasts.

Author

Micutkova L, Diener T, Li C, Rogowska-Wrzesinska A, Mueck C, Huetter E, Weinberger B, Grubeck-Loebenstein B, Roepstorff P, Zeng R, and Jansen-Duerr P

Subjects
Adult, Aged, Aging blood, Amino Acid Sequence, Apoptosis genetics, Apoptosis physiology, Base Sequence, Cell Proliferation, Cell Survival genetics, Cell Survival physiology, Cells, Cultured, Cellular Senescence genetics, DNA Primers genetics, Down-Regulation, Fibroblasts cytology, Fibroblasts physiology, Gene Knockdown Techniques, Humans, Insulin-Like Growth Factor Binding Protein 6 antagonists & inhibitors, Insulin-Like Growth Factor Binding Protein 6 genetics, Molecular Sequence Data, RNA, Small Interfering genetics, Real-Time Polymerase Chain Reaction, Up-Regulation, Cellular Senescence physiology, Insulin-Like Growth Factor Binding Protein 6 physiology
Abstract

Cellular senescence can be induced by a variety of mechanisms, and recent data suggest a key role for cytokine networks to maintain the senescent state. Here, we have used a proteomic LC-MS/MS approach to identify new extracellular regulators of senescence in human fibroblasts. We identified 26 extracellular proteins with significantly different abundance in conditioned media from young and senescent fibroblasts. Among these was insulin-like growth factor binding protein-6 (IGFBP-6), which was chosen for further analysis. When IGFBP-6 gene expression was downregulated, cell proliferation was inhibited and apoptotic cell death was increased. Furthermore, downregulation of IGFBP-6 led to premature entry into cellular senescence. Since IGFBP-6 overexpression increased cellular lifespan, the data suggest that IGFBP-6, in contrast to other IGF binding proteins, is a negative regulator of cellular senescence in human fibroblasts., (Copyright © 2011 Elsevier Ireland Ltd. All rights reserved.)

Published
2011
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24. Identification of evolutionarily conserved genetic regulators of cellular aging.

Author

Laschober GT, Ruli D, Hofer E, Muck C, Carmona-Gutierrez D, Ring J, Hutter E, Ruckenstuhl C, Micutkova L, Brunauer R, Jamnig A, Trimmel D, Herndler-Brandstetter D, Brunner S, Zenzmaier C, Sampson N, Breitenbach M, Fröhlich KU, Grubeck-Loebenstein B, Berger P, Wieser M, Grillari-Voglauer R, Thallinger GG, Grillari J, Trajanoski Z, Madeo F, Lepperdinger G, and Jansen-Dürr P

Subjects
Adult, Child, Preschool, Databases, Genetic, Humans, Middle Aged, Oxidative Stress, Saccharomyces cerevisiae genetics, Cellular Senescence genetics, Evolution, Molecular, Gene Expression Regulation
Abstract

To identify new genetic regulators of cellular aging and senescence, we performed genome-wide comparative RNA profiling with selected human cellular model systems, reflecting replicative senescence, stress-induced premature senescence, and distinct other forms of cellular aging. Gene expression profiles were measured, analyzed, and entered into a newly generated database referred to as the GiSAO database. Bioinformatic analysis revealed a set of new candidate genes, conserved across the majority of the cellular aging models, which were so far not associated with cellular aging, and highlighted several new pathways that potentially play a role in cellular aging. Several candidate genes obtained through this analysis have been confirmed by functional experiments, thereby validating the experimental approach. The effect of genetic deletion on chronological lifespan in yeast was assessed for 93 genes where (i) functional homologues were found in the yeast genome and (ii) the deletion strain was viable. We identified several genes whose deletion led to significant changes of chronological lifespan in yeast, featuring both lifespan shortening and lifespan extension. In conclusion, an unbiased screen across species uncovered several so far unrecognized molecular pathways for cellular aging that are conserved in evolution., (© 2010 The Authors. Aging Cell © 2010 Blackwell Publishing Ltd/Anatomical Society of Great Britain and Ireland.)

Published
2010
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25. Role of endonuclease G in senescence-associated cell death of human endothelial cells.

