The Role of CARD14 in Skin Barrier Homeostasis and Allergic Disease

Devore, Stanley

31 May 2023

No description available.

Cellular Biology

Atopic Dermatitis

Allergy

CARD14

MYC

Skin

Keratinocyte

Glycogen Synthase Kinase-3 Loss-Of-Function Studies in Mus musculus and Murine Embryonic Stem Cells

Popkie, Anthony P.

21 March 2011

No description available.

Molecular Biology

Gsk-3

DNA methylation

N-Myc

Dnmt3a

THE ROLE OF THE STRESS RESPONSE GENE GADD45A IN MODULATING MYC MEDIATED APOPTOSIS AND DIFFERENTIATION

Mohamed-Hadley, Alisha

January 2011

The Gadd45 family of proteins is known to play a central role as cellular stress sensors that modulate the response of mammalian cells to different stressors, including oncogenic stress. Gadd45a expression is regulated during myeloid cell differentiation, and is also induced in response to acute stimulation with cytokines, myeloablation and inflammation. The proto-oncogene C-myc plays a pivotal role in growth control, differentiation and apoptosis in hematopoietic cells. Deregulated Myc in hematopoietic cells blocks the differentiation program and prevents normal homeostatic cellular apoptosis, which alters the balance of cell populations, often participating in leukemogenesis. The status of Gadd45a expression has been shown to impact on different cancers, including breast cancer and leukemia. How the stress response gene Gadd45a modulates oncogenic stress imparted by deregulated c-Myc in myeloid cells has not been investigated. We hypothesized that Gadd45a and its interacting partner proteins can modulate specific pro-survival or pro-apoptotic signaling pathways, altering the cellular response to oncogenic myc in myeloid cells. Gadd45a may play different roles in proliferating and differentiating cells, and myeloid cells in vivo are at all stages of myeloid development. Therefore, to understand how Gadd45a status impacts on proliferating and differentiating myeloid cells, we decided to study the effect of loss of Gadd45a in myc-expressing cells that are either proliferating or stimulated to undergo differentiation. Therefore, to address this issue we utilized bone marrow from wild-type (wt) and Gadd45a null mice, and retrovirally infected these cells to express constitutive Myc or empty vector control. Using these cells we have shown that bone marrow deficient in Gadd45a and expressing constitutive Myc, display decreased apoptosis under proliferating conditions, yet increased apoptosis in media containing the differentiation inducing cytokine GM-CSF. We show that in expansion media loss of Gadd45a in the presence of Myc elicits its function through the activation of p38, with evidence supporting a role for PU.1 and Mcl-1 expression, which are downstream of p-p38. In contrast, deregulated C-Myc and loss of Gadd45a does not signal through p-38 in GM-CSF, but surprisingly there is a decrease in cytokine receptor expression. This data demonstrates that Gadd45a may be required for optimal cytokine receptor expression in myeloid cells, which can impact on survival of the cells. Although in primary bone marrow Gadd45a status had no effect on differentiation of Myc expressing cells, the loss of Gadd45a in Hoxb8 generated cell lines shifted differentiation towards increased neutrophils. Determining the role of Gadd45a on the biological outcome of myeloid cells in response to deregulated c-Myc will provide vital information in understanding the function of Gadd45a in the development and progression of Myc expressing myeloid leukemia. / Molecular Biology and Genetics

