The Role of Differential Phosphorylation of the Retinoblastoma Protein in Regulating Cell Proliferation and Elastogenesis

Sen, Sanjana

25 August 2011

Previous studies suggest that the IGF-I stimulates the elastin gene transcription through the unique responsive sequence on the elastin promoter, which is a putative retinoblastoma control element (RCE). This site interacts with (Sp)-family transcription factors whose delivery is mediated by the retinoblastoma protein (Rb). Since Rb (phosphorylated on serine 780) has been implicated in the initiation of the cell cycle, we speculated that a different phosphorylation of Rb might determine Rb involvement in elastogenesis. Obtained results demonstrated that, IGF-I-induced elastogenic signaling pathway in human dermal fibroblasts includes activation of cyclinE/cdk2 causing a site specific phosphorylation of Rb on threonine 821. This permits the sequestration of Sp1 by Rb before it could bind the elastin promoter, thereby allowing the elastin gene transcription. We also found that blocking of H-Ras in Costello syndrome fibroblasts (characterized by heightened proliferation and impaired elastogenesis), selectively down-regulated Rb phosphorylation on serine 780 and normalized impaired elastogenesis.

Elastin

Retinoblastoma protein

Cell proliferation

Retinoblastoma control element

Cyclin E

Cyclin D

cdk-2

cdk-4

Costello Syndrome

Serine 780

Threonine 821

Elastin gene promoter

Sp-1

0307

Incorporation of recombinant fibronectin into genetically engineered elastin-based polymers

Balderrama, Fanor Alberto

17 November 2009

Cardiovascular disease is the main cause of death in the United States. Many of these conditions require the grafting or bypassing of compromised blood vessels. To this effect, biological vascular grafts (autografts and allografts) are the first line of action. However, when the patient lacks vasculature suitable for grafting use, several synthetic grafting options are available. The search for an inert biomaterial for vascular grafts has proven to be unsuccessful. This makes the interaction taking place on the blood-biomaterial interface critical for the success of the grafts. This thesis introduces a new bio-inspired approach to tackle the mechanical and biological challenges of vascular material design. The hypothesis of this research is that recombinant fibronectin protein can be stably incorporated onto elastin-mimetic polymers to increase endothelialization. Recombinant elastin, designed to recreate the mechanical properties of natural elastin as a candidate material for vascular graft fabrication, was used as a model surface. Recombinant fibronectin-functionalized elastin-mimetic polymer displayed significant improvement in cell adhesion. Quantification of surface bound recombinant fibronectin verified the concentration dependence of this cell adhesive behavior. Modified elastin-mimetic polymer also demonstrated an enhanced ability to support endothelial cell proliferation. Furthermore, the stability of recombinant fibronectin-modified polymers was assessed. These studies provide the foundation for fabricating elastin-mimetic vascular grafts with improved endothelialization and subsequent biological performance.

Functionalization

Coating

Protein

Crosslinking

Genipin

HUVEC

Stability

Cell proliferation

Vascular graft

Elastin

FNIII7-10

Cell adhesion

Endothelialization

Endothelial

Fibronectins

Globulins

Biomedical materials

Vascular grafts

Interaction of the anti-apoptotic protein BAG-1 with the vitamin D receptor /

Witcher, Michael,

January 1999

Thesis (M.Sc.)--Memorial University of Newfoundland, Faculty of Medicine, 1999. / Bibliography: leaves 98-114.

L’étude du rôle d’ARF1 dans la migration et la prolifération des cellules du cancer du sein

