Your search keyword '"Fernandez, Soledad A."' showing total 8 results

1. BRAF activates and physically interacts with PAK to regulate cell motility.

Author

McCarty, Samantha K., Motoyasu Saji, Xiaoli Zhang, Knippler, Christina M., Kirschner, Lawrence S., Fernandez, Soledad, and Ringel, Matthew D.

Subjects

THYROID cancer, PROTEIN kinases, CELLULAR signal transduction, GENE expression, CANCER cells, CELL motility

Abstract

Increased p21-activated kinase (PAK) signaling and expression have been identified in the invasive fronts of aggressive papillary thyroid cancers (PTCs), including those with RET/PTC, BRAFV600E, and mutant RAS expression. Functionally, thyroid cancer cell motility in vitro is dependent on group 1 PAKs, particularly PAK1. In this study, we hypothesize that BRAF, a central kinase in PTC tumorigenesis and invasion, regulates thyroid cancer cell motility in part through PAK activation. Using three well-characterized human thyroid cancer cell lines, we demonstrated in all cell lines that BRAF knockdown reduced PAK phosphorylation of direct downstream targets. In contrast, inhibition of MEK activity either pharmacologically or with siRNA did not reduce PAK activity, indicating MEK is dispensable for PAK activity. Inhibition of cell migration through BRAF loss is rescued by overexpression of either constitutive active MEK1 or PAK1, demonstrating that both signaling pathways are involved in BRAF-regulated cell motility. To further characterize BRAF-PAK signaling, immunofluorescence and immunoprecipitation demonstrated that both exogenously overexpressed and endogenous PAK1 and BRAF co-localize and physically interact, and that this interaction was enhanced in mitosis. Finally, we demonstrated that acute induction of BRAFV600E expression in vivo in murine thyroid glands results in increased PAK expression and activity confirming a positive signaling relationship in vivo. In conclusion, we have identified a signaling pathway in thyroid cancer cells which BRAF activates and physically interacts with PAK and regulates cell motility. [ABSTRACT FROM AUTHOR]

Published

2014

2. Ets2 in Tumor Fibroblasts Promotes Angiogenesis in Breast Cancer.

Author

Wallace, Julie A., Li, Fu, Balakrishnan, Subhasree, Cantemir-Stone, Carmen Z., Pecot, Thierry, Martin, Chelsea, Kladney, Raleigh D., Sharma, Sudarshana M., Trimboli, Anthony J., Fernandez, Soledad A., Yu, Lianbo, Rosol, Thomas J., Stromberg, Paul C., Lesurf, Robert, Hallett, Michael, Park, Morag, Leone, Gustavo, and Ostrowski, Michael C.

Subjects

BREAST cancer, FIBROBLASTS, PROMOTERS (Genetics), NEOVASCULARIZATION, CANCER cells, STROMAL cells, CANCER invasiveness, EPITHELIAL cells, GENE expression

Abstract

Tumor fibroblasts are active partners in tumor progression, but the genes and pathways that mediate this collaboration are ill-defined. Previous work demonstrates that Ets2 function in stromal cells significantly contributes to breast tumor progression. Conditional mouse models were used to study the function of Ets2 in both mammary stromal fibroblasts and epithelial cells. Conditional inactivation of Ets2 in stromal fibroblasts in PyMT and ErbB2 driven tumors significantly reduced tumor growth, however deletion of Ets2 in epithelial cells in the PyMT model had no significant effect. Analysis of gene expression in fibroblasts revealed a tumor- and Ets2-dependent gene signature that was enriched in genes important for ECM remodeling, cell migration, and angiogenesis in both PyMT and ErbB2 driven-tumors. Consistent with these results, PyMT and ErbB2 tumors lacking Ets2 in fibroblasts had fewer functional blood vessels, and Ets2 in fibroblasts elicited changes in gene expression in tumor endothelial cells consistent with this phenotype. An in vivo angiogenesis assay revealed the ability of Ets2 in fibroblasts to promote blood vessel formation in the absence of tumor cells. Importantly, the Ets2-dependent gene expression signatures from both mouse models were able to distinguish human breast tumor stroma from normal stroma, and correlated with patient outcomes in two whole tumor breast cancer data sets. The data reveals a key function for Ets2 in tumor fibroblasts in signaling to endothelial cells to promote tumor angiogenesis. The results highlight the collaborative networks that orchestrate communication between stromal cells and tumor cells, and suggest that targeting tumor fibroblasts may be an effective strategy for developing novel anti-angiogenic therapies. [ABSTRACT FROM AUTHOR]