Biology, Molecular

Apoptosis

Cytokine

Gadd45a

Myc

Myeloid Cells

Pin1: WW domain ligands, catalytic inhibitors, and the mechanism

Mercedes-Camacho, Ana Yokayra

25 May 2011

The peptidyl prolyl cis/trans isomerase, PPIase, has been the focus of numerous studies in the field of cell cycle regulation since proline-directed phosphorylation is an essential signaling mechanism that might arrest cancer proliferation. Pin1 is the first phosphorylation-dependent PPIase enzyme to be discovered. The Pin1 regulatory mechanism, acting on other mitotic proteins in vivo and in vitro, remains largely unknown. For the study of Pin1 function, two types of assays were used to identity ligands for Pin1: (1) The Enzyme-Linked Enzyme Binding Assay (ELEBA) for the identification of WW domain ligands, (2) a catalytic assay to identified inhibitors of Pin1 catalytic activity. The ELEBA offers a selective approach for detecting ligands that bind to the Pin1 WW domain from chemical libraries. By using the ELEBA, a pSer-Pro peptidomimetic library of 315 ligands was screened, identifying three promising ligands cis-D2, O2, and M18. Competitive Kd values for cis-D2, O2, and M18 were determined to be 263 ± 6.4, 206 ± 3.4, and 130 ± 3.0μM, respectively. Furthermore, we screened the pSer-Pro peptidomimetic library using a Pin1 discontinuous-catalytic assay to identify inhibitors of Pin1. Ligands D20 and K7 were identified to decrease more than 90% of the Pin1 catalytic activity. To investigate the nature of the Pin1 interaction with c-Myc, we synthesized and characterized four peptides corresponding to the c-Myc sequence. These peptides were used in NMR isomerization studies of Pin1 by our collaborator Dr. Jeffry Peng (University of Notre Dame). Preliminary work shows that Pin1 binds and isomerizes the Ac–LLPpTPPLSPS–NH₂ peptide at the cMyc pThr58 position. Finally, we measured a secondary kinetic isotope effect (2º KIE) to study the Pin1 catalytic mechanism of proline isomerization. The ratio of kH/kD for unlabeled and [d₃]Ser-labeled substrate gave a SKIE value of 1.34 ± 0.01. The normal 2º KIE value indicates that carbonyl-serine hybridization is not changing from sp² to sp³. This result supports substrate analogue inhibitor studies, and previous solvent and SKIE results on Pin1, that suggest a twisted amide mechanism assisted by a transient hydrogen bond in the transition state. / Ph. D.

PPIases

Pin1 inhibitors

WW domain ligands

KIE

c-Myc

ELEBA

Mécanismes de l'auto-renouvellement non-tumoral des macrophages matures / Identification of Non-tumorigenic Self-renewal Mechanisms of Differentiated macrophages

Beniazza, Meryam

29 September 2014

Chez les métazoaires, la différenciation terminale est généralement accompagnée par une sortie définitive du cycle cellulaire. Cependant, les macrophages et très peu d'autres types cellulaires rompent avec ce dogme. En effet, il est maintenant admis que les macrophages conservent la capacité de s'auto-renouveler indépendamment des cellules souches ou progénitrices. À cet égard, nous avons démontré que la double déficience en facteurs Maf dans les macrophages (Maf-DKO) leur confère la capacité de s'auto-renouveler indéfiniment en culture sans se dé-différencier ou devenir tumorigènes. Ce phénotype d'auto-renouvellement semble être médié par un réseau transcriptionnel de de gènes régissant l'auto-renouvellement qui sont également actifs dans les cellules souches embryonnaires, parmi lesquels Myc et Klf4. Ces deux facteurs sont activés et nécessaires pour l'auto-renouvellement des Maf-DKO. De façon intéressante, l'expression de Myc seul induit une prolifération illimitée des macrophages, mais provoque une transformation tumorale. Nous avons donc cherché à décrypter les mécanismes grâce auxquels Myc et Klf4 induisent l'auto-renouvellement des macrophages, en comparaison à la transformation cellulaire causée par l'expression de Myc uniquement. En outre, nous nous sommes concentrés sur l'identification de gènes candidats permettant un auto-renouvellement illimité des macrophages, tout en les protégeant de la transformation cancéreuse. Notre objectif est de contribuer à l'identification du programme transcriptionnel régulant l'auto-renouvellement non tumoral des macrophages. / In metazoan, terminal differentiation is generally accompanied by permanent exit from the cell cycle. Yet, macrophages and very few other examples break with this dogma. Indeed, it has become evident that macrophages retain the ability to self-renew independently of stem or progenitor cells. In this regard, we have previously shown that MafB/c-Maf double deficient (Maf-DKO) macrophages are able to self-renew indefinitely in vitro without dedifferentiating or becoming tumorigenic. This self-renewal phenotype appears to be mediated by a transcriptional network of self-renewal genes also active in embryonic stem cells, among which Myc and Klf4. Interestingly, these two factors are activated and required for Maf-DKO self-renewal. By contrast, Myc alone induces an unlimited proliferation of macrophages but causes malignant transformation. We aimed to decipher the mechanisms by which Myc and Klf4 induce stem cell-like self-renewal in macrophages, in comparison to cellular transformation caused by the expression of Myc alone. Additionally, we focused on identifying candidate genes allowing an unlimited self-renewal of macrophages while protecting them from tumorigenic transformation or aberrant proliferation. Our objective is to contribute to the identification of the transcriptional program regulating non-tumorigenic self-renewal in macrophages.