Author

Diener T, Neuhaus M, Koziel R, Micutkova L, and Jansen-Dürr P

Subjects
Active Transport, Cell Nucleus, Aging genetics, Aging metabolism, Cells, Cultured, Endodeoxyribonucleases antagonists & inhibitors, Gene Expression, Gene Knockdown Techniques, Humans, Lentivirus genetics, Membrane Potential, Mitochondrial, Necrosis enzymology, Necrosis genetics, Necrosis pathology, RNA, Small Interfering genetics, Apoptosis genetics, Apoptosis physiology, Cellular Senescence genetics, Cellular Senescence physiology, Endodeoxyribonucleases genetics, Endodeoxyribonucleases metabolism, Endothelial Cells cytology, Endothelial Cells enzymology
Abstract

Mitotic cells in culture show a limited replicative potential and after extended subculturing undergo a terminal growth arrest termed cellular senescence. When cells reach the senescent phenotype, this is accompanied by a significant change in the cellular phenotype and massive changes in gene expression, including the upregulation of secreted factors. In human fibroblasts, senescent cells also acquire resistance to apoptosis. In contrary, in human endothelial cells, both replicative and stress-induced premature senescence is accompanied by increased cell death; however mechanisms of cell death are poorly explored. In this communication, we addressed the role of endonuclease G (EndoG), a mitochondrial mediator of caspase-independent cell death, in senescence-associated cell death of human endothelial cells. Using immunofluorescence microscopy, we found, that EndoG is localized in the mitochondria in young cells, but relocalizes to the nucleus upon senescence. When EndoG gene expression was downregulated by lentiviral shRNA vectors, we found a significant reduction in the replicative life span and a corresponding increase in cell death. We also observed a slight shift in the cell death phenotype from necrosis to apoptosis. Together these observations suggest an important role of EndoG in the senescence program of human endothelial cells., (Copyright (c) 2010 Elsevier Inc. All rights reserved.)

Published
2010
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26. A new method for the purification of bioactive insulin-like growth factor-binding protein-3.

Author

Pircher H, Matscheski A, Laich A, Hermann M, Moser B, Viertler HP, Micutkova L, Lindner H, Sarg B, Zwerschke W, and Jansen-Dürr P

Subjects
Humans, Protein Binding, Recombinant Proteins metabolism, Signal Transduction, Chromatography, Affinity, Fibroblasts metabolism, Insulin-Like Growth Factor Binding Protein 3 metabolism, Insulin-Like Growth Factor Binding Proteins metabolism, Somatomedins metabolism
Abstract

We present a novel efficient procedure for high level purification of human IGFBP-3. Insulin-like growth factor-binding proteins (IGFBPs) are key regulators of insulin-like growth factor mediated signal transduction and thereby can profoundly influence cellular phenotypes. Certain IGFBPs, including IGFBP-3, have also been described to possess additional IGF-independent activities, which rely, at least in part, on their nuclear localization. However, the mechanisms of IGF-independent biological activities of IGFBP-3 are not well understood. For the study of these functions, recombinant IGFBP-3 is used. However, it has traditionally been difficult to obtain recombinant protein in sufficient quality and quantity. Here we describe a new procedure for the purification of recombinant IGFBP-3 from cell culture supernatants involving a two-step affinity purification procedure. Using this new protocol, we obtained pure IGFBP-3 free of any visible contaminants. We also provide evidence that the protein purified in this way retains biological activity, to bind IGF and modulate IGF-dependent signal transduction. We also show that the purified protein produced by the new procedure is readily internalized by human fibroblasts, suggesting that this protein is also suitable to study intracellular trafficking of IGFBP-3.

Published
2010
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27. miR-17, miR-19b, miR-20a, and miR-106a are down-regulated in human aging.

Author

Hackl M, Brunner S, Fortschegger K, Schreiner C, Micutkova L, Mück C, Laschober GT, Lepperdinger G, Sampson N, Berger P, Herndler-Brandstetter D, Wieser M, Kühnel H, Strasser A, Rinnerthaler M, Breitenbach M, Mildner M, Eckhart L, Tschachler E, Trost A, Bauer JW, Papak C, Trajanoski Z, Scheideler M, Grillari-Voglauer R, Grubeck-Loebenstein B, Jansen-Dürr P, and Grillari J

Subjects
CD8-Positive T-Lymphocytes cytology, CD8-Positive T-Lymphocytes metabolism, Cell Proliferation, Cells, Cultured, Humans, Oligonucleotide Array Sequence Analysis, Aging, Down-Regulation, MicroRNAs genetics
Abstract

