Your search keyword '"Seo Yoon Chang"' showing total 12 results

1. Activity control of autodisplayed proteins on the same outer membrane layer of E. coli by using Z-domain/streptavidin/and lipase/foldase systems

Author

Joachim Jose, Gu Yoo, Jae Chul Pyun, Misu Lee, Ji Hong Bong, Seo Yoon Chang, and Min Jung Kang

Subjects

0301 basic medicine, Streptavidin, Recombinant Fusion Proteins, Bioengineering, 02 engineering and technology, medicine.disease_cause, Applied Microbiology and Biotechnology, Biochemistry, 03 medical and health sciences, chemistry.chemical_compound, Protein Domains, Escherichia coli, medicine, Lipase, Surface plasmon resonance, biology, Cell Membrane, 021001 nanoscience & nanotechnology, 030104 developmental biology, chemistry, Foldase, biology.protein, Cell Surface Display Techniques, 0210 nano-technology, Bacterial outer membrane, Layer (electronics), Biosensor, Biotechnology

Abstract

The autodisplay technology has been applied for expression of a desired protein on the outer membrane (OM) of Escherichia coli. In this work, the OM fractions of E. coli with two autodisplayed proteins were separately prepared and mixed to demonstrate the feasibility of control over the ratio of two autodisplayed proteins. As the first model, Z-domain and streptavidin were autodisplayed, and their activities were tested by means of the combined OM layer in a 96-well microplate and a surface plasmon resonance (SPR) biosensor. As the second model, lipase and foldase were autodisplayed which required an interaction between two proteins to obtain the activity of lipase. The OM fractions of E. coli with an autodisplayed lipase and foldase were separately prepared and mixed to demonstrate the feasibility of control over the ratio of two autodisplayed proteins when the interaction of two proteins is required within the same OM layer for the activity of the lipase.

Published

2017

2. A magnetite suspension-based washing method for immunoassays using Escherichia coli cells with autodisplayed Z-domains

Author

Seo Yoon Chang, Jae Chul Pyun, Ji Hong Bong, Gu Yoo, Young Wook Chang, Min Jung Kang, Dohoon Kim, and Joachim Jose

Subjects

0301 basic medicine, Analyte, Bioengineering, Nanotechnology, 02 engineering and technology, medicine.disease_cause, Applied Microbiology and Biotechnology, Biochemistry, 03 medical and health sciences, chemistry.chemical_compound, Protein Domains, Suspensions, Limit of Detection, Escherichia coli, medicine, Centrifugation, Suspension (vehicle), Magnetite, Immunoassay, Detection limit, Chromatography, medicine.diagnostic_test, Immunomagnetic Separation, Chemistry, Autodisplay, Flow Cytometry, 021001 nanoscience & nanotechnology, Ferrosoferric Oxide, C-Reactive Protein, 030104 developmental biology, Cell Surface Display Techniques, 0210 nano-technology, Antibodies, Immobilized, Biotechnology

Abstract

Escherichia coli cells with autodisplayed Z-domains have been used for immunoassays of specific target analytes. In this study, a magnetite suspension was used for the washing step in immunoassays of E. coli cells with autodisplayed Z-domains. This approach enhanced the washing conditions for these immunoassays by determining (1) the optimal concentration of the magnetite suspension, (2) the capacity of the magnetite suspension-based washing method to recover E. coli cells, and (3) the level at which the activity of autodisplayed Z-domains is maintained. In immunoassays of C-reactive protein (CRP), the immunoassay incorporating the magnetite suspension-based washing method showed a sensitivity and limit of detection considerably higher than those of the conventional centrifugation-based washing method. The results indicated that immunoassays incorporating the magnetite suspension-based washing method are effective for medical diagnoses based on CRP assay.

