Functional Consequences of Matrix Metalloproteinase-1 Over-Expression in Human Gliomas

Mullet, Emily

01 January 2006

Malignant brain tumors are among the deadliest of human cancers. Despit recent advancements in conventional therapies, glioblastomas remain incurable, largel y due to their ability to invade surrounding tissue. Matrix metalloproteinases are thought to contribute to the invaseive phenotype of human gliomas. Absent in normal brain, matrix metalloproteinase-1 (MMP-1) has been shown to be present in gliomas, and in particular in glioblastoma multiforme (GBM). To begin to examine the role of MMP-1 in these tumore, two human glioma cell lines were stably transfected with MMP-1 cDNA. Confirmation of MMP-1 over-expression in these cells was achieved through real-time PCR and Western blot analysis. The functional consequences of MMP-1 over-expression were analyzed using a collagen type-I invasion assay along with clonogenic and ATP viability assays. Data presented demonstrate that MMP-1 over-expressing cells were more invasive in both cell types and interestingly more clonogenic in on of the glioma cell lines, supporting a possible role for MMP-1 in glioma growth and invasion.

MMP-1

GBM

matrix metalloproteinases

brain tumor

Life Sciences

Physiology

"Efeito da terapia com laser em baixa intensidade (LILT) na produção de proteínas por macrófagos estimulados por cimentos endodônticos" / Effect of low level laser therapy (LILT) on the protein secretion by endodontic sealers stimulated macrophages

Sousa, Lorena Ribeiro de

08 March 2006

A terapia endodôntica visa o selamento biológico do complexo sistema apical, contribuindo para isso, as substâncias usadas no tratamento e a resposta imune do paciente. A LILT tem mostrado atividade antiinflamatória, favorecendo o processo reparacional. Sendo assim, este trabalho objetivou analisar o efeito da LILT na atividade secretória de macrófagos, previamente ativados por IFN-? e LPS de E.coli, e estimulados por substâncias liberadas de três tipos de cimentos endodônticos, um a base de óxido de zinco e eugenol, outro a base de hidróxido de cálcio e um terceiro resinoso. A citotoxicidade dessas substâncias foi avaliada usando a técnica de análise do MTT. Macrófagos ativados foram estimulados por essas substâncias ou não (controle) e então, irradiados ou não (controle) e a secreção de proteínas próinflamatórias (interleucina-1 b, fator de necrose tumoral-a e metaloproteinase da matriz-1) foram analisadas pelo teste ELISA. As irradiações foram realizadas com um laser GaAlAs (780 nm, 70 mW, ponta da fibra de 4 mm2, 1.67 seg, 3 J/cm2). Foram usadas duas aplicações de irradiação com intervalo de 6 h. Os dados obtidos foram tratados por Análise de Variância, quando de distribuição normal, ou teste de Friedman, quando de distribuição não normal, com nível de significância de 5 % (p = 0,05). A viabilidade dos controles e células tratados pelos cimentos endodônticos foi similar. Produção de IL-1 b e TNF-a foram observadas. Houve alta produção de MMP-1. Entretanto, sem diferenças estatísticas entre os grupos experimentais. Os grupos irradiados apresentaram resultados similares aos não irradiados. Substâncias liberadas pelos cimentos endodônticos testados não se mostraram citotóxicas nas condições deste experimento. Essas substâncias, bem como a LILT, no parâmetro utilizado, não causam alteração na atividade de secreção de MMP-1, IL-1 b e TNF-a por macrófagos ativados. / The endodontic therapy seeks the dental root canal biological sealing, depending on substances used in this process and patient’s defense immune factors. LILT has shown an anti-inflammatory activity, improving the periapical repair process. This in vitro study aimed to analyze the effect of LILT at the secretory activity of macrophages previously activated by interferon-gamma and lypopolisaccharide from E.coli, and stimulated by substances leached from three endodontic sealers (zinc oxide-eugenol based, resinous and calcium hydroxide-based). Cytotoxicity of these substances was assessed by the MTT test. Activated macrophages were stimulated by the substances or not (control) and then, irradiated or not (control) and the secretion of pro-inflammatory proteins (interleukin-1 b, tumor necrosis factor-a and matrix metalloproteinase-1) was analyzed by ELISA test. The LILT was performed using a GaAlAs laser (780 nm, 70 mW, focal spot of 4.0 mm2, 1.67 sec, 3 J/cm2). Two irradiations with 6 h-intervals were done. The data was compared by either ANOVA test or Friedman’s test. The cell viabilities of controls and cells treated by the sealers were similar. Production of IL -1 b and TNF-a were observed. There was a high production of MMP-1. However, statistical differences were not observed amongst the groups. The irradiated groups presented results similar to those of non irradiated groups. Substances leached from the endodontic sealers are non cytotoxic at these experiments conditions . These substances, as well as the LILT, at the parameter used, were not able to change the secretion of MMP-1, IL-1 b e TNF-a by activated macrophages.

