Étude d'un inhibiteur de la protéine anti-angiogénique thrombospondine-1 comme traitement de la prééclampsie chez la souris

Marc, Casandra

09 1900

Introduction : La prééclampsie (PE) est un trouble hypertensif caractérisé par une tension artérielle au-dessus de 140/90 mmHg et touche 2 à 8% des grossesses globalement. À ce jour, la plupart des médicaments ne peuvent traiter ou prévenir la PE. La thrombospondine-1 (THBS1) est un facteur anti-angiogénique et un activateur principal du TGF-β, ce qui pourrait également être impliqué dans l'altération de l'angiogenèse dans les placentas prééclamptiques. Objectif : Notre objectif est de décrire l'expression de la THBS1 et de tester l’effet d’un inhibiteur, le peptide LSKL, sur la vascularisation placentaire dans les placentas d'un modèle murin de PE (in vivo) et sur la capacité angiogénique des cellules endothéliales placentaires humaines (in vitro). Méthodes : L'expression de THBS1 a été mesurée dans les placentas de souris par western blot et dans les placentas humains par immunohistochimie (IHC). Des cellules endothéliales placentaires (pECs) extraites de placentas humains et des souris enceintes hétérozygotes femelles surexprimant la rénine et l’angiotensinogène humaines (hR+A+) sont traitées avec LSKL, ou son peptide témoin SLLK (cellules : 30 μmol/L pendant24h ; animal 129 μmol/mL s.c. au jour de gestation 14,5). Des pEC ont été soumises à des conditions contrôle (8% d’oxygène) ou hypoxie (0,5% d’oxygène) ou thrombine (10 unités/mL) pendant 24 h. L’angiogenèse cellulaire a été évaluée sur matrigel, les protéines évaluées par western blot et la localisation de la THBS1 ainsi que la vascularisation placentaire par IHC. Résultats : Le traitement avec LSKL augmente le nombre de tubes formées dans les pECs exposées à la thrombine ou à l’hypoxie. L’inhibiteur de la voie canonique du TGF-β, ALK5/Smad2/3 (SB-505124, SB), n’a pas modifié la capacité de formation de tubes, contrairement à l’inhibiteur de la voie non canonique, TAK1/p38 ((5Z) -7-oxozeaenol, (OXO) qui a réduit la capacité angiogénique (p<0,05). Chez le modèle de souris de PE, LSKL a significativement amélioré la vascularisation placentaire, évaluée par le contenu des cellules endothéliales CD31+ marquées par IHC (p<0,05), qui s’est accompagnée d’une phosphorylation réduite de TAK1 et ERK dans ce tissu. Conclusion : Nos résultats indiquent une augmentation de l’expression de la THBS1 dans les vaisseaux et cellules endothéliales placentaires des grossesses atteintes de PE, ainsi qu’un effet pro-angiogénique placentaire du LSKL par inhibition de la vie non-canonique du TGF-β. Ces résultats contribueront à identifier de nouvelles cibles thérapeutiques capables d'améliorer la vascularisation placentaire dans PE. / Introduction: Pre-eclampsia (PE) is a hypertensive disorder characterized by blood pressure above 140/90 mmHg and affects 2% to 8% of pregnancies globally. To date, most drugs cannot treat or prevent PE. Thrombospondin-1 (THBS1) is an anti-angiogenic factor and a major activator of TGF-β, which may also be involved in impaired angiogenesis in pre-eclamptic placentas. Objective: Our aim is to describe the expression of THBS1 and to test the effect of its inhibitor, LSKL peptide, on placental vascularization in placentas from a mouse model of PE (in vivo) and on the angiogenic capacity of human placental endothelial cells (in vitro). Methods: THBS1 expression was measured in placentas of mouse by western blot and in human placentas by immunohistochemistry (IHC). Placental endothelial cells (pECs) extracted from hu-man placentas and pregnant female heterozygous mice overexpressing human renin and angio-tensinogen (hR+A+) were treated with LSKL or its control peptide SLLK (cells: 30 μmol/L for 24h; animals: 129 μmol/mL subcutaneously on gestation day 14.5). pECs were subjected to control conditions (8% oxygen) or hypoxia (0.5% oxygen) or thrombin (10 units/mL) for 24 hours. Cellular angiogenesis was assessed on Matrigel, proteins were evaluated by western blot, and the locali-zation of THBS1 as well as placental vascularization were examined by immunohistochemistry (IHC). Results: Treatment with LSKL increased the number of tubes formed in pECs exposed to thrombin or hypoxia. The inhibitor of the canonical TGF-β pathway, ALK5/Smad2/3 (SB-505124, SB), did not alter tube formation capacity, unlike the inhibitor of the non-canonical pathway, TAK1/p38 ((5Z)-7-oxozeaenol, (OXO)), which reduced angiogenic capacity. In the mouse model of PE, LSKL significantly improved placental vascularization, assessed by CD31+ endothelial cell content marked by IHC, which was accompanied by reduced phosphorylation of TAK1 and ERK in this tissue. Conclusion: Our results indicate an increase in THBS1 expression in the vessels and placental endothelial cells of pregnancies affected by PE, as well as a pro-angiogenic effect of LSKL through the inhibition of the non-canonical TGF-β pathway. These findings contribute to identifying new therapeutic targets capable of improving placental vascularization in PE.