Published

2013

3. Pten in stromal fibroblasts suppresses mammary epithelial tumours.

Author

Trimboli, Anthony J., Cantemir-Stone, Carmen Z., Fu Li, Wallace, Julie A., Merchant, Anand, Creasap, Nicholas, Thompson, John C., Caserta, Enrico, Hui Wang, Chong, Jean-Leon, Naidu, Shan, Guo Wei, Sharma, Sudarshana M., Stephens, Julie A., Fernandez, Soledad A., Gurcan, Metin N., Weinstein, Michael B., Barsky, Sanford H., Yee, Lisa, and Rosol, Thomas J.

Subjects

MAMMARY gland tumors, EPITHELIAL cell tumors, FIBROBLASTS, LABORATORY mice, NEOVASCULARIZATION, PHOSPHORYLATION, BREAST cancer, CANCER cells, TUMOR growth

Abstract

The tumour stroma is believed to contribute to some of the most malignant characteristics of epithelial tumours. However, signalling between stromal and tumour cells is complex and remains poorly understood. Here we show that the genetic inactivation of Pten in stromal fibroblasts of mouse mammary glands accelerated the initiation, progression and malignant transformation of mammary epithelial tumours. This was associated with the massive remodelling of the extracellular matrix (ECM), innate immune cell infiltration and increased angiogenesis. Loss of Pten in stromal fibroblasts led to increased expression, phosphorylation (T72) and recruitment of Ets2 to target promoters known to be involved in these processes. Remarkably, Ets2 inactivation in Pten stroma-deleted tumours ameliorated disruption of the tumour microenvironment and was sufficient to decrease tumour growth and progression. Global gene expression profiling of mammary stromal cells identified a Pten-specific signature that was highly represented in the tumour stroma of patients with breast cancer. These findings identify the Pten–Ets2 axis as a critical stroma-specific signalling pathway that suppresses mammary epithelial tumours. [ABSTRACT FROM AUTHOR]

Published

2009

4. Cytomegalovirus Contributes to Glioblastoma in the Context of Tumor Suppressor Mutations.

Author

Price, Richard L., Jieun Song, Bingmer, Katherine, Tae Hyong Kim, Ji-Yeun Yi, Nowicki, Michal O., Xiaokui Mo, Hollon, Todd, Murnan, Eric, Alvarez-Breckenridge, Christopher, Fernandez, Soledad, Kaur, Balveen, Rivera, Andreana, Oglesbee, Michael, Cook, Charles, Chiocca, E. Antonio, and Chang-Hyuk Kwon

Subjects

*CYTOMEGALOVIRUS diseases, *GLIOBLASTOMA multiforme, *TUMOR suppressor genes, *GENETIC mutation, *CANCER cells