Myc

Klf4

Macrophage

Tumeur

Auto-Renouvellement

Cellule souche

Myc

Klf4

Macrophage

Tumor

Self-Renewal

Stem cells

571

Estudos das proteínas hnRNP K, SET e MARK3 como potenciais marcadores de prognóstico em câncer epidermóide de cabeça e pescoço (HNSCC) / Study of protein hnRNP K, SET and MARK3 as potential markers of prognosis in squamous cell cancer of head and neck (HNSCC).

Silva, Flávia Amoroso Matos e

31 July 2009

As neoplasias de cabeça e pescoço constituem um importante problema de saúde pública devido à alta incidência e alguns tipos estão associados a fatores comportamentais como consumo de álcool e tabaco. Apesar desses dados, a doença, especialmente em sua fase inicial, pode ser curada e alguns tipos podem ser prevenidos. Portanto, existe a necessidade de identificar e validar novos biomarcadores em câncer de cabeça e pescoço com aplicação em prognóstico e seleção de terapias mais adequadas. Neste sentido, o objetivo deste trabalho foi validar o perfil de três proteínas, SET, hnRNP K e MARK3 em tumores de cabeça e pescoço, e verificar a potencial aplicação como marcadores de diagnóstico e prognóstico em HNSCC, bem como propor um papel para estas proteínas na tumorigênese. Foram analisadas 22 amostras de tumores de cabeça e pescoço por western blotting (WB) e 96 amostras (91 tumores, 4 biópsias e 1 controle) dispostas em duplicata em lâmina de tissue microarray, obtidas no Brasil e cedidas pelo Grupo GENCAPO, por imunohistoquímica (IHC). Os dados obtidos foram correlacionados com todos os parâmetros clínicos e patológicos e com prognóstico do paciente com HNSCC por um período de 48 meses. Os resultados obtidos por WB e IHC mostraram acúmulo e fragmentação da SET e acúmulo nuclear e citoplasmático da hnRNP K nos tumores comparado a respectiva margem cirúrgica e tecido normal. A hnRNPK mostrou valor prognóstico sendo associada a sobrevida global do paciente. A proteína c-Myc e a sua forma fosforilada foram analisadas nas amostras de tumores e suas respectivas margens cirúrgicas devido a sua relação com SET, PP2A e hnRNP K. Os resultados mostraram acúmulo da c-Myc fosforilada e total nas amostras tumorais, o que coincidiu com aumento de SET e hnRNP K. Com relação à proteína MARK3, observou-se sua redução no tumor e menor sobrevida livre de doença. Foi realizado ensaio de RNA de interferência (RNAi) contra hnRNP K e SET em linhagem de carcinoma oral (HN13). A redução da proteína SET por RNAi levou a redução significativa da hnRNP K, enquanto a hnRNP K gerou menor efeito na proteína SET, sugerindo um efeito regulatório na expressão ou manutenção da hnRNP K pela SET na célula tumoral. A interferência contra a hnRNP K também reduziu a proliferação celular tumoral. Em conclusão, o aumento da proteína SET está associado à desmoplasia em HNSCC e pode ser um potencial marcador específico para essa condição. hnRNP K e MARK3 podem servir como potenciais marcadores em HNSCC e ajudar a identificar um subgrupo de pacientes com pobre prognóstico. A hnRNPK exerce efeito positivo na proliferação da célula tumoral. SET e hnRNP K podem atuar como fatores oncogênicos favorecendo o aumento de c-Myc. / The head and neck cancers constitute a major public health problem due to the high incidence and some types are associated with behavioral factors such as consumption of alcohol and tobacco. Despite these data, the disease, especially in its early stage can be cured and some types can be prevented. Therefore, there is a need to identify and validate new biomarkers in head and neck cancer, with applications in prognosis and selection of therapies most appropriate. Accordingly, the objectives of this study were validation of the profile of three proteins, SET, hnRNP K and MARK3 in tumors of head and neck, and verify the potential application as markers for diagnosis and prognosis in HNSCC, and suggest a role for these proteins in tumorigenesis. We analyzed 22 samples of head and neck tumors by western blotting (WB) and 96 samples (91 tumors, 4 biopsies and 1 control) arranged in duplicate in the tissue microarray slide, obtained in Brazil and assigned by the GENCAPO Group, by immunohistochemistry (IHC). The data were correlated with all clinical and pathological parameters and prognosis of patients with HNSCC for a period of 48 months. The results obtained by WB and IHC showed the SET accumulation and fragmentation and hnRNP K nuclear and cytoplasmic accumulation in tumor compared to the surgical margin and normal tissue. The hnRNPK prognostic value has been associated with overall survival of patients. The c-Myc protein and its phosphorylated form were analyzed in tumor and surgical margins samples due to its relationship with SET, PP2A and hnRNP K. The results showed accumulated total and phosphorylated c-Myc in tumor samples, which was coincided with increase in SET and hnRNP K. Regarding the protein MARK3 was observed its reduction in tumor and lower disease-free survival. RNA interference (RNAi) against hnRNP K and SET were performed in oral squamous cell carcinoma line (HN13). SET protein reduction by RNAi led to significant reduction of hnRNP K, and hnRNP K showed a minor effect on SET protein, suggesting a regulatory effect on expression or maintenance of hnRNP K by SET in tumor cells. Interference against hnRNP K also reduced tumor cell proliferation. In conclusion, increased SET protein is associated with desmoplasia in HNSCC and may be a potential specific marker for this condition. hnRNP K and MARK3 can serve as potential markers in HNSCC and help identify a subgroup of patients with poor prognosis. The hnRNPK must act a positive effect on cell proliferation of the tumor. SET and hnRNP K may act as oncogenic factors contributing for c-Myc activity.