Cimentos Endodônticos

endodontic sealers

IFN-?

IL-1 b

LILT

LILT

LPS

Macrófagos

Macrophages

MMP-1 IL-1 b

MMP-1 IL-1 b

TNF-a

TNF-a

"Efeito da terapia com laser em baixa intensidade (LILT) na produção de proteínas por macrófagos estimulados por cimentos endodônticos" / Effect of low level laser therapy (LILT) on the protein secretion by endodontic sealers stimulated macrophages

Lorena Ribeiro de Sousa

08 March 2006

A terapia endodôntica visa o selamento biológico do complexo sistema apical, contribuindo para isso, as substâncias usadas no tratamento e a resposta imune do paciente. A LILT tem mostrado atividade antiinflamatória, favorecendo o processo reparacional. Sendo assim, este trabalho objetivou analisar o efeito da LILT na atividade secretória de macrófagos, previamente ativados por IFN-? e LPS de E.coli, e estimulados por substâncias liberadas de três tipos de cimentos endodônticos, um a base de óxido de zinco e eugenol, outro a base de hidróxido de cálcio e um terceiro resinoso. A citotoxicidade dessas substâncias foi avaliada usando a técnica de análise do MTT. Macrófagos ativados foram estimulados por essas substâncias ou não (controle) e então, irradiados ou não (controle) e a secreção de proteínas próinflamatórias (interleucina-1 b, fator de necrose tumoral-a e metaloproteinase da matriz-1) foram analisadas pelo teste ELISA. As irradiações foram realizadas com um laser GaAlAs (780 nm, 70 mW, ponta da fibra de 4 mm2, 1.67 seg, 3 J/cm2). Foram usadas duas aplicações de irradiação com intervalo de 6 h. Os dados obtidos foram tratados por Análise de Variância, quando de distribuição normal, ou teste de Friedman, quando de distribuição não normal, com nível de significância de 5 % (p = 0,05). A viabilidade dos controles e células tratados pelos cimentos endodônticos foi similar. Produção de IL-1 b e TNF-a foram observadas. Houve alta produção de MMP-1. Entretanto, sem diferenças estatísticas entre os grupos experimentais. Os grupos irradiados apresentaram resultados similares aos não irradiados. Substâncias liberadas pelos cimentos endodônticos testados não se mostraram citotóxicas nas condições deste experimento. Essas substâncias, bem como a LILT, no parâmetro utilizado, não causam alteração na atividade de secreção de MMP-1, IL-1 b e TNF-a por macrófagos ativados. / The endodontic therapy seeks the dental root canal biological sealing, depending on substances used in this process and patient’s defense immune factors. LILT has shown an anti-inflammatory activity, improving the periapical repair process. This in vitro study aimed to analyze the effect of LILT at the secretory activity of macrophages previously activated by interferon-gamma and lypopolisaccharide from E.coli, and stimulated by substances leached from three endodontic sealers (zinc oxide-eugenol based, resinous and calcium hydroxide-based). Cytotoxicity of these substances was assessed by the MTT test. Activated macrophages were stimulated by the substances or not (control) and then, irradiated or not (control) and the secretion of pro-inflammatory proteins (interleukin-1 b, tumor necrosis factor-a and matrix metalloproteinase-1) was analyzed by ELISA test. The LILT was performed using a GaAlAs laser (780 nm, 70 mW, focal spot of 4.0 mm2, 1.67 sec, 3 J/cm2). Two irradiations with 6 h-intervals were done. The data was compared by either ANOVA test or Friedman’s test. The cell viabilities of controls and cells treated by the sealers were similar. Production of IL -1 b and TNF-a were observed. There was a high production of MMP-1. However, statistical differences were not observed amongst the groups. The irradiated groups presented results similar to those of non irradiated groups. Substances leached from the endodontic sealers are non cytotoxic at these experiments conditions . These substances, as well as the LILT, at the parameter used, were not able to change the secretion of MMP-1, IL-1 b e TNF-a by activated macrophages.