Abstract

To study the controversial role of cytomegalovirus (CMV) in glioblastoma, we assessed the effects of murine CMV (MCMV) perinatal infection in a GFAP-cre; Nf1loxP/+; Trp53+/- genetic mouse model of glioma (Mut3 mice). Early on after infection, MCMV antigen was predominantly localized in CD45+ lymphocytes in the brain with active viral replication and local areas of inflammation, but, by 7 weeks, there was a generalized loss of MCMV in brain, confirmed by bioluminescent imaging. MCMV-infected Mut3 mice exhibited a shorter survival time from their gliomas than control Mut3 mice perinatally infected with mock or with a different neurotropic virus. Animal survival was also significantly shortened when orthotopic gliomas were implanted in mice perinatally infected with MCMV versus controls. MCMV infection increased phosphorylated STAT3 (p-STAT3) levels in neural stem cells (NSC) harvested from Mut3 mice subventricular zone, and, in vivo, there was increased p-STAT3 in NSCs in MCMV-infected compared with control mice. Of relevance, human CMV (HCMV) also increased p-STAT3 and proliferation of patient-derived glioblastoma neurospheres, whereas a STAT3 inhibitor reversed this effect invitro and in vivo. These findings thus associate CMV infection to a STAT3-dependent modulatory role in glioma formation/progression in the context of tumor suppressor mutations in mice and possibly in humans. [ABSTRACT FROM AUTHOR]

Published

2013

5. Indirubins Decrease Glioma Invasion by Blocking Migratory Phenotypes in Both the Tumor and Stromal Endothelial Cell Compartments.

Author

Williams, Shanté P., Nowicki, Michal O., Fang Liu, Press, Rachael, Godlewski, Jakub, Abdel-Rasoul, Mahmoud, Kaur, Balveen, Fernandez, Soledad A., Chiocca, E. Antonio, and Lawler, Sean E.

Subjects

*CANCER cells, *GLYCOGEN, *GLYCOGEN synthase kinase-3, *PROTEIN kinases, *GLIOMAS

Abstract

Invasion and proliferation in neoplasia require the cooperation of tumor cell and endothelial compartments. Glycogen synthase kinase-3 (GSK-3) is increasingly recognized as a major contributor to signaling pathways that modulate invasion and proliferation. Here we show that GSK-3 inhibitors of the indirubin family reduce invasion of glioma cells and glioma-initiating cell-enriched neurospheres both in vitro and in vivo, and we show that β-catenin signaling plays an important role in mediating these effects. Indirubins improved survival in glioma-bearing mice in which a substantial decrease in blood vessel density was seen in treated animals. In addition, indirubins blocked migration of endothelial cells, suggesting that anti-invasive glioma therapy with GSK-3 inhibitors not only inhibits invasion of tumor cells, but blocks migration of endothelial cells, which is also in vivo required for tumor angiogenesis. Overall, our findings suggest that indirubin inhibition of GSK-3 offers a novel treatment paradigm to target 2 of the most important interacting cellular compartments in heterotypic models of cancer. Cancer Res; 71(16); 5374 80. ©2011 AACR. [ABSTRACT FROM AUTHOR]

Published

2011

6. Interferon-γ Targets Cancer Cells and Osteoclasts to Prevent Tumor-associated Bone Loss and Bone Metastases.

Author

Zhiqiang Xu, Hurchla, Michelle A., Hongju Deng, Uluçkan, Ozge, Fang Bu, Berdy, Andrew, Eagleton, Mark C., Heller, Emanuela A., Floyd, Desiree H., Dirksen, Wessel P., Sherry Shu, Tanaka, Yuetsu, Fernandez, Soledad A., Rosol, Thomas J., and Weilbaecher, Katherine N.

Subjects

*CANCER cells, *OSTEOCLASTS, *BONE cells, *INTERFERONS, *ANTINEOPLASTIC agents, *HYPERCALCEMIA, *BONE metastasis