Prééclampsie

Hypertension

Angiogenèse

Vascularisation placentaire

Thrombospondine-1

TGF-β

Modèle animal

Cellules endothéliales placentaires

Preeclampsia

Angiogenesis

Placental vasculature

Thrombospondin-1

Animal model

Placental endothelial cells

PROFIBROTIC MACROPHAGE POLARIZATION AND REPROGRAMMING IN PRECISION CUT LUNG SLICES

Kumaran, Vaishnavi

January 2024

Idiopathic pulmonary fibrosis (IPF) is a progressive lung disease with worsening respiratory symptoms and physiological impairment. Pulmonary fibrosis is a chronic lung disease characterized by forming scar tissue (fibrosis) in the lungs. Alternatively activated macrophages (M2) known as pro-fibrotic are known to contribute to the fibrotic remodeling of the lung. In addition to the polarization of slices from naïve to pro-fibrotic, the addition of anti-fibrotic therapeutics reprogram slices back to a naïve condition. To polarize the slices, naïve slices are incubated with a previously investigated method in the lab known as the polarization cocktail. The polarization cocktail can be achieved by adding of IL-4, IL-6 and IL-13 to naïve(M0) slices in the Precision Cut lung slice (PCLS) model. For the therapeutic model, slices are incubated with the polarization cocktail and subsequently with the therapeutic. Our results have shown that the precision cut lung slice model can mimic previously investigated in-vivo experiments with the polarization cocktail. Secondly, the addition of therapeutics result in the slices exhibiting lower amounts of M2 markers and arginase activity concluding the model is suitable for the polarization and reprogramming of macrophages. / Thesis / Master of Science in Medical Sciences (MSMS)

Idiopathic pulmonary fibrosis

IPF

PCLS

Alternatively activated macrophage

M2

M1

Classically activated macrophage

Interstitial lung disease

Fibrotic lung disease

IHC

TGF-B

Beta-glucan

Microparticle

Yeast-Derived Beta Glucan

Ex vivo Models

Untersuchung der Differenzierungskapazität von Osteoblasten und Osteoblastensubpopulationen in vitro und ihre Beeinflussung durch verschiedene Wuchsfaktoren / In vitro differentiation potential of primary human osteoblasts subpopulations. Expression of adipocytic and osteoblastic markers

Ponce, María Laura

28 June 2005

No description available.

