Your search keyword '"Ashby WJ"' showing total 8 results

1. Abstract P3-05-09: The role of TGF-beta receptor type 3 in breast cancer progression

Author

Jovanovic, B, primary, Ashby, WJ, additional, Zijlstra, A, additional, Pietenpol, JA, additional, and Moses, HL, additional

Published

2012

2. Transforming growth factor beta receptor type III is a tumor promoter in mesenchymal-stem like triple negative breast cancer.

Author

Jovanović B, Beeler JS, Pickup MW, Chytil A, Gorska AE, Ashby WJ, Lehmann BD, Zijlstra A, Pietenpol JA, and Moses HL

Subjects

Animals, Cell Line, Tumor, Cell Movement genetics, Cell Proliferation, Cell Survival genetics, Cell Transformation, Neoplastic genetics, Cluster Analysis, Disease Models, Animal, Female, Gene Expression, Gene Expression Profiling, Gene Expression Regulation, Neoplastic, Gene Knockdown Techniques, Heterografts, Humans, Integrin alpha2 genetics, Mesenchymal Stem Cells pathology, Mice, RNA, Messenger genetics, RNA, Messenger metabolism, RNA, Small Interfering, Spheroids, Cellular, Tumor Burden, Tumor Cells, Cultured, Proteoglycans genetics, Receptors, Transforming Growth Factor beta genetics, Triple Negative Breast Neoplasms genetics, Triple Negative Breast Neoplasms pathology

Abstract

Introduction: There is a major need to better understand the molecular basis of triple negative breast cancer (TNBC) in order to develop effective therapeutic strategies. Using gene expression data from 587 TNBC patients we previously identified six subtypes of the disease, among which a mesenchymal-stem like (MSL) subtype. The MSL subtype has significantly higher expression of the transforming growth factor beta (TGF-β) pathway-associated genes relative to other subtypes, including the TGF-β receptor type III (TβRIII). We hypothesize that TβRIII is tumor promoter in mesenchymal-stem like TNBC cells., Methods: Representative MSL cell lines SUM159, MDA-MB-231 and MDA-MB-157 were used to study the roles of TβRIII in the MSL subtype. We stably expressed short hairpin RNAs specific to TβRIII (TβRIII-KD). These cells were then used for xenograft tumor studies in vivo; and migration, invasion, proliferation and three dimensional culture studies in vitro. Furthermore, we utilized human gene expression datasets to examine TβRIII expression patterns across all TNBC subtypes., Results: TβRIII was the most differentially expressed TGF-β signaling gene in the MSL subtype. Silencing TβRIII expression in MSL cell lines significantly decreased cell motility and invasion. In addition, when TβRIII-KD cells were grown in a three dimensional (3D) culture system or nude mice, there was a loss of invasive protrusions and a significant decrease in xenograft tumor growth, respectively. In pursuit of the mechanistic underpinnings for the observed TβRIII-dependent phenotypes, we discovered that integrin-α2 was expressed at higher level in MSL cells after TβRIII-KD. Stable knockdown of integrin-α2 in TβRIII-KD MSL cells rescued the ability of the MSL cells to migrate and invade at the same level as MSL control cells., Conclusions: We have found that TβRIII is required for migration and invasion in vitro and xenograft growth in vivo. We also show that TβRIII-KD elevates expression of integrin-α2, which is required for the reduced migration and invasion, as determined by siRNA knockdown studies of both TβRIII and integrin-α2. Overall, our results indicate a potential mechanism in which TβRIII modulates integrin-α2 expression to effect MSL cell migration, invasion, and tumorigenicity.

Published

2014

3. Established and novel methods of interrogating two-dimensional cell migration.

Author

Ashby WJ and Zijlstra A

Subjects

Biophysical Phenomena, Cell Count, Cytological Techniques methods, Electric Impedance, Magnetics, Microfluidic Analytical Techniques, Models, Biological, Systems Biology, Cell Movement physiology

Abstract

The regulation of cell motility is central to living systems. Consequently, cell migration assays are some of the most frequently used in vitro assays. This article provides a comprehensive, detailed review of in vitro cell migration assays both currently in use and possible with existing technology. Emphasis is given to two-dimensional migration assays using densely organized cells such as the scratch assay. Assays are compared and categorized in an outline format according to their primary biological readout and physical parameters. The individual benefits of the various methods and quantification strategies are also discussed. This review provides an in-depth, structured overview of in vitro cell migration assays as a means of enabling the reader to make informed decisions among the growing number of options available for their specific cell migration application.