Abstract

Interferon-γ (IFN-γ) has been shown to enhance anti-tumor immunity and inhibit the formation of bone-resorbing osteoclasts. We evaluated the role of IFN-γ in bone metastases, tumor-associated bone destruction, and hypercalcemia in human T cell lympho-trophic virus type 1-Tax transgenic mice. Compared with Tax+IFN-γ+/+ mice, Tax+IFN-γ-/- mice developed increased osteolytic bone lesions and soft tissue tumors, as well as increased osteoclast formation and activity. In vivo administration of IFN-γ to tumor-bearing Tax+IFN-γ-/- mice prevented new tumor development and resulted in decreased bromodeoxyuridine uptake by established tumors. In vitro, IFN-γ directly decreased the viability of Tax+ tumor cells through inhibition of proliferation, suppression of ERK phosphorylation, and induction of apoptosis and caspase 3 cleavage. IFN-γ also inhibited macrophage colony- stimulating factor-mediated proliferation and survival of osteoclast progenitors in vitro. Administration of IFN-γ to C57BL/6 mice decreased Tax+ tumor growth and prevented tumor-associated bone loss and hypercalcemia. In contrast, IFN-γ treatment failed to protect IFN-γRF-/- mice from Tax+ tumor-induced skeletal complications, despite decreasing tumor growth. These data demonstrate that IFN-γ suppressed tumor-induced bone loss and hypercalcemia in Tax+ mice by inhibiting both Tax+ tumor cell growth and host-induced osteolysis. These data suggest a protective role for IFN-γ in patients with bone metastases and hypercalcemia of malignancy. [ABSTRACT FROM AUTHOR]

Published

2009

7. Human bone marrow stromal cells enhance breast cancer cell growth rates in a cell line-dependent manner when evaluated in 3D tumor environments

Author

Sasser, A. Kate, Mundy, Bethany L., Smith, Kristen M., Studebaker, Adam W., Axel, Amy E., Haidet, Amanda M., Fernandez, Soledad A., and Hall, Brett M.

Subjects

*BREAST cancer, *CELL culture, *CANCER cells, *PROSPECTING

Abstract

Abstract: Our understanding of the impact that fibroblasts have on cancer cell behavior in vivo has been limited by the complexities of in vivo tumor microenvironments, which contain many distinct cell populations that influence tumor growth and survival. Herein, we describe a novel, three-dimensional (3D), in vitro, fluorometric, Tumor Growth Assay (TGA) that allows for non-invasive measurements of cancer cell expansion in the presence of multiple tumor-associated cell types or soluble factors, while embedded in Cultrex® or Matrigel™ Basement Membrane Extract (BME). Using this assay, we investigated the direct biological impact of primary human bone marrow stromal cells (hMSC) on the growth rates of a panel of metastatic breast cancer cell lines. Human MSC can be readily isolated from bone marrow, a principle site of breast cancer metastasis, and were found to significantly enhance the growth rate of MCF-7 (P-value<0.0001), an estrogen receptor-alpha (ERα) positive breast cancer cell line, in a soluble factor-dependent manner. MSC paracrine factors also enhanced the growth of other ERα positive breast cancer cell lines including T47D, BT474, and ZR-75-1 (P-value<0.05). In contrast, the ERα negative cell line MDA-MB-231 was unaffected by hMSC and the growth rate of another ERα negative cell line MDA-MB-468 was elevated in the presence of hMSC, albeit to a lesser extent than MCF-7 or the other ERα positive cell lines tested. [Copyright &y& Elsevier]

Published

2007

8. The Histone Deacetylase Inhibitor Valproic Acid Lessens NK Cell Action against Oncolytic Virus-Infected Glioblastoma Cells by Inhibition of STAT5/T-BET Signaling and Generation of Gamma Interferon.

Author

Alvarez-Breckenridge, Christopher A., Jianhua Yu, Price, Richard, Min Wei, Yan Wang, Nowicki, Michal O., Ha, Yoonhee P., Bergin, Stephen, Christine Hwang, Fernandez, Soledad A., Kaur, Balveen, Caligiuri, Michael A., and Chiocca, E. Antonio

Subjects

*HISTONE deacetylase inhibitors, *VALPROIC acid, *KILLER cells, *GLIOBLASTOMA multiforme, *CANCER cells, *INTERFERONS, *CELLULAR signal transduction, *LABORATORY mice

Published

2012