c-Myc

c-Myc

carcinoma oral

CTAK1

CTAK1

HNSCC

I2PP2A

I2PP2A

K protein

prognosis

prognóstico

proteína K

O papel das proteínas ras em células adrenocorticais Y-1 e na transdução do sinal de ACTH / The role of ras proteins in Y-1 adrenocortical cells and the transduction of the ACTH signal

Moraes, Miriam Santos de

05 September 2002

Células Y-1 apresentam o gene K-ras amplificado, o que resulta em altos níveis de expressão da proteína codificada por este gene. Este fato faz com que células Y-1 apresentem níveis cronicamente altos de K-Ras-GTP. Além disso, estas células apresentam uma relativa desregulação da transição G0→Gl→S, a qual é caracterizada por uma porcentagem de células entrando na fase S do ciclo celular na condição carenciada; e também, por um afrouxamento na regulação de Myc, o qual apresenta níveis basais significantes de mRNA e proteína. Para verificar se existe uma relação entre K-Ras-GTP elevado e os níveis basais de Myc e a desregulação na transição G0→Gl→S, células Y-1 foram transfectadas com uma forma dominante negativa de H-ras, H-ras Asn-17 (RasN 17). Os transfectantes resultantes também foram utilizados para verificar o papel de Ras na transdução do sinal iniciado por FGF-2 e ACTH. Com estes clones foi possível verificar uma redução nos níveis de ativação de K-Ras na condição carenciada, e com isso ficou claro que FGF-2 e ACTH são capazes de induzir a ativação de K-Ras, porém com cinética diferentes: uma ativação tardia e lenta para FGF-2, e rápida e transiente para ACTH. Com a redução nos níveis de Ras-GTP, verificamos uma concomitante redução no basal da proteína c-Myc e também no basal de entrada em S, indicando que existe uma correlação entre estes fatores. Além disso, os clones Yl-RasN17 foram determinantes para mostrar que em células Y-1 a presença de Akt/PKB constitutivamente ativada é conseqüência dos níveis cronicamente elevados de K-Ras-GTP (Forti et al, 2002). / Abstract not available.