Published

2012

4. Magnetically attachable stencils and the non-destructive analysis of the contribution made by the underlying matrix to cell migration.

Author

Ashby WJ, Wikswo JP, and Zijlstra A

Subjects

Cell Culture Techniques, Cell Line, Tumor, Elasticity, Extracellular Matrix chemistry, Humans, Cell Movement physiology, Magnets

Abstract

Cell migration is controlled by the integration of numerous distinct components. Consequently, the analysis of cell migration is advancing towards comprehensive, multifaceted in vitro models. To accurately evaluate the contribution of an underlying substrate to cell motility in complex cellular environments we developed a migration assay using magnetically attachable stencils (MAts). When attached to a culture surface, MAts create a defined void in the cell monolayer without disrupting the cells or damaging the underlying substrate. Quantitative analysis of migration into this void reveals the substrate's contribution to migration. The magnetically-guided placement of a microfabricated stencil allows for full experimental control of the substrate on which migration is analyzed. MAts enable the evaluation of intact, defined matrix, and make it possible to analyze migration on unique surfaces such as micropatterned proteins, nano-textured surfaces, and pliable hydrogels. These studies also revealed that mechanical disruption, including the damage that occurs during scratch assays, diminishes migration and confounds the analysis of individual cell behavior. Analysis of migration on increasingly complex biomaterials reveals that the contribution of the underlying matrix depends not only on its molecular composition but also its organization and the context in which it is presented., (Copyright © 2012 Elsevier Ltd. All rights reserved.)

Published

2012

5. Lack of transforming growth factor-β signaling promotes collective cancer cell invasion through tumor-stromal crosstalk.

Author

Matise LA, Palmer TD, Ashby WJ, Nashabi A, Chytil A, Aakre M, Pickup MW, Gorska AE, Zijlstra A, and Moses HL

Subjects

Animals, Cadherins metabolism, Cell Line, Tumor, Cell Movement, Epithelial-Mesenchymal Transition genetics, Fibroblasts metabolism, Gene Expression Regulation, Neoplastic, Gene Knockout Techniques, Humans, Intercellular Junctions metabolism, Mice, Neoplasms genetics, Phenotype, Protein Serine-Threonine Kinases metabolism, Protein Transport, Receptor, Transforming Growth Factor-beta Type II, Receptors, Transforming Growth Factor beta metabolism, Transforming Growth Factor beta genetics, beta Catenin metabolism, Cell Communication, Neoplasms metabolism, Neoplasms pathology, Signal Transduction, Stromal Cells metabolism, Transforming Growth Factor beta metabolism

Abstract

Introduction: Transforming growth factor beta (TGF-β) has a dual role during tumor progression, initially as a suppressor and then as a promoter. Epithelial TGF-β signaling regulates fibroblast recruitment and activation. Concurrently, TGF-β signaling in stromal fibroblasts suppresses tumorigenesis in adjacent epithelia, while its ablation potentiates tumor formation. Much is known about the contribution of TGF-β signaling to tumorigenesis, yet the role of TGF-β in epithelial-stromal migration during tumor progression is poorly understood. We hypothesize that TGF-β is a critical regulator of tumor-stromal interactions that promote mammary tumor cell migration and invasion., Methods: Fluorescently labeled murine mammary carcinoma cells, isolated from either MMTV-PyVmT transforming growth factor-beta receptor II knockout (TβRII KO) or TβRIIfl/fl control mice, were combined with mammary fibroblasts and xenografted onto the chicken embryo chorioallantoic membrane. These combinatorial xenografts were used as a model to study epithelial-stromal crosstalk. Intravital imaging of migration was monitored ex ovo, and metastasis was investigated in ovo. Epithelial RNA from in ovo tumors was isolated by laser capture microdissection and analyzed to identify gene expression changes in response to TGF-β signaling loss., Results: Intravital microscopy of xenografts revealed that mammary fibroblasts promoted two migratory phenotypes dependent on epithelial TGF-β signaling: single cell/strand migration or collective migration. At epithelial-stromal boundaries, single cell/strand migration of TβRIIfl/fl carcinoma cells was characterized by expression of α-smooth muscle actin and vimentin, while collective migration of TβRII KO carcinoma cells was identified by E-cadherin+/p120+/β-catenin+ clusters. TβRII KO tumors also exhibited a twofold greater metastasis than TβRIIfl/fl tumors, attributed to enhanced extravasation ability. In TβRII KO tumor epithelium compared with TβRIIfl/fl epithelium, Igfbp4 and Tspan13 expression was upregulated while Col1α2, Bmp7, Gng11, Vcan, Tmeff1, and Dsc2 expression was downregulated. Immunoblotting and quantitative PCR analyses on cultured cells validated these targets and correlated Tmeff1 expression with disease progression of TGF-β-insensitive mammary cancer., Conclusion: Fibroblast-stimulated carcinoma cells utilize TGF-β signaling to drive single cell/strand migration but migrate collectively in the absence of TGF-β signaling. These migration patterns involve the signaling regulation of several epithelial-to-mesenchymal transition pathways. Our findings concerning TGF-β signaling in epithelial-stromal interactions are important in identifying migratory mechanisms that can be targeted as recourse for breast cancer treatment.