Published

2016

3. Induction mechanism of lipocalin-2 expression by co-stimulation with interleukin-1β and interferon-γ in RINm5F beta-cells

Author

Myung-Jun Kim, Dong-Bin Kim, Seo-Yoon Chang, Yang-Hyeok Jo, and Seung Hyun Ko

Subjects

Interleukin-1beta, Molecular Sequence Data, Biophysics, Electrophoretic Mobility Shift Assay, Lipocalin, Biology, Real-Time Polymerase Chain Reaction, Biochemistry, Cell Line, Proinflammatory cytokine, Interferon-gamma, Islets of Langerhans, chemistry.chemical_compound, Lipocalin-2, Co-stimulation, Western blot, medicine, Animals, RNA, Messenger, Molecular Biology, Gene, Transcription factor, DNA Primers, Messenger RNA, Binding Sites, Base Sequence, medicine.diagnostic_test, NF-kappa B, NF-κB, Cell Biology, Molecular biology, Lipocalins, Rats, chemistry

Abstract

Lipocalin-2 (LCN-2) was known to play a role in obesity and insulin resistance, however, little is known about the expression of LCN-2 in pancreatic islet β-cells. We examined the molecular mechanisms by which proinflammatory cytokines interleukin-1β (IL-1β) and interferon-γ (IFN-γ) induce LCN-2 expression in RINm5F β-cells. IL-1β significantly induced LCN-2 expression while IFN-γ alone did not induce it. IFN-γ significantly potentiated IL-1β-induced LCN-2 protein and mRNA expression. However, promoter study and EMSA showed that IFN-γ failed to potentiate IL-1β-induced LCN-2 promoter activity and binding activity of transcription factors on LCN-2 promoter. Furthermore, LCN-2 mRNA stability and transcription factors NF-κB and STAT-1 were not involved in the stimulatory effect of IFN-γ on IL-1β-induced LCN-2 expression. Meanwhile, Western Blot and promoter analyses showed that NF-κB was a key factor in IL-1β-induced LCN-2 expression. Collectively, IL-1β induces LCN-2 expression via NF-κB activation in RINm5F β-cells. IFN-γ potentiates IL-1β-induced LCN-2 expression at mRNA and protein levels, but not at promoter level and the stimulatory effect of IFN-γ is independent of NF-κB and STAT-1 activation. These data suggest that LCN-2 may play a role in β-cell function under an inflammatory condition.

Published

2013

4. Exendin-4 inhibits iNOS expression at the protein level in LPS-stimulated Raw264.7 macrophage by the activation of cAMP/PKA pathway

Author

Yang-Hyeok Jo, Myung-Jun Kim, In-Kyung Jeong, Yu-Bae Ahn, Gyeong Ryul Ryu, Dong-Bin Kim, Seung Hyun Ko, and Seo-Yoon Chang

Subjects

Lipopolysaccharides, RNA Stability, Nitric Oxide Synthase Type II, Adenylate kinase, Cycloheximide, Biology, Nitric Oxide, Biochemistry, Gene Expression Regulation, Enzymologic, Glucagon-Like Peptide-1 Receptor, Cell Line, Mice, chemistry.chemical_compound, Enzyme Stability, Cyclic AMP, Receptors, Glucagon, Animals, Gene silencing, Electrophoretic mobility shift assay, Northern blot, Enzyme Inhibitors, Promoter Regions, Genetic, Receptor, 3' Untranslated Regions, Molecular Biology, Nitrites, Venoms, Macrophages, NF-kappa B, Cell Biology, Molecular biology, Enzyme Activation, IκBα, chemistry, Proteolysis, Dactinomycin, Exenatide, Phosphorylation, Imines, Peptides, Protein Binding

Abstract

Glucagon-like peptide-1 (GLP-1) and its potent agonists have been widely studied in pancreatic islet β-cells. However, GLP-1 receptors are present in many extrapancreatic tissues including macrophages, and thus GLP-1 may have diverse actions in these tissues and cells. Therefore, we examined the mechanism by which exendin-4 (EX-4), a potent GLP-1 receptor agonist, inhibits lipopolysaccharide (LPS)-induced iNOS expression in Raw264.7 macrophage cells. EX-4 significantly inhibited LPS-induced iNOS protein expression and nitrite production. However, Northern blot and promoter analyses demonstrated that EX-4 did not inhibit LPS-induced iNOS mRNA expression and iNOS promoter activity. Electrophoretic mobility shift assay (EMSA) showed that EX-4 did not alter the binding activity of NF-κB to the iNOS promoter. Consistent with the result of EMSA, LPS-induced IκBα phosphorylation and nuclear translocation of p65 were not inhibited by EX-4. Also, actinomycin D chase study and the promoter assay using the construct containing 3'-untranslated region of iNOS showed that EX-4 did not affect iNOS mRNA stability. Meanwhile, cycloheximide chase study demonstrated that EX-4 significantly accelerated iNOS protein degradation. The EX-4 inhibition of LPS-induced iNOS protein was significantly reversed by adenylate cyclase inhibitors (MDL-12330A and SQ 22536), a PKA inhibitor (H-89) and PKAα gene silencing. These findings suggest that EX-4 inhibited LPS-induced iNOS expression at protein level, but not at transcriptional mechanism of iNOS gene and this inhibitory effect of EX-4 was mainly dependent on cAMP/PKA system.