Adrenocortical cells

C-myc

C-myc

Células adrenocorticais

Fatores de crescimento

Growth factors

Proteínas Ras

Proteins Ras

Signal transduction

Transdução de sinal

O Gene c-myc e o controle do ciclo celular por ACTH em células adrenocorticais de camundongo da linhagem Y-1 / The c-myc gene and the control of cell cycle by ACTH and FGF2 in the Y-1 adrenocortical cell line

Lepique, Ana Paula

20 October 2000

ACTH é o hormônio trófico que estimula a esteroidogênese, promove o crescimento e a manutenção do córtex adrenal. Porém, em linhagens adrenocorticais, assim como em culturas primárias, ACTH inibe a proliferação celular. A linhagem Y-1 de células adrenocorticais de camundongo tem as seguintes respostas a ACTH: aumento da esteroidogênese, arredondamento celular, bloqueio do ciclo celular em G1 e indução dos proto-oncogenes fos e jun. Esta linhagem também responde muito Sem a FGF2, um protótipo da família dos FGFs (Fibroblast Growth Factors) que regula diferenciação e proliferação de diversos tipos celulares, sendo estimulada a transitar pelas fases G0→G1→S do ciclo celular. ACTH antagoniza este efeito de FGF2, inibindo parcialmente a entrada em S induzida por FGF2. Este projeto buscou compreender o papel de c-Myc no controle do ciclo celular de Y-1, com ênfase nos efeitos de ACTH e FGF2 na expressão e atividade de c-Myc. Mostramos que os dois principais controles da expressão de c-Myc em Y-1 são transcrição e degradação da proteína, sendo a concentração de c-Myc o único controle sobre o sistema Myc/Max/Mad, uma vez que a expressão de Max e de Mad-1 , Mad-4 e Mxi é constitutiva em células Y-1. FGF2 induz a expressão de c-Myc através da indução da transcrição e aumento da estabilidade da proteína de forma totalmente dependente da via de Erk-MAPK. ACTH, por outro lado, não interfere com a transcrição de c-myc, mas promove fortemente a degradação da proteína, dependentemente da via de PKA. Utilizando um sistema de transfecção transiente, transfectamos uma quimera da proteína c-Myc com o receptor de estrógeno, MycER. Quando ativada por tamoxifen, a quimera migra para o núcleo e reverte a ação anti-mitogênica de ACTH sobre FGF2, porém, não tem efeito sobre células carenciadas tratadas ou não com ACTH apenas. Em conclusão, o antagonismo entre ACTH e FGF2 no controle da transição G0→G1→S do ciclo celular de Y-1 pode ser explicado pelas suas ações antagônicas sobre a estabilidade da proteína c-Myc. / ACTH is the trophic hormone that stimulates steroidogenesis, promotes growth and maintenance of the adrenal cortex. However, in adrenal cell lines, as well as in primary cultures, ACTH inhibits cell proliferation. ACTH effects on Y-1 cells are: increasing in steroidogenesis, cell rounding, cell cycle blocking in G1 phase and induction of fos and jun proto-oncogenes expression. Y-1 cell line displays a robust response to FGF2, a member from the FGFs family (Fibroblast Growth Factors), which regulates differentiation and proliferation in many cell types, being induced to enter G0→G1→S phases of fhe cell cycle upon FGF2 stimulation. ACTH antagonizes FGF2 effect, partially inhibiting cell cycle progression stimulated by FGF2. This project aimed to investigate c-Myc role in Y-1 cell cycle control, with emphasis on ACTH and FGF2 effects on its expression and activity control. We have shown that there are two main controls of c-Myc expression in Y-1 cells, transcription and protein stability. c-Myc concentration regulates the system Myc/Max/Mad, once Max and also Mad-1, Mad-4 and Mxi expression is constitutive in Y-1 cells. FGF2 induces c-Myc expression by increasing its transcription rate and stabilizing the protein in an Erk-MAPK pathway dependent manner. ACTH, on the other hand, does not control c-myc transcription but promotes a strong degradation of the protein through the PKA pathway. Using a transient transfection system, we were able to express MycER, a chimera of c-Myc and estrogen receptor in Y-1 cells. When activated by tamoxlfen, MycER is translocated to cell nucleus, where it abolishes the anti-mitogenic effect of ACTH over FGF2. However, it has no effect on cell cycle progression of serum starved cells treated or not with ACTH only. In conclusion, their antagonist effects on c-Myc protein stability can explain the antagonist effects of ACTH and FGF2 on the control of G0→G1→S transition of Y-1 cell cycle.