Cimentos Endodônticos

IFN-?

IL-1 b

LILT

LPS

Macrófagos

MMP-1 IL-1 b

TNF-a

endodontic sealers

LILT

Macrophages

MMP-1 IL-1 b

TNF-a

FUNCTION AND REGULATION OF MATRIX METALLOPROTEINASE-1 IN GLIOBLASTOMA MULTIFORME

Anand, Monika

29 July 2010

Glioblastoma Multiforme (GBM) is an aggressive and fatal cancer of the brain. It is characterized with augmented morbidity and elusion to therapies due in part to the incessant infiltration and spread of tumor cells in normal brain. We investigated the function of Matrix metalloproteinase-1, an important enzyme noted to be responsible for invasion in other cancers, in GBM and its regulation by epidermal growth factor receptor (EGFR) signaling. Previous studies from our laboratory demonstrated elevated levels of MMP-1 in GBM. Further studies indicated the involvement of MMP-1 in GBM invasion. The GBM cell lines T98G, U251MG and U87MG were used for this study. In T98G cell lines, inhibition of MMP-1 by siRNA significantly suppressed basal in vitro invasion without impacting cell viability. The over-expression of MMP-1 was accomplished in U251MG and U87MG using the mammalian expression vector, pIRES, encoding full length MMP-1 cDNA. The MMP-1 over-expressing U251MG and U87MG cells exhibited significantly enhanced invasion in vitro with no modification in the cell proliferation rates. A majority of GBM patients present defective EGFR signaling due to over-expression, amplification or mutation in the receptor. MMP-1 is known to be up-regulated by various stimulatory agents including growth factors. We examined the regulation of MMP-1 by EGFR activation and observed the induction of MMP-1 after EGF treatment. Inhibition of the receptor by pharmaceutic inhibitor treatment and genetic approaches led to reduction in MMP-1 levels. We also observed that this regulation is primarily mediated by the downstream MAPK pathway. Inhibition of MAPK and not PI3K pathway resulted in diminished MMP-1 protein levels even in the presence of EGF. These studies demonstrate the importance of the EGFR-MAPK signaling pathway in the induction of MMP-1 in glioma cell lines. In addition, MMP-1 plays a role in glioma cell invasion in vitro. These results along with the reports of MMP-1 over-expression in GBM warrant future studies examining the function of MMP-1 in vivo.

GBM

MMP-1

Invasion

EGFR

MAPK

Life Sciences

EPIGENETIC REGULATION OF GENES INVOLVED IN VASCULAR DYSFUNCTION IN PREECLAMPTIC WOMEN

Mousa, Ahmad

23 January 2012

DNA methylation is the most recognizable epigenetic mechanism. In general, DNA hypomethylation is associated with increased gene expression whereas DNA hypermethylation is associated with decreased gene expression. To date, little is known about the role of DNA methylation in the pathophysiology of preeclampsia. In this study, we examined the differences in DNA methylation in omental arteries of normal pregnant and preeclamptic women using the high throughput Illumina HumanMethylation27 BeadChip assay. We found 1,685 genes with a significant difference in DNA methylation at a false discovery rate of < 10% with many inflammatory genes having reduced methylation. The thromboxane synthase gene was the most hypomethylated gene in preeclamptic women as compared to normal pregnant women. When we examined the expression of thromboxane synthase in omental arteries of normal pregnant and preeclamptic women we found it to be significantly increased in preeclamptic women. The increased expression was observed in vascular smooth muscle cells, endothelial cells and infiltrating neutrophils. Experimentally induced DNA hypomethylation increased the expression of thromboxane synthase in the neutrophil-like HL-60 cell line, whereas tumor necrosis factor α (TNFα), a neutrophil product, increased its expression in cultured human vascular smooth muscle cells (VSMC). These finding suggest that DNA methylation and release of TNFα by infiltrating neutrophils could contribute to the increased expression of thromboxane synthase in systemic blood vessels of preeclamptic women, contributing to the hypertension and coagulation abnormalities. We also explored the possible contribution of DNA methylation to the altered expression of genes involved in collagen metabolism in preeclampsia. Several matrix metalloproteinase (MMP) genes, including MMP1 and MMP8, were significantly less methylated in preeclamptic women, whereas TIMP and COL genes were either significantly more methylated or had no significant change in their DNA methylation status. Experimentally induced DNA hypomethylation increased the expression of MMP-1, but not TIMP-1 or COL1A1, in cultured VSMCs and increased the expression of MMP-1 and MMP-8 in HL-60 cells. These findings suggest that DNA methylation contributes to the imbalance in genes involved in collagen metabolism in blood vessels of preeclamptic women.