Published

2013

5. The level of nitric oxide regulates lipocalin-2 expression under inflammatory condition in RINm5F beta-cells

Author

Myung-Jun Kim, Seo-Yoon Chang, Dong-Bin Kim, Seung Hyun Ko, Yang-Hyeok Jo, and Hyun-Jong Jang

Subjects

0301 basic medicine, Cell Survival, Interleukin-1beta, Biophysics, 030209 endocrinology & metabolism, Apoptosis, Protein degradation, Biology, Nitric Oxide, Biochemistry, Nitric oxide, Proinflammatory cytokine, Cell Line, 03 medical and health sciences, chemistry.chemical_compound, Interferon-gamma, 0302 clinical medicine, Lipocalin-2, Insulin-Secreting Cells, MG132, medicine, Animals, Viability assay, RNA, Messenger, Molecular Biology, Inflammation, Cell Biology, Molecular biology, Rats, Nitric oxide synthase, 030104 developmental biology, chemistry, Gene Expression Regulation, Proteasome inhibitor, biology.protein, medicine.drug

Abstract

We previously reported that proinflammatory cytokines (interleukin-1β and interferon-γ) induced the expression of lipocalin-2 (LCN-2) together with inducible nitric oxide synthase (iNOS) in RINm5F beta-cells. Therefore, we examined the effect of nitric oxide (NO) on LCN-2 expression in cytokines-treated RINm5F beta-cells. Additionally, we observed the effect of LCN-2 on cell viability. First, we found the existence of LCN-2 receptor and the internalization of exogenous recombinant LCN-2 peptide in RINm5F and INS-1 beta-cells. Next, the effects of NO on LCN-2 expression were evaluated. Aminoguanidine, an iNOS inhibitor and iNOS gene silencing significantly inhibited cytokines-induced LCN-2 expression while sodium nitroprusside (SNP), an NO donor potentiated it. Luciferase reporter assay showed that transcription factor NF-κB was not involved in LCN-2 expression. Both LCN-2 mRNA and protein stability assays were conducted. SNP did not affect LCN-2 mRNA stability, however, it significantly reduced LCN-2 protein degradation. The LCN-2 protein degradation was significantly attenuated by MG132, a proteasome inhibitor. Finally, the effect of LCN-2 on cell viability was evaluated. LCN-2 peptide treatment and LCN-2 overexpression significantly reduced cell viability. FACS analysis showed that LCN-2 induced the apoptosis of the cells. Collectively, NO level affects LCN-2 expression via regulation of LCN-2 protein stability under inflammatory condition and LCN-2 may reduce beta-cell viability by promoting apoptosis.

Published

2016

6. Effects of physiological quercetin metabolites on interleukin-1β-induced inducible NOS expression

Author

Dong-Bin Kim, Jae Min Cho, Myung-Jun Kim, Paul W. Needs, Seo-Yoon Chang, and Yang-Hyeok Jo

Subjects

Endocrinology, Diabetes and Metabolism, Interleukin-1beta, Clinical Biochemistry, Nitric Oxide Synthase Type II, Biochemistry, Gene Expression Regulation, Enzymologic, Nitric oxide, Islets of Langerhans, chemistry.chemical_compound, Insulin Secretion, Gene expression, medicine, Animals, Insulin, heterocyclic compounds, Phosphorylation, Promoter Regions, Genetic, Molecular Biology, Cells, Cultured, Nitrites, Isorhamnetin, Regulation of gene expression, Nutrition and Dietetics, biology, Pancreatic islets, NF-kappa B, Molecular biology, Rats, Nitric oxide synthase, IκBα, medicine.anatomical_structure, chemistry, biology.protein, I-kappa B Proteins, Quercetin