500 Naturwissenschaften allgemein

Mathematics and Computer Science

BMP

TGF

Osteoblasten

Adipozyten

Transdifferenzierung

Plastizität

alkalische Phosphatase

Osteokalzin

Osteoporose

Osteoblastendifferenzierung

primäre humane Osteoblasten

Coexpression

PPAR

LPL

BMP

TGF

osteoblasts

adipocytes

transdifferentiation

Plasticity

alkaline phosphatase

osteocalcin

Osteoporosis

osteoblastic markers

primary human osteoblasts

PPAR

LPL

42 Biologie

42.15 Zellbiologie

44 Medizin

44.68 Gerontologie

Geriatrie

44.37 Physiologie

44.03 Methoden und Techniken der Medizin

W Biologie

WH Cytologie

Histologie

Zellbiologie

Zellkultur

Zytologie

WH 100 Cytologische Methoden

WHF 200 Zelldifferenzierung

Zellstoffwechsel und -differenzierung

WHM 000 Cytohistochemie

Zyto-und Histochemie

Estudo da expressão da <font face=\"symbol\">a-actina de músculo liso em cultura de células de polpas dentárias e gengivas humanas tratadas com o fator de transformação de crescimento <font face=\"symbol\">b1(TGF-<font face=\"symbol\">b1). / Expression of <font face=\"symbol\">a-smooth muscle actin in cultured human dental pulp and gingival fibroblasts induced by transforming growth factor-<font face=\"symbol\">b1 (TGF-<font face=\"symbol\">b1).

Martinez, Elizabeth Ferreira

12 June 2008

Durante o processo de reparação tecidual, o fator de transformação de crescimento <font face=\"symbol\">b1 (TGF-<font face=\"symbol\">b1) apresenta um importante papel na regulação da expressão da <font face=\"symbol\">a-actina de músculo liso (<font face=\"symbol\">a-AML) e portanto, na diferenciação miofibroblástica. Como os fibroblastos pulpares apresentam características peculiares, com a expressão de proteínas específicas que os diferem de fibroblastos de outros tecidos conjuntivos, o presente estudo avaliou in vitro se o TGF-<font face=\"symbol\">b1 aumenta a expressão de <font face=\"symbol\">a-AML em fibroblastos pulpares humanos comparando-os com fibroblastos de gengiva. Para tal, diferentes doses de TGF-<font face=\"symbol\">b1 (5 à 10 ng/ml) foram adicionadas às culturas de células, sendo a expressão da <font face=\"symbol\">a-AML analisada por imunofluorescência e western-blotting. Ambos os tipos celulares imunoexpressaram <font face=\"symbol\">a-AML mesmo sem o tratamento com o TGF-<font face=\"symbol\">b1, estando aumentada consideravelmente, quando o TGF-<font face=\"symbol\">b1 foi adicionado às culturas. Os resultados do presente estudo demonstraram que o TGF-<font face=\"symbol\">b1 induz a expressão de <font face=\"symbol\">a-AML, sugerindo a indução do fenótipo miofibroblástico em fibroblastos pulpares. / Transforming growth factor-beta 1 (TGF-<font face=\"symbol\">b1) has been related to induce the expression of <font face=\"symbol\">a-smooth muscle actin (<font face=\"symbol\">a-SMA) in fibroblasts during repair. Since pulpal fibroblasts seem to be somewhat different from other fibroblasts, the present study investigated in vitro whether TGF-<font face=\"symbol\">b1 enhances the expression of <font face=\"symbol\">a-SMA in human pulpal fibroblasts. TGF-<font face=\"symbol\">b1 was added in doses between 5-10 ng/ml to cultures of both dental pulp and gingiva human fibroblasts. The expression of <font face=\"symbol\">a-SMA was analyzed by immunofluorescence and western-blotting. Both cell types were immunoreactive for <font face=\"symbol\">a-SMA even without TGF-<font face=\"symbol\">b1. When TGF-<font face=\"symbol\">b1 was added to cell cultures, the expression of <font face=\"symbol\">a-SMA increased dramatically in pulpal fibroblasts, independent of the concentration used. It was confirmed by the western blot analysis. The present findings showed that TGF-<font face=\"symbol\">b1 up-regulated the expression of <font face=\"symbol\">a-SMA thus inducing pulpal fibroblasts to acquire the myofibroblast phenotype.

Alfa-smooth muscle actin

Cell culture

Cultura celular

Fibroblastos de polpa

Human dental pulp

Miofibroblasto

Myofibroblast

Polpa dentária humana

Pulpal fibroblasts

Transforming growth

Exploration of the Cerebral Dysfunctions Induced by Arterial Rigidity and/or the Overexpression of TGFβ in a Mouse Model

Bloch, Sherri

06 1900

No description available.