preeclampsia

epigenetics

thromboxane synthase

MMP-1

MMP-8.

Life Sciences

Physiology

NEUTROPHIL PRODUCTS CONTROL THE EXPRESSION OF PROGESTERONE RECEPTORS AND MATRIX METALLOPROTEINASE-1 IN THE DECIDUAL AND MYOMETRIUM AND ARE POSSIBLE REGULATORS OF PREMATURE LABOR

Solotskaya, Anna

04 May 2010

Neutrophils infiltrate myometrium and decidual tissue prior to parturition. Activated neutrophils release reactive oxygen species (ROS) and tumor necrosis factor α (TNFα), which might increase expression of pro-labor genes such as matrix metalloproteinase-1 (MMP-1), progesterone receptor (PR) A/B ratio, and cause demethylation of DNA. These changes might cause labor. Decidual tissue was obtained from consented, healthy women at term (37+ weeks of gestation) not in labor (no contractions, without cervical effacement), term labor and preterm labor (under 37 weeks of pregnancy). Decidual and myometrial cells in culture were treated with (1) ROS, (2) TNFα, or (3) 5-aza-2’-deoxycytidine. Total RNA was extracted, converted to cDNA and evaluated by qRT-PCR for MMP-1, PR-A+B and PR-B. TNFα increased MMP-1 by 17 fold in decidual cells and more than 12 fold in myometrial cells. PR-A/B was increased by 5.6 fold in decidua. ROS up-regulated MMP-1 by 6 fold and elevated the PR-A/B ratio by 4.5 fold in decidual tissue. DNA demethylation increased MMP-1 by about 4 and 11 fold in decidual and myometrium, respectively. The PR-A/B ratio was increased by 4 fold in decidua and the PR-B was decreased by 40% in the myometrium due to DNA demethylation. Decidual tissue in preterm labor showed a 7-fold increase in MMP-1 over term laboring and over a 15-fold increase over term not in labor tissue. In conclusion, MMP-1 expression and PR-A/B ratio was increased by neutrophil products possibly through a mechanism of DNA methylation in decidua and myometrium. Preterm decidua showed a dramatic increase in MMP-1 over normal labor tissue. TNFα and ROS increased expression of MMP-1 to possibly initiate parturition. These data might help explain mechanisms responsible for preterm labor unrelated to infection or premature rupture of membranes.

Preterm Labor

MMP-1

Progesterone Receptor

Neutrophils

Myometrium

Decidua

Life Sciences

Physiology

SPECTROSCOPIC CHARACTERIZATION OF ZINC HYDROLASES NDM-1 AND MMP-1 FOR DRUG DISCOVERY

yang, hao

27 July 2015

No description available.

Biochemistry

Chemistry

Effets de la prostaglandine D₂ (PGD₂) sur les réponses inflammatoires et cataboliques dans les chondrocytes humains

Mfuna Endam, Leandra

January 2007

Mémoire numérisé par la Direction des bibliothèques de l'Université de Montréal.