Boulay, Pierre-Luc

09 1900

Les facteurs d’ADP-ribosylation (ARFs) sont des petites GTPases impliquées dans le transport vésiculaire, la synthèse des lipides membranaires et la réorganisation du cytosquelette d’actine. Les isoformes 1 (ARF1) et 6 (ARF6) sont les plus étudiées. ARF1 est connue pour être distribuée à l’appareil de Golgi, alors qu’ARF6 est confinée principalement à la membrane plasmique. Récemment, il a été démontré qu’ARF6 est hautement exprimée et activée dans plusieurs cellules de cancer du sein invasif et que celle-ci contrôle les processus de migration et d’invasion. Cependant, le rôle d’ARF1 dans ces processus biologiques impliqués dans la formation de métastases du cancer du sein demeure méconnu. Dans la présente étude, nous avons utilisé comme modèle d’étude pour ARF1 les MDA-MB-231, une lignée de cellules invasives du cancer du sein exprimant de haut niveau de récepteurs au facteur de croissance épidermique (EGFR). Afin d’évaluer le rôle d’ARF1 dans la migration, dans la transition épithéliale mésenchymateuse (EMT) et dans la prolifération cellulaire, nous avons procédé à deux types d’approches expérimentales, soit l’inhibition de l’expression endogène d’ARF1 par l’interférence à l’ARN de même que la surexpression de formes mutantes dominante négative (ARF1T31N) et constitutivement active d’ARF1 (ARF1Q71L), qui miment les formes inactive et active de la GTPase, respectivement. De manière intéressante, la suppression d’ARF1 et la surexpression de la forme inactive d’ARF1 induisent l’arrêt de la migration et de la prolifération des MDA-MB-231 de manière dépendante à l’activation de l’EGFR et ce, en bloquant l’activation de la voie PI3Kinase. De plus, nous démontrons qu’ARF1, de même que les ARF GEFs Cytohésine-1 et Cytohésine-2, contribuent au phénotype invasif des cellules tumorales de cancer du sein. Dans les mêmes approches expérimentales, nous montrons que l’inactivation d’ARF1 dans les MDA-MB-231 déclenche un arrêt de croissance irréversible associé à l’induction de la sénescence et ce, en régulant la fonction de la protéine du rétinoblastome pRb. Enfin, cette étude a permis de mettre en évidence le rôle physiologique d’ARF1 dans les processus de migration et de prolifération cellulaire, deux événements biologiques responsables de la progression du cancer du sein. / The ADP-ribosylation factors (ARFs) are small GTPases involved in vesicular transport, lipids synthesis and cytoskeleton remodelling. The isoforms 1 (ARF1) and 6 (ARF6) are the most studied. ARF1 is classically distributed at the Golgi apparatus whereas ARF6 is found at the plasma membrane and onto recycling endosomes. It was recently demonstrated that ARF6 is highly expressed and activated in several breast cancer cell lines and is associated with enhanced migration and invasiveness. However, the role of ARF1, in these biologicals processes necessary for metastasis formation, remains unclear. In this study, we used MDA-MB-231 cells, an invasive breast cancer cell line, that expressed high levels of EGFR (Epidermal Growth Factor Receptor) to investigate the role of ARF1 in migration and proliferation. To further establish the role of ARF1 in cell migration, EMT and proliferation, we used two experimental approaches. First, we decreased endogenous ARF1 expression by RNA interference and second we overexpressed the dominant negative (ARF1T31N) and constitutively active (ARF1Q71L) ARF1 mutants, which mimick the inactive and active forms of ARF1, respectively. We demonstrated that depletion of ARF1 as well as overexpression of the inactive form of ARF1 blocked EGFR-mediated cell migration and proliferation by inhibiting the activation of PI3Kinase. Moreover, we showed, using invasive and non invasive breast cancer cell lines, that ARF1 and both Cytohesin-1 and Cytohesin-2 are required for invasivness. Using similar approaches, we reported that inactivation of ARF1 in MDA-MB-231 cells promotes cell growth arrest associated to senescence program by regulating the function of the Retinoblastoma protein pRb. Altogether, these findings demonstrate a physiological role for ARF1 in cell migration and proliferation. These two biologicals events are necessary for breast cancer progression.

ARF1

cell proliferation

EGFR

PI3Kinase

Cytohésine-1

Cytohésine-2

pRb

migration

prolifération

Cytohesin-1

Cytohesin-2

cell migration

Immune Dysfunction Associated with Hemodialysis Modalities

Slatculescu, Andreea M.

24 January 2014

Infection is a leading cause of death in hemodialysis patients, partly due to dysfunctional immunity. Frequent dialysis therapy improves patient outcomes and quality of life. We hypothesize that extended home hemodialysis (EHHD) also improves immune function compared to conventional in-hospital hemodialysis (CHD); therefore, we designed a prospective matching-cohort clinical study to assess serum inflammatory markers and the functional capacity of monocyte-derived dendritic cells (MDDCs) and T-lymphocytes. Serum CRP was decreased in EHHD patients suggesting that extended dialysis may decrease inflammatory solute/cytokine levels. Compared to controls, MDDCs from hemodialysis patients had similar endocytic capacity, expression of co-stimulatory molecules, and T-cell activation capacity. However, CHD was associated with the highest expression of CD83 and CD40. Activated T-cells in CHD patients also produced significantly more immunosuppressive IL-10 compared to EHHD patients and controls. Therefore, EHHD may improve immune function by decreasing inflammation, MDDC pre-activation, and synthesis of immunosuppressive cytokines.