ACTH

ACTH

Adrenocortical tumor cells

C-myc

C-myc

Cell cyclo

Células adrenorticais tumorais

Ciclo celular

FGF2

FGF2

Effets d'inhibiteurs de la cyclooxygénase-2 sur la prolifération et la survie de cellules cancéreuses hématopoïétiques / Effects of cyclooxygenase-2 inhibitors on cell proliferation and cell death in human hematopoietic cancer cell lines

Sobolewski, Cyril

10 November 2011

Les cyclooxygénases (COXs) sont une famille d'enzymes impliquées dans la biosynthèse des prostaglandines. COX-2 est la forme inductible qui est induite pendant l'inflammation et qui est surexprimée dans plusieurs cancers. Plusieurs évidences suggèrent que COX-2 joue un rôle dans la prolifération cellulaire et l'apoptose. Ces évidences concernent surtout les tumeurs solides et les mécanismes impliqués ne sont pas complètement connus et surtout pour les cancers d'origine hématopoïétique. Pour notre étude, nous avons étudié l'effet d'inhibiteurs de COX-2 (nimésulide, NS-398 et célécoxib) sur la prolifération et l'apoptose de lignées cellulaires leucémiques et lymphoblastiques, Hel, Jurkat, Raji et U937. Nous avons montré que les différents inhibiteurs de COX-2 diminuent la prolifération des différentes lignées cellulaires. Les cellules U937 sont apparues comme les cellules les plus sensibles à ces inhibiteurs alors que les cellules K562 étaient les plus résistantes. Nous avons montré que cette modulation correspond à une accumulation des cellules en phase G0/G1 du cycle cellulaire, accompagnée d'une diminution précoce de l'expression de c-Myc et d'une augmentation de l'expression de marqueurs de différenciation dans les cellules U937 (CD15) et Hel (CD41a et CD61). Dans la deuxième partie de ce projet, nous avons étudié les effets des différents inhibiteurs de COX-2 sur l'apoptose induite par différents agents chimiothérapeutiques dans nos modèles cellulaires. Nous avons ainsi montré que les inhibiteurs de COX-2 inhibent fortement l'apoptose induite par plusieurs agents chimiothérapeutiques. Nous avons démontré que la prévention de l'apoptose se situe avant l'activation de Bax et de Bak. Par ailleurs, cet effet est caractérisé par une incapacité des agents chimiothérapeutiques à déclencher un stress apoptotique. Toutes nos données ont donc démontré un effet anti-apoptotique des inhibiteurs de COX-2 sur l?apoptose intrinsèque vs l'apoptose extrinsèque à un stade précoce de l'induction de l'apoptose. Ces données suggèrent des précautions quant à l'utilisation des inhibiteurs de COX-2 en combinaison avec la chimiothérapie. Dans la troisième partie de notre projet, nous avons étudié la combinaison des inhibiteurs de COX-2 avec la curcumine, une substance naturelle connue pour ses propriétés antitumorales. Nos travaux ont montré que la curcumine seule conduit à une accumulation des cellules U937 en phase G2/M du cycle cellulaire, suivie d'une induction d'apoptose. Cependant, le prétraitement des cellules U937 avec du célécoxib à des concentrations non-apoptogéniques contrecarre l'apoptose induite par la curcumine, suggérant ainsi que ce type de combinaison ne serait pas une bonne stratégie dans les cellules hématopoïétiques. L'utilisation chronique des inhibiteurs de COX-2 peut être associée à des effets secondaires importants consécutifs à l'inhibition de l'activité de COX-2. Dans la dernière partie de notre projet, nous avons démontré que le 2,5 diméthyl-célécoxib (DMC), un analogue du célécoxib qui n'inhibe pas l'activité de COX-2, induit une diminution de la prolifération cellulaire et induit l'apoptose des cellules U937 et K562. Par ailleurs, ces effets sont plus importants que ceux observés avec le célécoxib. Par conséquent, ce composé a démontré de meilleures propriétés antitumorales et représente une voie thérapeutique prometteuse contre les leucémies. Tous nos résultats soutiennent donc l'idée que les inhibiteurs de COX-2 présentent