Abstract

Cytokines released by inflammatory cells around the pancreatic islets are implicated in the pathogenesis of diabetes mellitus. Specifically, interleukin-1β (IL-1β) is known to be involved in islet β-cell damage by activation of nuclear factor-κB (NF-κB)-mediated inducible nitric oxide synthase (iNOS) gene expression. Though most flavonoids are shown to have various beneficial effects, little is known about the anti-inflammatory effects of their metabolites. Therefore, we investigated the effects of quercetin and its metabolites quercetin 3'-sulfate, quercetin 3-glucuronide and isorhamnetin 3-glucuronide on IL-1β-stimulated iNOS gene expression in RINm5F β-cells. The nitrite level, iNOS protein and its mRNA expression levels and iNOS promoter activity were measured. In addition, IκBα protein phosphorylation, nuclear translocation of nuclear factor-κB (NF-κB) and NF-κB DNA binding activity were determined. Adenosine 5'-triphosphate disodium salt-induced insulin release was also measured. Quercetin significantly reduced IL-1β-induced nitrite production, iNOS protein and its mRNA expression levels, and it also inhibited IL-1β-induced IκBα phosphorylation, NF-κB activation and iNOS promoter activity. Additionally, quercetin significantly restored the inhibition of insulin secretion by IL-1β. Meanwhile, quercetin metabolites did not show any effect on IL-1β-induced iNOS gene expression and also on insulin secretion. Therefore, in terms of iNOS expression mechanism, dietary ingestion of quercetin is unlikely to show anti-inflammatory effects in rat islet β-cells exposed to IL-1β.

Published

2012

7. Inhibition of trichostatin A-induced antiangiogenesis by small-interfering RNA for thrombospondin-1

Author

Susie Hong, Seo-Yoon Chang, Soo-A Kim, Jung Hoon Kang, and Kyong-Ja Hong

Subjects

endocrine system, Small interfering RNA, Angiogenesis, viruses, Clinical Biochemistry, Neovascularization, Physiologic, Angiogenesis Inhibitors, Biology, Hydroxamic Acids, Biochemistry, Cell Line, Thrombospondin 1, Cell Movement, immune system diseases, medicine, Animals, Humans, RNA, Messenger, RNA, Small Interfering, Molecular Biology, Tube formation, Messenger RNA, Neovascularization, Pathologic, organic chemicals, Endothelial Cells, virus diseases, Cell migration, Trichostatin A, Tumor progression, Cancer research, Molecular Medicine, Cattle, medicine.drug

Abstract

Expression of thrombospondin-1 (TSP-1), which is a known inhibitor of tumor growth and angiogenesis, is reciprocally regulated by positive regulators, such as VEGF. Additionally, trichostatin A (TSA) suppresses tumor progression by altering VEGF levels and VEGF-mediated signaling. Thus, understanding TSA-regulated TSP-1 expression and the effects of altered TSP-1 levels might provide insights into the mechanism of action of TSA in anti-tumorigenesis, and provide an approach to cancer therapy. Here, we examined the effect of TSA on TSP-1 expression, and the effects of TSA-induced TSP-1 on cell motility and angiogenesis, in HeLa and bovine aortic endothelial cells. TSA remarkably increased TSP-1 expression at the mRNA and protein levels, by controlling the TSP-1 promoter activity. Both TSA and exogenous TSP-1 reduced cell migration and capillary-like tube formation and these activities were confirmed by blocking TSP-1 with its neutralizing antibody and small-interfering RNA. Our results suggest that TSP-1 is a potent mediator of TSA-induced anti- angiogenesis.