Aging is a multifactorial process where deterioration of body functions is driven by stochastic damage while counteracted by distinct genetically encoded repair systems. To better understand the genetic component of aging, many studies have addressed the gene and protein expression profiles of various aging model systems engaging different organisms from yeast to human. The recently identified small non-coding miRNAs are potent post-transcriptional regulators that can modify the expression of up to several hundred target genes per single miRNA, similar to transcription factors. Increasing evidence shows that miRNAs contribute to the regulation of most if not all important physiological processes, including aging. However, so far the contribution of miRNAs to age-related and senescence-related changes in gene expression remains elusive. To address this question, we have selected four replicative cell aging models including endothelial cells, replicated CD8(+) T cells, renal proximal tubular epithelial cells, and skin fibroblasts. Further included were three organismal aging models including foreskin, mesenchymal stem cells, and CD8(+) T cell populations from old and young donors. Using locked nucleic acid-based miRNA microarrays, we identified four commonly regulated miRNAs, miR-17 down-regulated in all seven; miR-19b and miR-20a, down-regulated in six models; and miR-106a down-regulated in five models. Decrease in these miRNAs correlated with increased transcript levels of some established target genes, especially the cdk inhibitor p21/CDKN1A. These results establish miRNAs as novel markers of cell aging in humans.

Published
2010
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28. Identification of Hsc70 as target for AGE modification in senescent human fibroblasts.

Author

Unterluggauer H, Micutkova L, Lindner H, Sarg B, Hernebring M, Nystrom T, and Jansen-Dürr P

Subjects
Cells, Cultured, Humans, Oxidation-Reduction, Cellular Senescence, Endothelial Cells metabolism, Fibroblasts metabolism, Glycation End Products, Advanced metabolism, HSC70 Heat-Shock Proteins metabolism, Protein Carbonylation, Protein Processing, Post-Translational
Abstract

Cellular senescence is known as a potent mechanism of tumor suppression, and cellular senescence in vitro also reflects at least some features of aging in vivo. The Free Radical Theory of aging suggests that reactive oxygen species are important causative agents of aging and cellular senescence. Besides damage of nucleic acids and lipids, also oxidative modifications of proteins have been described as potential causative events in the senescence response. However, the identity of protein targets for post-translational modifications in senescent cells has remained unclear. In the present communication, we analyzed the occurrence of oxidative posttranslational modifications in senescent human endothelial cells and dermal fibroblasts. We found a significant increase in the level of protein carbonyls and AGE modification with senescence in both cell types. Using 2D-Gel electrophoresis and Western Blot we found that heat shock cognate protein 70 is a bona fide target for AGE modification in human fibroblasts.

Published
2009
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29. Role of insulin-like growth factor binding protein-3 in human umbilical vein endothelial cell senescence.

Author

Muck C, Micutkova L, Zwerschke W, and Jansen-Durr P

Subjects
Blotting, Western, Cell Proliferation, Humans, Transduction, Genetic, Cellular Senescence, Endothelial Cells cytology, Endothelial Cells metabolism, Insulin-Like Growth Factor Binding Protein 3 metabolism, Umbilical Veins cytology, Umbilical Veins metabolism
Abstract

Whereas insulin-like growth factor binding protein-3 (IGFBP-3) is frequently upregulated in senescent replicatively exhausted human umbilical vein endothelial cells (HUVEC), a systematic analysis of four different HUVEC donors revealed that IGFBP-3 is not consistently upregulated in all isolates at senescence. Lentiviral overexpression of IGFBP-3 inhibited cell proliferation, induced apoptosis and senescence in young HUVEC. Knockdown of IGFBP-3 in senescent HUVEC by lentivirally expressed shRNA did not revert but rather enforced senescence-associated beta-galactosidase staining and apoptosis. Together the data suggest that, although IGFBP-3 acts as an anti-proliferative and premature senescence-inducing protein, the role of IGFBP-3 on senescence depends on the genetic background of the donor, and additional factors might be important to maintain the senescent phenotype.

Published
2008
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30. Changes in gene expression of phenylethanolamine N-methyltransferase in the transplanted human heart.