Arthrose

Prostaglandine D₂

IL-1[Beta]

MMP-1

MMP-13

NO

DP-1

CRTH2

MAPKs

NF-kB

Rôle de l’acide 12- Hydroxyeicosatétraénoïque dans la régulation des réponses inflammatoires et cataboliques dans les tissus articulaires dans la pathogenèse de l'arthrose

Mba Dassi, Habib

08 1900

Mémoire en recherche-création / L'arthrose (OA) est la maladie musculosquelettique la plus fréquente au monde et peut affecter toutes les articulations. L’arthrose est caractérisée par la dégradation progressive du cartilage, l’inflammation de la synoviale et le remodelage de l’os sous-chondral. Ces changements sont dus à une augmentation d’expression des médiateurs pro-inflammatoires tels que la cyclooxygénase 2 (COX-2) et de facteurs cataboliques, notamment les métalloprotéinases 1 et 13 (MMP-1 et 13). Les métabolites de la 12-lipoxygénase jouent un rôle important dans de nombreux processus physiologiques et pathologiques. À la suite des réactions d'oxygénation / réduction de la 12 LOX, un facteur eicosanoïde particulier est produit: le 12-HydroxyEicosaTétraÉnoique (12-HETE), dont le rôle dans la pathogenèse de l’OA n’est pas caractérisé. L’objectif de ce travail est de définir le rôle de la 12-HETE dans la régulation des réponses inflammatoires et cataboliques dans les tissus articulaires, chondrocytes et synoviocytes, humains. Nous avons démontré que la 12-HETE n’affecte pas la prolifération (test MTT) des chondrocytes et des synoviocytes et n’a aucun effet sur leur migration (test de rayure). Un traitement avec la 12-HETE augmente l’induction de l’expression de la COX-2 dans les deux types cellulaires. La 12-HETE n’avait aucun effet sur l’expression de la MMP-1 et la MMP-13. La 12-HETE induit ses effets à l’aide d’un récepteur couplé à la protéine G : la GRP31. Nous avons décrit l’arthrose sur des coupes histologiques humaines, puis nous avons observé que l’expression de GPR31 était similaire dans le cartilage dégradé et le cartilage non dégradé. Finalement, nous avons montré que les chondrocytes et les synoviocytes expriment la GPR31 et son niveau est diminué en présence de l’interleukine-1 béta (IL-1β). En conclusion, nous avons démontré que la 12-HETE a des effets divers sur les réponses inflammatoires et cataboliques dans les tissus articulaires : elle augmente l’expression de la cyclooxygénase 2 (COX- 2) et n’a pas d’effet sur l’expression de la MMP-1 et la MMP-13. / Osteoarthritis (OA) is the world's most common musculoskeletal disease and can affect all joints. Osteoarthritis is characterized by progressive degradation of cartilage, inflammation of the synovium and remodelling of the subchondral bone. These changes are due to increased expression of pro-inflammatory mediators such as cyclooxygenase 2 (COX-2) and catabolic factors including metalloproteinases 1 and 13 (MMP-1 and 13). 12-lipoxygenase metabolites play an important role in many physiological and pathological processes. Following the oxygenation/reduction reactions of 12 LOX, a particular eicosanoid factor is produced: 12-HydroxyEicosaTetraenoic (12-HETE), whose role in the pathogenesis of AO is uncharacterized. This work aims to define the role of 12-HydroxyEicosaTetraenoic (12-HETE) in regulating inflammatory and catabolic responses in human joint tissues, chondrocytes and synoviocytes. We have demonstrated that 12-HETE does not affect the proliferation (MTT assay) of chondrocytes and synoviocytes and has no effect on their migration (scratch assay). Treatment with 12-HETE increased the induction of COX-2 expression in both cell types. 12-HETE had no effects on MMP-1 and MMP-13 expression. 12-HETE induces its effects using a G protein-coupled receptor: GRP31. We described osteoarthritis on human histological sections and then observed that GPR31 expression was the same in degraded and non-degraded cartilage. Finally, we showed that chondrocytes and synoviocytes express GPR31 and its level is decreased in the presence of Interleukin-1 beta (IL-1β). In conclusion, we demonstrated that 12-HETE has different effects on inflammatory and catabolic responses in joint tissues by increasing COX-2 expression and has no effect on MMP-1 and MMP-13 expression.