Published

2007

8. Molecular mechanisms of early growth response protein-1 (EGR-1) expression by quercetin in INS-1 beta-cells

Author

Dong-Bin Kim, Jae Min Cho, Myung-Jun Kim, Seung Hyun Ko, Yang-Hyeok Jo, Hyun-Jong Jang, and Seo-Yoon Chang

Subjects

MAP Kinase Signaling System, p38 mitogen-activated protein kinases, Glutamate-Cysteine Ligase, Response element, Molecular Sequence Data, Gene Expression, Biology, Biochemistry, p38 Mitogen-Activated Protein Kinases, Cell Line, Insulin-Secreting Cells, Serum response factor, Animals, heterocyclic compounds, Electrophoretic mobility shift assay, RNA, Messenger, RNA, Small Interfering, Promoter Regions, Genetic, Molecular Biology, Early Growth Response Protein 1, Messenger RNA, Base Sequence, Cell Biology, Transfection, Serum Response Element, Molecular biology, Cyclic AMP-Dependent Protein Kinases, Rats, body regions, GCLC, Gene Knockdown Techniques, Quercetin, hormones, hormone substitutes, and hormone antagonists

Abstract

Early growth response-1 (EGR-1), one of immediate early response genes, is involved in diverse cellular response. We recently reported that quercetin increased catalytic subunit of γ-glutamylcysteine ligase (GCLC) via the interaction of EGR-1 to GCLC promoter in INS-1 beta-cells. Therefore, this study investigated molecular mechanisms of quercetin-induced EGR-1 expression in INS-1 cells. Quercetin significantly induced EGR-1 protein and its mRNA expressions. This induction of EGR-1 was completely blocked by pretreatment with a PKA inhibitor, H89 and partially blocked by a p38 inhibitor, SB203580. Additionally, the siRNA-mediated inhibition of PKAα and p38 resulted in significant reduction of quercetin-induced EGR-1 promoter activity. Also, quercetin-induced EGR-1 protein expression was significantly decreased in the cells transfected with PKAα siRNA. Study using truncated EGR-1 promoter constructs showed that serum response element (SRE) sites, not cAMP response element site, were essential for EGR-1 transcription. However, electrophoretic mobility shift assay showed that quercetin did not affect the band intensity of DNA-protein complex on SRE site of EGR-1 promoter. Also, immune-shift assay using serum response factor (SRF) and phospho-SRF antibodies showed no difference between control and quercetin-treated groups. Collectively, quercetin-induced EGR-1 expression is largely dependent on PKA and partly on p38 MAPK pathway, and SRE sites of EGR-1 promoter are involved in quercetin-induced EGR-1 transcriptional activity.

Published

2011

9. Quercetin-induced upregulation of human GCLC gene is mediated by cis-regulatory element for early growth response protein-1 (EGR1) in INS-1 beta-cells

Author

Myung-Jun Kim, Seung Hyun Ko, Seong Su Lee, Yong-Moon Park, Hyun-Jong Jang, Dong-Bin Kim, Yang-Hyeok Jo, Jung-Hoon Kang, Jae Min Cho, Paul W. Needs, and Seo-Yoon Chang

Subjects

endocrine system, Sp1 Transcription Factor, Glutamate-Cysteine Ligase, Nitric Oxide Synthase Type II, Biology, Regulatory Sequences, Nucleic Acid, Biochemistry, Antioxidants, Transactivation, Insulin-Secreting Cells, Animals, Humans, Insulin, heterocyclic compounds, Electrophoretic mobility shift assay, RNA, Messenger, Binding site, Molecular Biology, Early Growth Response Protein 1, Messenger RNA, Promoter, Cell Biology, Molecular biology, Rats, Up-Regulation, DNA binding site, GCLC, Regulatory sequence, Quercetin