les effets anti-tumoraux les plus efficaces que lorsqu'ils sont administrés seuls. Les effets observés avec le DMC suggèrent que ce composé pourrait représenté une voie alternative aux inhibiteurs de COX-2 en thérapie anti-cancéreuse. / Cyclooxygenases (COXs) are a family of enzymes, which catalyze the rate-limiting step in prostaglandin biosynthesis. COX-2 is the inducible isoform, upregulated during inflammation and overexpressed in various cancers. There are evidences of a role for COX-2 in cell proliferation and apoptosis especially in solid tumors, whereas little is known for cancers of hematopoietic origin. In our study, we analyzed the effect of COX-2 inhibitors (nimesulide, NS-398 and celecoxib) on cell proliferation and apoptosis of a panel of leukemic and lymphoblastic cell lines, Hel, Jurkat, K562, K562, Raji and U937. We found that the different inhibitors slow down cell proliferation in the different hematologic cell lines tested. U937 cells appeared as the most sensitive, whereas K562 were the most resistant to this effect. We provide evidence that this modulation corresponds to an accumulation of the cells in G0/G1 paralleled by an early downregulation of c-Myc and the expression of cell type-specific differentiation markers in U937 (CD15) and Hel (CD41a and CD61). In the second part of our study, we investigate the effect of COX-2 inhibitors on apoptosis induced by chemotherapeutic agents in our cell models. We demonstrated that COX-2 inhibitors strongly prevent apoptosis induced by a panel of chemotherapeutic agents. We demonstrated an early prevention of apoptotic signaling, prior to Bax/Bak activation. The preventive effect is associated with an impairment of the ability of chemotherapeutic agents to trigger their apoptogenic stress. Altogether, our results demonstrate an anti-apoptotic effect of COX-2 inhibitors on intrinsic vs. extrinsic apoptosis at early steps of apoptosis commitment. These results suggest cautions in the use of COX-2 inhibitors with chemotherapy. In the third part of our project, we investigated the combination of COX-2 inhibitors with curcumin, a natural product known for its anti-tumor properties. Our findings show that curcumin alone leads to an accumulation of U937 cells in G2/M phase of cell cycle, followed by an induction of apoptosis. However, the pretreatment of U937 cells with celecoxib at non-apoptogenic concentrations, counteracted curcumin-induced apoptosis, thus showing that this combination is not a good anti-cancer strategy in our cell models. The chronic use of COX-2 inhibitors can be associated with severe side effects due to the inhibition of COX-2 enzyme. In the last part of our project, we demonstrated that 2,5 dimethyl-celecoxib (DMC), a structurally analogue of celecoxib, which is not able to inhibit COX-2 activity, induces an inhibition of cell proliferation and an induction of apoptosis in U937 and K562 cells. These effects are stronger than those observed with celecoxib. Thus, this compound demonstrated better anti-tumor properties and may represent a promising therapeutic approach against leukemia. Altogether, our study supports the idea that COX-2 inhibitors display anti-tumor effects in our cell models, but only when administrated alone. The effects observed with DMC suggest that this compound may represent an alternative approach to COX-2 inhibitors in cancer therapy.

Cox-2

Leucémie

Inflammation

Apoptose

Cycle cellulaire

C-Myc

Cox-2

Leukemia

Inflammation

Apoptosis

Cell cycle

C-Myc

616.994 1906

Pharmacological regulation of c-myc gene expression in human breast cancer cells

Melkoumian, Zaroui K.,

January 2001

Thesis (Ph. D.)--West Virginia University, 2001. / Title from document title page. Document formatted into pages; contains x, 152 p. : ill. (some col.). Vita. Includes abstract. Includes bibliographical references (p. 119-149).