TGF beta

behavioral testing

Morris Water Maze

Neurovascular coupling

Alzheimer's disease

Vascular dementia

Dementia

Neurovascular unit

Mouse model

Oxidative stress

Gliosis

Novel object recognition

Cerebral dysfunction

Calcification

Arterial rigidity

TGFβ

Rigidité artérielle

Démence

Alzheimer

Démence vasculaire

Piscine de Morris

Dysfunction cérébrale

Unité neurovasculaire

Lifestyle and Biological Risk Factors for Liver Fibrosis in the Miami Adult Studies on HIV (MASH) Cohort: An HIV Infected and HIV/HCV Co-infected Population

Stewart, Tiffanie S.

15 April 2016

Liver disease is now a leading cause of non-AIDS related morbidity and mortality in people living with HIV (PLWH). The present study investigated the interplay between adverse lifestyle factors that are prevalent in PLWH, biological mediators of liver pathogenesis, and a non-invasive measure of liver fibrosis (FIB-4 index) in HIV mono- and HIV/HCV co-infected individuals. The results of this investigation in the Miami Adult Studies of HIV (MASH) cohort show that the odds of liver fibrosis progression significantly increased over two years for HIV mono-infected participants who drank alcohol hazardously (OR 3.038, P=0.048), and had BMI ≥ 28kg/m2 (OR 2.934, P=0.027). Cocaine use reduced the odds of advancing one stage of liver fibrosis (OR 0.228, P=0.038), but an interaction between high BMI and cocaine use slightly raised the odds by 4.8% of liver fibrosis progression (P=0.072). HIV/HCV co-infected participants showed interactions between cocaine use and high BMI with increased FIB-4 stage (OR 4.985, P= 0.034), however no lifestyle factors could independently predict FIB-4 stage in this group. Biological mediators previously associated with liver pathogenesis were associated with higher FIB-4 index over 2 years in a subset of (n=65) HIV mono-infected participants. Plasma measures of oxidative stress (% oxidized glutathione: OR 4.342, P= 0.046), hepatocyte-specific apoptosis (Cytokeratin-18 (CK-18): OR 1.008, P=0.021), and microbial endotoxin (lipopolysaccharide (LPS): OR 1.098, P= 0.097) were associated with having higher odds of progressing at least one stage of FIB-4 over 2 years. The same biological mediators were also associated with liver fibrosis within HIV infected people who also had a harmful lifestyle characteristic. FIB-4 index was significantly associated with % oxidized glutathione in obese subjects (β=0.563, P=0.018), TGF-β1 in cocaine users (β=0.858, P=0.027), and CK-18 in HIV infected individuals without any adverse lifestyle factors (β=0.435, P=0.015). Taken together, the findings of these studies describe interrelationships between HIV disease status, lifestyle, and biological mediators of liver fibrosis. The results show interactions between lifestyle conditions and the mediators of liver fibrosis may account for higher rates of liver disease in HIV infection. Research is warranted to develop personalized therapeutics for PLWH to curb the burden of liver disease.

HIV infection

HIV/HCV co-infection

liver fibrosis

alcohol

AUDIT

cocaine

body mass index

FIB-4 index

oxidative stress

hepatocyte apoptosis

transforming growth factor-beta1

microbial endotoxin

malondialdehyde

glutathione

MDA

GSH

TGF-β1

CK-18

LPS

Community Health and Preventive Medicine

Dietetics and Clinical Nutrition

Hepatology

Medical Biochemistry

Medical Immunology

Medical Nutrition

Other Medical Sciences

Etiopathology Of Oral Submucous Fibrosis : Role Of Areca Nut Constituents And Transforming Growth Factor-β Signalling