Abstract

The catalytic subunit of gamma-glutamylcysteine ligase (GCLC) catalyses the rate-limiting step in the de novo synthesis of glutathione (GSH), which is involved in maintaining intracellular redox balance. GSH is especially important for antioxidant defense system since beta-cells show intrinsically low expression of antioxidant enzymes. In the present study, we investigated the regulatory mechanisms by which quercetin, a flavonoid, induces the expression of the GCLC gene in rat pancreatic beta-cell line INS-1. Promoter study found that the proximal GC-rich region (from -90 to -34) of the GCLC promoter contained the quercetin-responsive cis-element(s). The quercetin-responsive region contains consensus DNA binding site for early growth response 1 (EGR1) at -67 (5'-CGCCTCCGC-3') which overlaps with a putative Sp1 binding site. Electrophoretic mobility shift assay showed that an oligonucleotide containing the EGR1 site was bound to nuclear factors EGR1, Sp1, and Sp3. In the promoter analysis, mutation of EGR1 site significantly reduced the quercetin response, whereas mutation of Sp1 site decreased only the basal activity of the GCLC promoter. Additionally, the transient overexpression of EGR1 significantly increased basal activity of the GCLC promoter. Finally, we showed that quercetin potently induced both EGR1 mRNA and its protein levels without affecting the expression of Sp1 and Sp3 proteins. Therefore, we concluded that EGR1 was bound to GC-rich region of the GCLC gene promoter, which was prerequisite for the transactivation of the GCLC gene by quercetin.

Published

2009

10. Exendin-4 induction of Egr-1 expression in INS-1 beta-cells: interaction of SRF, not YY1, with SRE site of rat Egr-1 promoter

Author

Seo-Yoon Chang, Yang-Hyeok Jo, Myung Suk Kim, Seung Hyun Ko, Myung-Jun Kim, Hyun-Jong Jang, In-Kyung Jeong, Gyeong Ryul Ryu, and Jung-Hoon Kang

Subjects

Serum Response Factor, Transcription, Genetic, Electrophoretic Mobility Shift Assay, Biology, CREB, Response Elements, Biochemistry, Cell Line, Transcription (biology), Insulin-Secreting Cells, Serum response factor, Cyclic AMP, Animals, RNA, Messenger, Extracellular Signal-Regulated MAP Kinases, Molecular Biology, Transcription factor, YY1 Transcription Factor, Early Growth Response Protein 1, Messenger RNA, Kinase, Venoms, MEK inhibitor, Cell Biology, Molecular biology, Rats, body regions, Gene Expression Regulation, biology.protein, Phosphorylation, Exenatide, Peptides, hormones, hormone substitutes, and hormone antagonists

Abstract

Glucagon-like peptide-1 (GLP-1) induces several immediate early response genes such as c-fos, c-jun, and early growth response-1 (Egr-1), which are involved in cell proliferation and differentiation. We recently reported that exendin-4 (EX-4), a potent GLP-1 agonist, upregulated Egr-1 expression via phosphorylation of CREB, a transcription factor in INS-1 β-cells. This study was designed to investigate the role of another transcription factors, serum response factor (SRF) and Yin Yang-1 (YY1), in EX-4-induced Egr-1 expression. EX-4 significantly increased Egr-1 mRNA and subsequently its protein level. EX-4-induced Egr-1 expression was inhibited by pretreatment with a PKA inhibitor, H-89, and an MEK inhibitor, PD 98059. The siRNA-mediated inhibition of PKA and ERK1 resulted in significant reduction of EX-4-induced Egr-1 expression. Promoter analyses showed that SRE clusters were essential for Egr-1 transcription, and YY1 overexpression did not affect Egr-1 promoter activity. EMSA results demonstrated that EX-4-induced transient increase in DNA–protein complex on SRE site, and that both SRF and phospho-SRF were bound to this site. Treatment of either YY1 consensus oligonucleotide or YY1 antibody did not effect the change of density or migration of the DNA–protein complex. Collectively, EX-4-induced Egr-1 expression is largely dependent on cAMP-mediated extracellular signal-regulated kinase activation, and EX-4 induces Egr-1 transcription via the interaction of SRF and phospho-SRF to SRE sites. J. Cell. Biochem. 104: 2261–2271, 2008. © 2008 Wiley-Liss, Inc.