Hemodialysis

Dialysis

Home Hemodialysis

Adaptive immunity

Monocyte-derived dendritic cells

T-lymphocytes

Serum cytokines

C reactive protein

co-stimulatory molecules

FITC-dextran endocytosis

Flow Cytometry

Cell proliferation

Delineating epigenetic regulatory mechanisms of cell profileration and differentiation

Islam, Abul, 1978-

25 June 2012

Recent advances in high throughput technology have opened the door to systematic studies of epigenetic mechanisms. One of the key components in the regulation of the cell cycle and differentiation is the retinoblastoma protein (pRB), a component of the RB/E2F tumor suppressor pathway that is frequently deregulated in cancer. The RBP2/KDM5A histone demethylase was shown to interact with pRB and regulate pRB function during differentiation. However, how precisely differentiation is coupled with halted cell cycle progression and whether an epigenetic mechanism is involved remain unknown. In the present study, I analyzed gene expression levels of human histone methyltransferases (HMT) and demethylases (HDM), as well as their targets in human cancers; and focused on RB/KDM5A connection in control of cell cycle and differentiation. In particular, I used Drosophila as a model to describe a novel mechanism where the RB/E2F pathway interacts with the Hippo tumor suppressor pathway to synergistically control cell cycle exit upon differentiation. Studying the role of miR-11, I found that the inhibition of dE2F1-induced cell death is its highly specialized function. Furthermore, I studied the induction of differentiation and apoptosis as the consequences of KDM5A deletion in cells derived from Rb knockout mice. I concluded that during differentiation, KDM5A plays a critical role at the enhancers of cell type-specific genes and at the promoters of E2F targets; in cooperation with other repressor complexes, it silences cell cycle genes. I found that KDM5A binds to transcription start sites of the majority of genes with H3K4 methylation. These are highly expressed genes, involved in certain biological processes, and occupied by KDM5A in an isoform-specific manner. KDM5A plays a unique and non-redundant role in histone demethylation and its promoter binding pattern highly overlaps with the opposing enzyme, MLL1. Finally, I found that HMT and HDM enzymes exhibit a distinct co-expression pattern in different cancer types, and this determines the level of expression of their target genes. / Los avances recientes en las tecnologías de alto flujo han abierto el camino a los estudios sistemáticos de los mecanismos epigenéticos. La proteína retinoblastoma (pRB), uno de los elementos de la ruta de supresión de tumores RB/E2F que se encuentra desregulado con frecuencia en el cáncer, es uno de los componentes esenciales de la regulación del ciclo celular y la diferenciación. Sin embargo, aún no se conoce de qué manera precisa la diferenciación se acopla a la detención del avance del ciclo celular y si hay algún mecanismo epigenético vinculado a este proceso. En este estudio, he analizado los niveles de expresión de histona metiltransferasas (HMT) y desmetilasas humanas (HDM), así como sus dianas en cánceres humanos, y me he centrado en la conexión de RB/KDM5A en el control del ciclo celular y la diferenciación. Específicamente, utilicé Drosophila como modelo para describir un mecanismo nuevo mediante el cual RB/E2F interactúa con la ruta Hippo de supresión de tumores para controlar de manera sinérgica la detención del ciclo celular relacionada con la diferenciación. Mediante la investigación del papel de miR-11, determiné que su función altamente especializada es la inhibición de la muerte celular inducida por dE2F1. Además, estudié la inducción de la diferenciación y la apoptosis como consecuencia de la pérdida de KDMA5 en células obtenidas a partir de ratones sin Rb. Extraje como conclusión que, durante la diferenciación, KDMA5 desempeña un papel esencial sobre los estimuladores de los genes específicos de los tipos celulares, así como en los promotores de las dianas de E2F; en cooperación con otros complejos represores silencia a los genes del ciclo celular. Investigué el mecanismo de reclutamiento de KDM5A y encontré que se une al sitio de inicio de la transcripción de la mayoría de los genes que poseen metilación en H3K4. Estos genes tienen elevados niveles de expresión, están involucrados en determinados procesos biológicos y están ocupados por diferentes isoformas de KDM5A. KDM5A desempeña un papel único y no redundante en la desmetilación de las histonas y que en gran medida se solapa con la enzima con la función opuesta, MLL1. Para terminar, encontré que las enzimas HMT y HDM muestran patrones de co-expresión distintos en diferentes tipos de cáncer, y que este hecho determina los niveles de expresión de sus genes diana.