Khan, Imran

07 1900

Oral Submucous Fibrosis (OSF) is a chronic inflammatory disease resulting in progressive fibrosis of the oral tissues that can cause difficulty in chewing, swallowing, speaking, and mouth opening. Epidemiological studies have shown that OSF is a precancerous condition and 2-8% of the OSF patients develop squamous cell carcinoma. This disease affects 0.5% of the population in the Indian subcontinent and is now a growing public health issue in many parts of the world. Habit of chewing betel quid has been proposed as an important etiological factor in the development of this disease and is coline, a principle alkaloid of areca nut is considered as major causative factor for OSF development. But the exact molecular mechanism of OSF pathogenesis is not known. Therefore, we set the following objectives for this study: 1) Gene expression profiling of OSF using microarray. 2) Role of areca nut constituents in OSF pathogenesis. 3) Effect of areca nut on epithelial and fibroblast cells. In order to delineate the possible molecular mechanism of OSF pathogenesis, we took microarray approach and identified differentially regulated genes in ten OSF tissues against eight pooled normals using whole human genome oligonucleotide arrays. Microarray results revealed differential expression of 5288 genes (p≤0.05 and Fold change≥1.5), among them 2884 were up-regulated and 2404 were down-regulated. Validation employing quantitative real-time PCR and immunohistochemistry confirmed up-regulation of transforming growth factor-β1 (TGF-β1), TGFBI, THBS1, SPP1, TIG1 and down-regulation of bone morphogenic protein 7 (BMP7), C4orf7 and ALOX12 in OSF tissues. Furthermore, activation of TGF-β pathway was evident in OSF tissues as demonstrated by p-SMAD2 strong immunoreactivity. Analysis of IHC data showed that in all the normal tissues and in 70% of the OSF tissues the expression of TGF-β and BMP7 are inversely correlated. In good correlation, treatment of keratinocytes (HaCaT) by TGF-βdown-regulated BMP7, while BMP7 expression could not be detected in fibroblast cells. Hence, the imbalance between TGF-βand BMP7 signalling, which are positive and negative modulators of extracellular matrix production, respectively may trigger the manifestation of OSF. We also studied the regulation few genes (CTGF, TGM2 and THBS1) identified in OSF microarray in response to TGF-βand arecoline. TGF-βwas able to induce all the above genes in both HaCaT and hGF cells but arecoline could only induce TGM2 in hGF and THBS1 in HaCaT. Therefore TGF-βpathway came out to be the most important pathway in OSF microarray and subsequent validations. But areca nut constituents responsible for TGF-βpathway activation and the source (epithelial or fibroblast cells) through which it activates TGF-βare not known. In an attempt to understand the role of areca nut and its constituents in inducing TGF-βsignalling in epithelial cells, we performed microarray on epithelial cells (HaCaT) treated with areca nut water extract. Surprisingly, 64% of the differentially regulated genes by areca nut water extract matched with TGF-βinduced gene expression profile. To find out areca nut induced genes through TGF-β, epithelial cells were treated with areca nut in presence of ALK5 (TβRI) inhibitor. Out of 64% differentially induced genes, 57% genes induced by areca nut got compromised in presence of ALK5 and 7% were independently induced by areca nut, highlighting the effect of areca nut via TGF-β. Accordingly, areca nut treatment induced both p-SMAD2 and TGF-βdownstream targets TGFBI, TGM2, TMEPAI and THBS1 in HaCaT cells. One possible mechanism of TGF-βsignalling induction by areca nut could be via induced ligand (TGF-β2) and its activator (THBS1). Induction of TGF-β2 ligand by areca nut was shown at both RNA (Real Time) and protein (ELISA) levels. To find out areca nut components responsible for inducing TGF-β signalling, areca nut fractionation was performed which gave three fractions namely, Ethyl acetate (polyphenol), water supernatant (alkaloids) and Dichloromethane (impurity). Out of these; polyphenol and alkaloid fractions