Published

2008

11. CCAAT box is required for the induction of human thrombospondin-1 gene by trichostatin A

Author

Jung-Hoon Kang, Yang-Hyeok Jo, Myung-Jun Kim, Seo-Yoon Chang, Sang Soo Sim, and Myung Suk Kim

Subjects

CAAT box, Angiogenesis Inhibitors, Hydroxamic Acids, Biochemistry, Thrombospondin 1, Histone H3, medicine, Humans, Electrophoretic mobility shift assay, RNA, Messenger, Promoter Regions, Genetic, Molecular Biology, Transcription factor, biology, Cell Biology, Molecular biology, Histone Deacetylase Inhibitors, Histone, Trichostatin A, CCAAT-Binding Factor, Gene Expression Regulation, biology.protein, Histone deacetylase, Chromatin immunoprecipitation, medicine.drug, HeLa Cells

Abstract

Histone deacetylase (HDAC) inhibitors have been reported to inhibit angiogenesis as well as tumor growth. Thrombospondin-1 (TSP1) has been recognized as a potent inhibitor of angiogenesis. Such an action of TSP1 may account for the effect of HDAC inhibitors. In the present study, we investigated the molecular mechanism by which trichostatin A, a HDAC inhibitor, induces the expression of TSP1 gene. Trichostatin A increased both mRNA and protein levels of TSP1 in HeLa cells. Promoter and actinomycin D chase assays showed that trichostatin A-induced TSP1 expression was regulated at the transcriptional level without changing mRNA stability. CCAAT box on the TSP1 promoter was found to primarily mediate the trichostatin A response by deletion and mutation analyses of the TSP1 promoter. Electrophoretic mobility shift assay indicated that CCAAT-binding factor (CBF) was specifically bound to the CCAAT box of TSP1 promoter. Moreover, chromatin immunoprecipitation assay showed that trichostatin A increased the binding of acetylated form of histone H3 to the CCAAT box region of TSP1 promoter. Taken together, these results strongly suggest that trichostatin A activates the transcription of TSP1 gene through the binding of transcription factor CBF to CCAAT box and the enhanced histone acetylation. Thus, the present study provides the clue that the inhibition of angiogenesis by trichostatin A is accomplished through the upregulation of TSP1, the anti-angiogenic factor.

Published

2008

12. Weakening of the repressive YY-1 site on the thrombospondin-1 promoter via c-Jun/YY-1 interaction

Author

Dong-Hoon Yeom, Seo-Yoon Chang, Kyong-Ja Hong, Soo-A Kim, Soo-Jong Um, and Jung-Hoon Kang

Subjects

Proto-Oncogene Proteins c-jun, Clinical Biochemistry, Repressor, Down-Regulation, Electrophoretic Mobility Shift Assay, Biology, Biochemistry, Thrombospondin 1, Genes, Reporter, Cell Line, Tumor, Gene expression, Humans, Nucleotide, Luciferase, Electrophoretic mobility shift assay, Binding site, Nuclear protein, Luciferases, Promoter Regions, Genetic, Molecular Biology, Transcription factor, YY1 Transcription Factor, Sequence Deletion, chemistry.chemical_classification, Binding Sites, Molecular biology, DNA-Binding Proteins, Repressor Proteins, Transcription Factor AP-1, chemistry, Molecular Medicine, Erythroid-Specific DNA-Binding Factors, Transcription Factors

Abstract

Thrombospondin-1 (TSP-1) level is tightly regulated at the transcriptional level. To determine the detailed molecular mechanisms of TSP-1 expression, nine serial 5'-deletion constructs of the human genomic tsp-1 promoter (nucleotides -2,220 to +756) were prepared, inserted into luciferase reporter plasmids, and transiently transfected into the Hep3B human hepatocarcinoma cell. Among the nine 5'-deletion constructs, pTSP-Luc-4 (-767 approximately +756) had consistently decreased luciferase activity with or without PMA stimulation, whereas a further truncated construct [pTSP-Luc-4' (-407 approximately +756)] had increased levels of expression. By searching the nucleotides from -767 to -407, a consensus binding sequence (5'-CCATTTT-3') for the repressor Yin Yang-1 (YY-1) at nucleotide -440 was identified. The suppression induced by this site was weakened in the presence of the region upstream of nucleotide -767 (pTSP-Luc-1 and -2). Nuclear protein directly bound to an oligonucleotide containing the repressive YY-1 sequence but the binding capacity of the sequence was decreased by the increased c-Jun levels. Moreover, proteins immunoprecipitated with anti-YY-1 revealed an interaction between c-Jun and YY-1 factor. These data suggest that the repressive YY-1 site of the tsp-1 promoter could not be functional via activating positive cis-elements on the upstream from this site and weakened via c-Jun/YY-1 interactions.

Published

2004