GRP31

COX-2

MMP-1

MMP-13

Arthrose

Chondrocytes

Synoviocytes

Osteoarthritis

12-HETE

Efeitos da ciclosporina, fenitoína e nifedipina sobre a síntese e degradação de colágeno da gengiva de macacos-prego (Cebus apella): estudo histoquímico e através de RT-PCR

Kanno, Cláudia Misue [UNESP]

27 March 2006

Made available in DSpace on 2014-06-11T19:32:06Z (GMT). No. of bitstreams: 0 Previous issue date: 2006-03-27Bitstream added on 2014-06-13T20:22:59Z : No. of bitstreams: 1 kanno_cm_dr_araca.pdf: 1730975 bytes, checksum: 620b9c72f44529033f574688f3ea9bde (MD5) / INTRODUÇÃO: As alterações em gengiva induzidas por medicamentos têm sido pouco estudadas quanto à expressão in vivo dos genes das metoloproteinases (MMPs). O objetivo do presente trabalho foi avaliar o padrão histológico de distribuição de fibras colágenas após a administração de ciclosporina, nifedipina ou fenitoína e correlacionar com a expressão dos genes do colágeno do tipo I, MMP-1 e MMP2. MATERIAL E MÉTODO: Amostras da gengiva da área de canino superior direito foram obtidas de doze macacos prego (Cebus apella) machos. A extremidade mesial de cada amostra foi imediatamente congelada em nitrogênio líquido enquanto que a distal foi processada para inclusão em parafina. Após uma semana, os animais foram divididos em três grupos que receberam doses diárias de ciclosporina, fenitoína ou nifedipina, durante 120 dias. Procedeu-se à remoção de amostras da gengiva da área do canino superior esquerdo de dois animais de cada grupo aos 52 e 120 dias. Os cortes histológicos foram corados pelas técnicas da hematoxilina e eosina, vermelho picrosirius, além da marcação imunoistoquímica para colágeno do tipo IV. O RT-PCR semiquantitativo foi realizado para se determinar os níveis de mRNA. RESULTADOS: No grupo controle, houve o predomínio de fibras colágenas maduras, evidenciadas com a cor vermelha em cortes corados pela técnica do vermelho picrosirius analisados com microscópio de luz polarizada. Observou-se nos grupos tratados aos 52 e 120 dias um aumento da porcentagem de áreas ocupadas por fibras imaturas, em todos os grupos, independentemente da idade do animal. No entanto, não foram observadas diferenças morfológicas entre os grupos controle e tratado nos cortes corados pela hematoxilina e eosina. Houve uma tendência a valores médios mais baixos... / Background: Few studies have focused on the in vivo expression of matrix metalloproteinase (MMP) genes in gingival changes induced by drugs. The aim of the present study was to evaluate the histological pattern of collagen fiber distribution after phenytoin, cyclosporine or nifedipine medication and correlate with collagen type 1, MMP-1 and MMP-2 gene expression levels. Methods: Gingival samples were obtained from superior right canine area of twelve male capuchin monkeys (Cebus apella). The mesial part of the biopsy specimens was immediately frozen in liquid nitrogen, while the distal one was processed for paraffin inclusion. One week after the control biopsy, the animals were divided in three groups that received daily doses of cyclosporine, phenytoin or nifedipine during 120 days. Gingival samples were obtained from left superior canine area on 52nd and 120th day of treatment (two animal of each experimental group). Histologic sections were subjected to hematoxylin and eosin, picrosirius red stainings, and to immunohistochemical reaction for collagen type IV. MMP-1, MMP-2 and collagen type I mRNA levels were determined by RT-PCR. Results: Predominance of mature collagen fibers was observed in the control group after picrosirius red staining, visualized as red fibers under polarized microscope. Increased percentage of areas occupied by immature collagen fibers was observed on 52 and 120 experimental periods, in all groups, despite the animal age. However, no morphological differences between treated and control groups were observed on hematoxilin and eosin stained sections. There was a trend to lower levels of MMP-1 expression on 52-day samples. However, MMP-2 and collagen type I gene expressions seemed to be phased and drug-related. Conclusions: The results allowed the ...(Complete abstract click electronic access below)

Gengivas

Ciclosporina

Fenitoina

Colageno

Cebus apella

Crescimento excessivo da gengiva

Nifedipino

Colágeno tipo I

Gingival overgrowth

Cyclosporine

Phenytoin

Nifedipine

Collagen type I

MMP-1

MMP-2