were found to be responsible for the induction of TGF-β signalling and its downstream targets. Upon treatment with purified components, catechin and tannin of polyphenol fraction and arecoline, arecaidine and guvacine of alkaloid fraction were found to be responsible for inducing TGF-β signalling, as seen by increased appearance of phopho-SMAD2 in HaCaT cells. Areca nut treatment on human gingival fibroblast cells (hGF) did not induce TGF-β signalling, highlighting that the source of TGF-β induction by areca nut could possibly be the epithelium. Further treatment of areca nut along with TGF-β on hGF cells potentiated TGF-β effect both in terms of TGF-β downstream targets like TGFBI, TGM2, TMEPAI, COL1A1 etc and activation of fibroblast by inducing α-SMA. Increasing concentration of areca nut is cytotoxic on HaCaT cells and pro-proliferative on hGF cells. This could provide a possible explanation for epithelial atrophy and proliferating fibroblast cells in connective tissue of OSF patients. Further exploration on HaCaT cell cytotoxicity by areca nut suggests the involvement of Reactive Oxygen Species (ROS) as a key molecule induced by areca nut. Compromising ROS generation by NAC (N-Acetyl-L-Cysteine) led to reversal of Sub-G1 peak induced by areca nut in HaCaT cells. This highlighted that cell death caused by areca nut could be ROS mediated. Areca nut treatment on hGF cells did not induce ROS generation, leading to no cytotoxicity on these cells. A possible explanation of this differential ROS generation can be due to dose dependent suppression of Catalase activity by areca nut in HaCaT cells but not in hGF cells. We also compared cytotoxicity of areca nut with all the alkaloids and found a good match with arecoline as both of them induce ROS, apoptotic ladder formation, annexin V positivity, suppression of Catalase activity and the cell death induced by them was compromised by NAC. The above results indicated that arecoline could be a mediator of areca nut water extract cytotoxicity on HaCaT cells. Betel nut chewer’s oral epithelium gets regularly exposed to areca nut and hence this exposure could be cytotoxic to oral epithelial cells too. We performed Terminal deoxynucleotidyl transferase dUTP nick end labeling (TUNEL) in normal and OSF tissues. Our data showed 62.5% of OSF patients having significant percentage of epithelial cells with TUNEL positivity (Labeling index = 2-60%) compared to all normal tissues that were TUNEL negative. TUNEL positivity was predominantly seen in the upper keratin and supra basal layer of the epithelium. We also studied proliferation status of OSF epithelium and observed that 3-17% (LI) of epithelial cells in all normal tissues showed Ki-67 positivity in the germinal layer of epithelium. However, 65% of the OSF patients showed staining for Ki-67 (LI=.2-58%) in their epithelium. Also analysis of TUNEL positive and Ki-67 positive sections indicated that OSF patients with high TUNEL positivity have high Ki-67 labeling index, but stains in the supra basal or keratin layer (TUNEL) and basal layer (Ki-67) of epithelium respectively. This induced proliferation of epithelial cells could be the result of heavy apoptosis in the outer epithelium. But as these patients are regularly exposed to areca nut, this increased proliferation may not be able to cope up with the heavy apoptosis induced by areca nut, leading to atrophied epithelium. To understand the germinal status of OSF atrophied epithelium we performed staining for OCT4 in OSF tissues. To our surprise there were no OCT4 positive nuclei in the epithelium of 53% of OSF patients but a regular spread of OCT4 positivity has been seen in the epithelium of normal subjects. In conclusion, this thesis highlights the involvement of TGF-β pathway in OSF patho-physiology. In addition, activation of TGF-β pathway by areca nut constituents has been demonstrated. Moreover, the atrophied epithelium of OSF appears to be a consequence of apoptosis and stem cell deprivation. Taken together, areca nut perhaps causes atrophy of the epithelium and activates TGF-β pathway that may lead to manifestation of OSF.