Published

2012

6. Targeting tumor cell motility to prevent metastasis.

Author

Palmer TD, Ashby WJ, Lewis JD, and Zijlstra A

Subjects

Animals, Cell Adhesion, Cell Communication, Humans, Neoplasm Metastasis prevention & control, Neoplasms pathology, Cell Movement drug effects, Drug Delivery Systems, Neoplasms drug therapy

Abstract

Mortality and morbidity in patients with solid tumors invariably result from the disruption of normal biological function caused by disseminating tumor cells. Tumor cell migration is under intense investigation as the underlying cause of cancer metastasis. The need for tumor cell motility in the progression of metastasis has been established experimentally and is supported empirically by basic and clinical research implicating a large collection of migration-related genes. However, there are few clinical interventions designed to specifically target the motility of tumor cells and adjuvant therapy to specifically prevent cancer cell dissemination is severely limited. In an attempt to define motility targets suitable for treating metastasis, we have parsed the molecular determinants of tumor cell motility into five underlying principles including cell autonomous ability, soluble communication, cell-cell adhesion, cell-matrix adhesion, and integrating these determinants of migration on molecular scaffolds. The current challenge is to implement meaningful and sustainable inhibition of metastasis by developing clinically viable disruption of molecular targets that control these fundamental capabilities., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2011

7. Single-photon-counting detector for increased sensitivity in two-photon laser scanning microscopy.

Author

Benninger RK, Ashby WJ, Ring EA, and Piston DW

Subjects

Animals, Humans, Islets of Langerhans pathology, Microscopy, Confocal instrumentation, Microscopy, Fluorescence instrumentation, NAD chemistry, NADP chemistry, Optics and Photonics, Scattering, Radiation, Lasers, Microscopy, Confocal methods, Microscopy, Fluorescence methods, Photons

Abstract

We present the use and characterization of a photon-counting detector for increased sensitivity at low signal levels in fluorescence laser scanning microscopy (LSM). Conventional LSM photomultiplier tube detectors utilize analog current integration and thus suffer from excessive noise at low signal levels, introduced during current measurement. In this Letter we describe the implementation of a fast single-photon-counting (SPC) detector on a conventional two-photon laser scanning microscope and detail its use in imaging low fluorescence intensities. We show that for a low photon flux, the SPC detector is shot-noise limited and thus provides increased detection sensitivity compared with analog current integration.

Published

2008

8. Biomedical engineering at King's College Hospital.

Author

Roberts VC, Sabri S, Cotton LT, Ashby WJ, Cave FD, Higgins RF, Frewer RA, and Brand PJ

Subjects

Animals, Arteries surgery, Blood Flow Velocity, Curriculum, Education, Medical, Fiber Optic Technology, Financing, Organized, Health Facility Size, Humans, London, Postoperative Complications prevention & control, Thrombophlebitis prevention & control, Varicose Veins etiology, Vascular Diseases surgery, Biomedical Engineering education, Hospitals, Teaching

Published

1971