Navegando por Palavras-chave "Timp1"
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- ItemAcesso aberto (Open Access)Associação entre Timp1, β1-integrinas e CD63 ao longo da gênese do melanoma(Universidade Federal de São Paulo (UNIFESP), 2010-11-24) Pinto, Mariana Toricelli [UNIFESP]; Jasiulionis, Miriam Galvonas [UNIFESP]; Universidade Federal de São Paulo (UNIFESP)Although malignant melanoma is the less frequently diagnosed skin cancer, it shows a poor prognosis due its chemoresistance and metastasis development. One of the adquired abilities of transformed cells is anoikis resistance and this property is closely related to metastasis formation. In our laboratory, we developed a model that allows us to study different steps of melanocyte malignant transformation. Melan-a melanocytes surviving after 1, 2, 3 and 4 deadhesion cycles showed modified morphology and independent PMA growth and have been named, 1C, 2C, 3C and 4C cells, respectively. Different melanoma cell lines were established after submitting 4C spheroids to limiting dilution. Previous results of our group showed increased expression of Timp1 along melanoma genesis and its correlation with anoikis resistance. However, the mechanism involved in this signaling is unknown. Published data demonstrated interaction between CD63, Timp1 and 1-integrins in human breast epithelial cells and its role in apoptosis. Furthermore, aberrant glycosylation in cell adhesion molecules such as integrins provides to cells the ability to survive under anchorage-independent conditions. The aim of this work was analyze the possible interaction among CD63, Timp1 and 1-integrins along melanocyte malignant transformation, possible aberrant N-glycosylation patterns of β1-integrins and their impact in anoikis resistance. Aberrant N-glycosylation patterns were observed in tumorigenic cells. We observed interaction between CD63 and Timp1 and between CD63 and 1-integrins in the melan-a-derived cells 4C, 4C11, and 4C11 +, and interaction between Timp1 and 1-integrins only in melanoma cell lines 4C11 - and 4C11 +. The presence of Timp1 in supernatant from 4C11+ conferred to melan-a cells anoikis resistance. The expression of 1-integrins in our study model is increased in aggressive melanoma lineage, 4C11+, as well as the expression of Mgat-V and aberrant N-glycosylation on cell surface. Moreover, the electrophoretic profile of 1-integrin suggests that melanoma metastatic 4C11+. Lineage present increased aberrant N-glycosylation in this molecule. Treatment of melanoma cells 4C11 + with the N-glycosylation inhibitor, swainsonine, resulted in reduced capacity of these cells to resist to anoikis. This seems to be the first study describing the interaction between Timp1, CD63 and 1-integrin in tumor cells and may contribute to a better understanding of how Timp1 regulates resistance to anoikis during the melanocyte malignant transformation.
- ItemAcesso aberto (Open Access)Timp1 interacts with beta-1 integrin and CD63 along melanoma genesis and confers anoikis resistance by activating PI3-K signaling pathway independently of Akt phosphorylation(Biomed Central Ltd, 2013-03-25) Toricelli, Mariana [UNIFESP]; Melo, Fabiana H. M. [UNIFESP]; Peres, Giovani B. [UNIFESP]; Silva, Debora C. P.; Jasiulionis, Miriam G. [UNIFESP]; Universidade Federal de São Paulo (UNIFESP); Ludwig Inst Canc ResBackground: Anoikis resistance is one of the abilities acquired along tumor progression. This characteristic is associated with metastasis development, since tumorigenic cells must survive independently of cell-matrix interactions in this process. in our laboratory, it was developed a murine melanocyte malignant transformation model associated with a sustained stressful condition. After subjecting melan-a melanocytes to 1, 2, 3 and 4 cycles of anchorage impediment, anoikis resistant cells were established and named 1C, 2C, 3C and 4C, respectively. These cells showed altered morphology and PMA independent cell growth, but were not tumorigenic, corresponding to pre-malignant cells. After limiting dilution of 4C pre-malignant cells, melanoma cell lines with different characteristics were obtained. Previous data from our group showed that increased Timp1 expression correlated with anoikis-resistant phenotype. Timp1 was shown to confer anchorage-independent growth capability to melan-a melanocytes and render melanoma cells more aggressive when injected into mice. However, the mechanisms involved in anoikis regulation by Timp1 in tumorigenic cells are not clear yet.Methods: the beta 1-integrin and Timp1 expression were evaluated by Western blotting and CD63 protein expression by flow cytometry using specific antibodies. To analyze the interaction among Timp1, CD63 and beta 1-integrin, immunoprecipitation assays were performed, anoikis resistance capability was evaluated in the presence or not of the PI3-K inhibitors, Wortmannin and LY294002. Relative expression of TIMP1 and CD63 in human metastatic melanoma cells was analyzed by real time PCR.Results: Differential association among Timp1, CD63 and beta 1-integrins was observed in melan-a melanocytes, 4C pre-malignant melanocytes and 4C11- and 4C11+ melanoma cells. Timp1 present in conditioned medium of melanoma cells rendered melan-a melanocytes anoikis-resistant through PI3-K signaling pathway independently of Akt activation. in human melanoma cell lines, in which TIMP1 and beta-1 integrin were also found to be interacting, TIMP1 and CD63 levels together was shown to correlate significantly with colony formation capacity.Conclusions: Our results show that Timp1 is assembled in a supramolecular complex containing CD63 and beta 1-integrins along melanoma genesis and confers anoikis resistance by activating PI3-K signaling pathway, independently of Akt phosphorylation. in addition, our data point TIMP1, mainly together with CD63, as a potential biomarker of melanoma.
- ItemAcesso aberto (Open Access)Timp1 Promotes Cell Survival by Activating the PDK1 Signaling Pathway in Melanoma(Mdpi Ag, 2017) Toricelli, Mariana [UNIFESP]; Melo, Fabiana H. M. [UNIFESP]; Hunger, Aline; Zanatta, Daniela; Strauss, Bryan E.; Jasiulionis, Miriam G. [UNIFESP]High TIMP1 expression is associated with poor prognosis in melanoma, where it can bind to CD63 and beta 1 integrin, inducing PI3-kinase pathway and cell survival. Phosphatidylinositol (3,4,5)-trisphosphate (PIP3), generated under phosphatidylinositol-3-kinase (PI3K) activation, enables the recruitment and activation of protein kinase B (PKB/AKT) and phosphoinositide-dependent kinase 1 (PDK1) at the membrane, resulting in the phosphorylation of a host of other proteins. Using a melanoma progression model, we evaluated the impact of Timp1 and AKT silencing, as well as PI3K, PDK1, and protein kinase C (PKC) inhibitors on aggressiveness characteristics. Timp1 downregulation resulted in decreased anoikis resistance, clonogenicity, dacarbazine resistance, and in vivo tumor growth and lung colonization. In metastatic cells, pAKT(Thr308) is highly expressed, contributing to anoikis resistance. We showed that PDK1(Ser241) and PKC beta IISer660 are activated by Timp1 in different stages of melanoma progression, contributing to colony formation and anoikis resistance. Moreover, simultaneous inhibition of Timp1 and AKT in metastatic cells resulted in more effective anoikis inhibition. Our findings demonstrate that Timp1 promotes cell survival with the participation of PDK1 and PKC in melanoma. In addition, Timp1 and AKT act synergistically to confer anoikis resistance in advanced tumor stages. This study brings new insights about the mechanisms by which Timp1 promotes cell survival in melanoma, and points to novel perspectives for therapeutic approaches.