Inflammatory Diseases

Oral Submucous Fibrosis (OSF)

Oral Submucous Fibrosis Pathogenesis

Fibroblast Cells

Areca Nut

Oral Submucous Fibrosis Microarray

Fibroblasts

Oral Submucous Pathogenesis

Oral Submucous Fibrosis Pathology

Human Gingival Fibroblast Cells (hGF)

TGF-β Pathway

Transforming Growth Factor Beta

Pathology

Estudo da expressão da <font face=\"symbol\">a-actina de músculo liso em cultura de células de polpas dentárias e gengivas humanas tratadas com o fator de transformação de crescimento <font face=\"symbol\">b1(TGF-<font face=\"symbol\">b1). / Expression of <font face=\"symbol\">a-smooth muscle actin in cultured human dental pulp and gingival fibroblasts induced by transforming growth factor-<font face=\"symbol\">b1 (TGF-<font face=\"symbol\">b1).

Elizabeth Ferreira Martinez

12 June 2008

Durante o processo de reparação tecidual, o fator de transformação de crescimento <font face=\"symbol\">b1 (TGF-<font face=\"symbol\">b1) apresenta um importante papel na regulação da expressão da <font face=\"symbol\">a-actina de músculo liso (<font face=\"symbol\">a-AML) e portanto, na diferenciação miofibroblástica. Como os fibroblastos pulpares apresentam características peculiares, com a expressão de proteínas específicas que os diferem de fibroblastos de outros tecidos conjuntivos, o presente estudo avaliou in vitro se o TGF-<font face=\"symbol\">b1 aumenta a expressão de <font face=\"symbol\">a-AML em fibroblastos pulpares humanos comparando-os com fibroblastos de gengiva. Para tal, diferentes doses de TGF-<font face=\"symbol\">b1 (5 à 10 ng/ml) foram adicionadas às culturas de células, sendo a expressão da <font face=\"symbol\">a-AML analisada por imunofluorescência e western-blotting. Ambos os tipos celulares imunoexpressaram <font face=\"symbol\">a-AML mesmo sem o tratamento com o TGF-<font face=\"symbol\">b1, estando aumentada consideravelmente, quando o TGF-<font face=\"symbol\">b1 foi adicionado às culturas. Os resultados do presente estudo demonstraram que o TGF-<font face=\"symbol\">b1 induz a expressão de <font face=\"symbol\">a-AML, sugerindo a indução do fenótipo miofibroblástico em fibroblastos pulpares. / Transforming growth factor-beta 1 (TGF-<font face=\"symbol\">b1) has been related to induce the expression of <font face=\"symbol\">a-smooth muscle actin (<font face=\"symbol\">a-SMA) in fibroblasts during repair. Since pulpal fibroblasts seem to be somewhat different from other fibroblasts, the present study investigated in vitro whether TGF-<font face=\"symbol\">b1 enhances the expression of <font face=\"symbol\">a-SMA in human pulpal fibroblasts. TGF-<font face=\"symbol\">b1 was added in doses between 5-10 ng/ml to cultures of both dental pulp and gingiva human fibroblasts. The expression of <font face=\"symbol\">a-SMA was analyzed by immunofluorescence and western-blotting. Both cell types were immunoreactive for <font face=\"symbol\">a-SMA even without TGF-<font face=\"symbol\">b1. When TGF-<font face=\"symbol\">b1 was added to cell cultures, the expression of <font face=\"symbol\">a-SMA increased dramatically in pulpal fibroblasts, independent of the concentration used. It was confirmed by the western blot analysis. The present findings showed that TGF-<font face=\"symbol\">b1 up-regulated the expression of <font face=\"symbol\">a-SMA thus inducing pulpal fibroblasts to acquire the myofibroblast phenotype.

Cultura celular

Fibroblastos de polpa

Miofibroblasto

Polpa dentária humana

Alfa-smooth muscle actin

Cell culture

Human dental pulp

Myofibroblast

Pulpal fibroblasts

Transforming growth

Modulation of Sodium Iodide Symporter-mediated Thyroidal Radioiodide Uptake by Small Molecule Inhibitors, Natural Plant-based Products and microRNAs

Lakshmanan, Aparna

27 May 2015

No description available.

Biomedical Research

Molecular Biology

Oncology

Thyroid cancer

Sodium Iodide Symporter

Radioactive iodide uptake

Akt

Akti1-2

Apigenin

p38MAPK

PKC-delta

PI3K

GDC-0941

Iodide efflux rate

MEK

Hsp90

BRAF

RET-PTC

TGF-beta

miR-339-5p

miR-195

Rottlerin

OSU-15

SREBP

Die Regulation des humanen Lipopolysaccharid bindenden Proteins (hLBP)