Author

Goncalvesova E, Micutkova L, Mravec B, Ksinantova L, Krizanova O, Fabian J, and Kvetnansky R

Subjects
Adult, Humans, Middle Aged, RNA, Messenger genetics, Gene Expression Regulation, Enzymologic, Heart Transplantation, Phenylethanolamine N-Methyltransferase genetics
Abstract

Heart transplantation (HTx) is an accepted treatment for precisely defined patients with chronic congestive heart failure; however, as a result of the procedure, the graft is completely denervated. Our study focused on the catecholamine biosynthetic pathway, that is, the production of epinephrine, which is known to have positive chronotropic and inotropic effects on the heart. mRNA levels of the phenylethanolamine N-methyltransferase (PNMT), the enzyme catalyzing epinephrine synthesis in myocardial tissue, were determined in 18 patients (0 to 10 yr after HTx). Samples of myocardium were obtained from the right ventricle at the time of a routine endomyocardial biopsy performed for the diagnosis of graft rejection. Results were correlated with the following clinical parameters: heart rate, heart rate variability, blood pressure, graft systolic function, and the presence of the rejection. We observed that heart PNMT mRNA levels were significantly higher during the first 3 yr as compared to longer periods after HTx. Also, a decrease in the average heart rate and an increase in the heart rate variability were documented. Levels of the PNMT mRNA do not correlate with blood pressure, left ventricular systolic function at rest, and rejection. Thus, a gradual decrease of the heart rate and an increase in the heart rate variability after HTx is considered to be a sign of cardiac graft reinervation. We speculate that the increased PNMT transcription in human myocardium in early intervals after HTx reflects "autonomous sympathicotrophy." A decrease in the PNMT gene expression with the number of years after HTx could be a consequence of the reinnervation process.

Published
2004
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31. Localization and regulation of phenylethanolamine N-methyltransferase gene expression in the heart of rats and mice during stress.

Author

Kvetnansky R, Micutkova L, Kubovcakova L, Sabban EL, Palkovits M, and Krizanova O

Subjects
Animals, Male, Mice, Mice, Knockout, Phenylethanolamine N-Methyltransferase metabolism, Polymerase Chain Reaction, RNA, Messenger genetics, Rats, Rats, Sprague-Dawley, Stress, Physiological enzymology, Gene Expression Regulation, Enzymologic physiology, Myocardium enzymology, Phenylethanolamine N-Methyltransferase genetics, Stress, Physiological physiopathology
Abstract

Recently we have described the existence of phenylethanolamine N-methyltransferase (PNMT) mRNA in the heart of adult rats. In this study, we report the first data on distribution of the PNMT protein in rat hearts, which follows the distribution of PNMT mRNA (high levels in the atria and low levels in ventricles). The main aim of this study was to determine the localization of the PNMT mRNA in the heart and to examine whether gene expression of this enzyme is affected by immobilization (IMO) stress in a time-dependent manner. PNMT mRNA levels were detected in all seven studied parts of the heart (atria without and with intramural ganglion cells, ventricles, and septum), with the highest levels in the left atrium and its ganglionic part. Both Southern blot and sequencing verified the specificity of PNMT detected by RT-PCR. Single IMO for 2-h increased gene expression of PNMT, as determined by both RT-PCR and Real-Time PCR in the right and left atria. Surprisingly, the ganglionic parts of the atria did not respond to stress stimulation. Peak levels of PNMT mRNA were found in the 3-h interval after the IMO terminated, and also 24 h after the first or sixth IMO. Expression of aromatic L-amino acids decarboxylase and dopamine-beta-hydroxylase has also been detected in the heart of control and stressed rats. In the atria, the effect of stress is clearly modulated by glucocorticoids, since in mice with corticotrophin-releasing hormone knocked out gene the immobilization-induced increase in the PNMT mRNA levels seen in wild-type animals was abolished. Thus, our data have shown that gene expression of the PNMT is localized, not predominantly in cardiac ganglion cells, but in a wide range in atrial cardiomyocytes. Mechanism responsible for the regulation of stress-induced increase of PNMT gene expression in cardiac atria is clearly dependent on the presence of glucocorticoids.

Published
2004
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32. Repeated immobilization stress decreases mRNA and protein levels of the type 1 IP3 receptor in rat heart.