Hallatschek, Werner

26 January 2005

Das Lipopolysaccharid Bindende Protein (LBP) ist ein überwiegend in der Leber synthetisiertes Akutphaseprotein. Es bindet den Zellwandbestandteil Lipopolysaccharid (LPS) Gram-negativer Bakterien und transportiert es zu zellulären Rezeptoren, wodurch das angeborene Immunsystem aktiviert wird. In dieser Arbeit wird die Regulation der LBP-Expression in Interleukin (IL)-1, IL-6 und Dexamethason (Dex) stimulierten humanen Hepatomzelllinien HuH-7 und HepG2 untersucht. Der wichtigste Stimulator ist dabei IL-6, dessen Wirkung über die Transkriptionsfaktoren (TF) Stat-3, C/EBP-beta und AP-1 vermittelt wird. Für alle 3 TF konnten aktive Bindungsstellen auf dem LBP-Promotor nachgewiesen werden. Für IL-1-Effekte die u. a. über den TF NF-kappaB vermittelt werden, konnten ebenfalls aktive Bindungsstellen nachgewiesen werden. Die Wirkung von Dex wird über Glucocorticoid Responsive Elements (GREs) vermittelt. Auf dem LBP-Promotor befinden, sich wie gezeigt werden konnte, mehrere aktive GREs, wobei einige verstärkend und einige hemmend wirken. Eine zu beobachtende Synergiewirkung von Dex und IL-6 wird durch die Aufregulation des IL-6-Rezeptors durch Dex verursacht. Die LBP-Expression kann durch TGF (Transforming Growth Factor)-beta gehemmt werden. Der TGF-beta-Signalweg über Smads ist in den Hepatomzellen aktiv, vermittelt aber nicht den TGF-beta-Hemmeffekt, sondern eine geringe stimulierende Wirkung, die bei alleiniger TGF-beta-Inkubation auftritt. Die inhibierende Wirkung von TGF-beta wird durch Gfi-1- und AP-1-Bindungsstellen vermittelt. Die Gfi-1-Bindungsstelle nimmt dabei, wie hier erstmals gezeigt werden konnte, eine herausragende Stellung ein. Die Aufklärung der LBP-Regulation und dabei besonders die Hemmung der LBP-Expression kann mittelfristig dazu beitragen, den klinischen Verlauf von inflammatorischen und infektiösen Erkrankungen zu beeinflussen und bietet daher Potenzial für neue Therapieansätze. / Lipopolysaccharide (LPS) binding protein (LBP) is an acute phase protein with the ability to bind and transfer LPS of Gram-negative bacteria. This soluble pattern recognition molecule represents an important defense principle of the host. Regulation of the hepatic acute phase response and its termination are important mechanisms for limiting systemic inflammatory activity of the host. Here were analyze the cooperation of Interleukin (IL)-1, IL-6, and Dexamethasone (Dex) at LBP expression in the hepatoma cell lines HuH-7 and Hep G2. The major inducer of LBP expression is IL-6. Within the LBP promoter numerously highly consensus binding sites such as AP-1, C/EBP-beta? and STAT3 are present, that confer transcriptional activity as shown by truncation and mutation experiments. Additionally, activate NF-kappaB sites activated by IL-1 were detected at the LBP promoter. By mutation experiments of the promoter furthermore were found differentially active glucocorticoid response elements (GREs). The promoter contains GREs enhancing the activity as well as inhibitory ones. The enhancing effect towards LBP expression by Dex was mediated by IL-6. Dex stimulated the expression of the IL-6 receptor and therefore upregulated the IL-6 pathway. Transforming Growth Factor (TGF)-beta is able to inhibit LBP expression in stimulated cells. An AP-1 binding site was identified mediating inhibitory TGF-beta effects towards LBP promoter activity. Furthermore it was shown that a growth factor independence (Gfi)-1 binding site localized near the AP-1 site is essential for mediating the TGF-beta inhibitory effect. The relevancy of the Gfi-1 site fore mediating TGF-beta effects indicates a novel mechanism for understanding inhibitory TGF-beta effects at the transcriptional level. In summary the complex regulation of LBP were elucidate which may help to eventually develop novel intervention strategies for acute phase, sepsis, and septic shock.

LPS binding protein (LBP)

Lipopolysaccharid (LPS)

Interleukin-6 (IL-6)

Dexamethason (Dex)

Aktivatorprotein-1 (AP-1)

Nuclear factor kappa B (NF kappa B)

Glucocorticoid responsive element (GRE)

Growth factor independence-1 (Gfi-1)

LPS binding protein (LBP)

lipopolysaccharid (LPS)

interleukin-6 (IL-6)

dexamethasone (Dex)

activator protein-1 (AP-1)

nuclear factor kappa B (NF kappa B)

glucocorticoid responsive element (GRE)

growth factor independence-1 (Gfi-1)

570 Biowissenschaften, Biologie

32 Biologie

WF 9900

ddc:570