Author

Krepsova K, Micutkova L, Novotova M, Kubovcakova L, Kvetnansky R, and Krizanova O

Subjects
Animals, Base Sequence, Blotting, Western, Calcium Channels genetics, DNA Primers, Inositol 1,4,5-Trisphosphate Receptors, Male, Myocardium ultrastructure, Polymerase Chain Reaction, RNA, Messenger genetics, Rats, Rats, Sprague-Dawley, Receptors, Cytoplasmic and Nuclear genetics, Stress, Physiological genetics, Calcium Channels metabolism, Immobilization, Myocardium metabolism, RNA, Messenger metabolism, Receptors, Cytoplasmic and Nuclear metabolism, Stress, Physiological metabolism
Abstract

Stress is one of the major contributors to the development of cardiovascular disorders and psychiatric illnesses. Immobilization stress belongs to severe stressors and is known to activate several calcium transport systems. The aim of this work was to determine whether repeated immobilization stress changes mRNA and protein levels of the type 1 and 2 inositol-1,4,5-trisphosphate (IP(3)) receptors in cardiac tissue. Rats were immobilized for 7 days, 2 h daily. After repeated immobilization, increased numbers of collagen fibers were accumulated in the heart atria compared to hearts of the control group of rats. Gene expression was determined after reverse transcription and subsequent real-time polymerase chain reaction, using SYBR Green fluorescent dye. Protein levels were determined by Western blot and hybridization with the primary antibody against IP(3) receptors. Contrary to single immobilization, repeated immobilization decreased a gene expression of the type 1 and 2 IP(3) receptors, and also protein levels of the IP(3) receptors. Although the physiologic relevance of our observations remains to be elucidated, we propose that the decrease in IP(3) receptors may have an impact on the development of the pathophysiologic changes in the heart.

Published
2004
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33. Modulation of catecholamine-synthesizing enzymes in the rat heart by repeated immobilization stress.

Author

Micutkova L, Krepsova K, Sabban E, Krizanova O, and Kvetnansky R

Subjects
Animals, Base Sequence, Blotting, Western, DNA Primers, Male, Polymerase Chain Reaction, Rats, Rats, Sprague-Dawley, Aromatic-L-Amino-Acid Decarboxylases metabolism, Catecholamines biosynthesis, Immobilization, Myocardium enzymology, Phenylethanolamine N-Methyltransferase metabolism
Abstract

Stress is one of the major risk factors responsible for the increased incidence of a number of common life-threatening disorders, predominantly of cardiovascular origin. The aim of the present study was to establish the effect of repeated immobilization stress on gene expression and protein levels of aromatic L-amino acid decarboxylase (AADC) and phenylethanolamine N-methyltransferase (PNMT) in cardiac left and right atria. In the process of repeated immobilization, rats were immobilized 2 h daily for 7 days and killed 3 h after the last immobilization. Gene expression was determined by regular and real-time reverse transcription with subsequent polymerase chain reaction, and protein levels were determined by Western blot analysis. In cardiac atria, we identified mRNA for AADC and PNMT. Repeated immobilization stress did not affect AADC mRNA levels. However, repeated immobilization significantly increased PNMT mRNA levels compared with unstressed control animals. No further increase was observed compared with adapted control rats (rats immobilized six times for 2 h daily and decapitated 24 h after the sixth immobilization). AADC protein levels corresponded with mRNA levels of this enzyme. However, we were not able to detect PNMT immunoreactive protein. The observed elevation in the gene expression of PNMT mRNA levels in the heart may be involved in the increased risk of cardiovascular diseases with stress.

Published
2004
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34. Inositol 1,4,5-trisphosphate receptors in the heart compared to other tissues are differently modulated by stress.

Author

Krizanova O, Krepsova K, Micutkova L, and Kvetnansky R

Subjects
Blotting, Western, Calcium Channels genetics, Humans, Immobilization, Inositol 1,4,5-Trisphosphate Receptors, Polymerase Chain Reaction, RNA, Messenger genetics, RNA, Messenger metabolism, Receptors, Cytoplasmic and Nuclear genetics, Calcium Channels metabolism, Myocardium metabolism, Receptors, Cytoplasmic and Nuclear metabolism, Stress, Physiological metabolism
Abstract

IP(3) receptors are intracellular calcium channels, releasing calcium from the sarcoplasmic reticulum. In the heart, IP(3) receptors of type 1 and 2 were found. These receptors predominate in atria, although they occur also in ventricles, as determined by real-time PCR and Western blot analysis. Single-immobilization stress was found to increase mRNA and/or protein levels of types 1 and 2 IP(3) receptors in cardiac atria. However, in stellate ganglia, which innervate the heart, no changes in the mRNA of the type 1 IP(3) receptors were observed after single-immobilization stress. In adrenal medulla, a moderate decrease in both mRNA and protein levels of IP(3) receptors was observed after single-immobilization exposure. After repeated immobilization, mRNA and protein levels of types 1 and 2 IP(3) receptors decreased significantly in all tested tissues. Our results point to different processing of the single stress in different tissues, while repeated stress results in rapid and significant decrease of the IP(3) receptors.

Published
2004
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35. Immobilization stress elevates IP(3) receptor mRNA in adult rat hearts in a glucocorticoid-dependent manner.

Author

Lencesova L, Ondrias K, Micutkova L, Filipenko M, Kvetnansky R, and Krizanova O

Subjects
Animals, Base Sequence, Blotting, Western, DNA Primers, Inositol 1,4,5-Trisphosphate Receptors, Male, RNA, Messenger metabolism, Rats, Rats, Sprague-Dawley, Calcium Channels genetics, Gene Expression Regulation physiology, Immobilization, Myocardium metabolism, RNA, Messenger genetics, Receptors, Cytoplasmic and Nuclear genetics, Stress, Physiological physiopathology
Abstract

Gene expression of the type 1 and 2 inositol 1,4,5-trisphosphate (IP(3)) receptors in the rat cardiac atria and ventricles and their possible modulation by single immobilization stress was studied. Single immobilization stress significantly elevated mRNA levels for both types of these receptors. To evaluate the involvement of glucocorticoids in the modulation of the gene expression of IP(3) receptors by immobilization stress, we used adrenalectomized and/or hypophysectomized rats. Since adrenalectomy and/or hypophysectomy completely abolished increase in IP(3) receptor's mRNA levels after the immobilization, we conclude that immobilization stress elevates mRNA of type 1 and 2 IP(3) receptors, mainly through the glucocorticoid responsive element.

Published
2002
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36. Gene expression of catecholamine synthesizing enzymes in A5 cell group and modulation of tyrosine hydroxylase mRNA by immobilization stress.

Author

Micutkova L, Kiss A, Filipenko M, Rychkova N, Krizanova O, Palkovits M, and Kvetnansky R

Subjects
Animals, Male, Neurons enzymology, Norepinephrine physiology, RNA, Messenger analysis, Rats, Rats, Sprague-Dawley, Restraint, Physical, Reverse Transcriptase Polymerase Chain Reaction, Time Factors, Brain enzymology, Dopamine beta-Hydroxylase genetics, Gene Expression, Phenylethanolamine N-Methyltransferase genetics, Stress, Physiological enzymology, Tyrosine 3-Monooxygenase genetics
Abstract

Objective: The A5 group of noradrenergic neurons plays a key role in autonomic mechanisms like cardiovascular regulation, nociception and respiration. The aim of this work was to detect the gene expression of catecholamine synthesizing enzymes in A5 brain nuclei., Methods: The gene expression of. tyrosine hydroxylase (TH), dopamine-beta-hydroxylase (DBH) and phenylethanolamine N-methyl-transferase (PNMT) in A5 brain nuclei was estimated. We also investigated various time intervals after the end of the single two-hour immobilization, as well as the effect of short-term repeated immobilization (120 min daily for 7 days) on tyrosine hydroxylase gene expression, the rate-limiting enzymes in catecholamines biosynthesis, in the A5 cell group. For all experiments, reverse transcription with subsequent polymerase chain reaction (RT-PCR) was used., Results: As expected, we detected a clear signal for TH and DBH mRNA but no signal for PNMT mRNA. Both, single and repeated immobilization stress exposure increased significantly the gene expression of TH in A5 area. Maximal elevation in TH mRNA levels occurred after single immobilization for two hours and subsequent decapitation 24 hours later., Conclusions: In this study we detected for the first time the presence of DBH mRNA in micro dissected A5 cell group. We also showed how the gene expression of tyrosine hydroxylase changed with the function of time after the single immobilization exposure. Thus, TH mRNA in A5 cell group is modulated by immobilization stress in a time-dependent manner.

Published
2001

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