Histone modifying enzymes

KDM5A/RBP2/JARID1A

RB/E2F

Hippo

miR-11

Cell proliferation

Differentiation

Bioinformatics

Oncogenomics

Epigenetics

Enzimas modificadoras de histonas

Proliferación celular

Diferenciación

Bioinformática

Oncogenómica

Epigenética

576

Mediation of Osteoblast Responses to Titanium Roughness by Adsorbed Proteins

Wilson, Cameron

January 2005

Stable fixation of implants such as artificial teeth depends on the direct apposition of bone to the implanted material. While endosseous implants were traditionally allowed to "osseointegrate" over several months without carrying load, clinical and experimental data show that prostheses with roughened surfaces allow successful integration when subject to earlier loading and more challenging implant sites. However, to design implant surfaces for an optimal biological response requires an understanding of the mechanism by which roughened surfaces promote osseointegration. Research into this mechanism has, to date, focussed primarily on the response of osteoblastic cells to surface topography in vitro. While these have demonstrated some consistent trends in cell behaviour, the fundamental means by which cells sense and respond to roughness remain unclear. It has been suggested that cell responses to changes in topography may relate to differences in the proteins adsorbed from serum (in vitro). While experimental evidence indirectly suggests that physical features can affect protein adsorption, few studies have examined this with respect to surface roughness, particularly as a mediator of cell responses. To address this issue, cell culture and protein adsorption experiments were conducted on a limited range of surface textures. Titanium samples were ground to produce morphologically similar surfaces with three grades of roughness. A duplicate set of specimens were heated at 600°C for one hour, with the aim of masking potential variations in physicochemical properties with differing degrees of grinding. Osteoblast attachment and proliferation studies were conducted over a short time-frame of 48 hours or less, to highlight the effects of proteins adsorbed from serum rather than secreted by adherent cells. Gel electrophoresis provided a profile of the proteins adsorbed to each surface after 15 minutes, corresponding to the time by which the cells had settled onto the surface. Finally, confocal microscopy was used to examine cell morphology on each surface, and to visualize specific interactions between cellular structures and adsorbed adhesion-mediating proteins. Although the effects were inconsistent, attachment assays showed some indications that fewer cells attached in the first 90 minutes as roughness increased. This inverse cell number-roughness trend was significant at 48 hours; however, the variability in attachment assays prevented reliable separation of attachment and proliferation rate effects. While the reduction in cell number with increasing roughness is consistent with previous reports, it is typically observed at later time points, and thus may be increasingly confounded by contact inhibition and differentiation. Thermal oxidation of the titanium did not impact on osteoblast responses to roughness, although it significantly slowed cell proliferation. The latter result was unexpected on the basis of previous reports. One-dimensional gel electrophoresis revealed no significant differences in the composition of adsorbed layers with variations in roughness. However, as expected on account of wettability changes, the heat-treatment did correspond to significant changes in the adsorption profile. While this was not a highly sensitive analysis, it suggests that the cell responses to roughness changes were not governed by broadscale differences in the proteins initially available to adhering cells. In addition to the composition of the adsorbed layer, the distribution of proteins may also vary with topography. The immunofluorescence methods were not sufficiently sensitive to reveal the distribution of adsorbed adhesion proteins (vitronectin and fibronectin). However, the lack of clear labelling does suggest an absence of large accumulations due to specific topographic features. Further work is required to address this issue conclusively. Observations of cell morphology were consistent with widely-reported contact guidance phenomena on grooved surfaces, with elongation and alignment (with topography) increasing with groove depth. Cell elongation was also enhanced on the more hydrophilic, heat-treated titanium, but this effect diminished over time. Although increased elongation at 90 minutes corresponded to lower cell numbers at 48 hours, no causal relationship has yet been established.

Biomaterials

Cell attachment

Cell morphology

Cell proliferation

Cell spreading

Fibronectin

Heat treatment

Osteoblasts

Protein adsorption

Roughness

Surface topography

Thermal oxidation

Titanium

Vitronectin.

Multiple modes of MDMX regulation affect p53 activation

Gilkes, Daniele M.

January 2008

Dissertation (Ph.D.)--University of South Florida, 2008. / Title from PDF of title page. Document formatted into pages; contains 197 pages. Includes vita. Includes bibliographical references.

Characterization of the dopaminergic potential of the human NTera2/d1 (NT2) cell line in vitro /

Misiuta, Iwona E.

January 2005

Thesis (Ph.D.)--University of South Florida, 2005. / Includes vita. Includes bibliographical references. Also available online.

Control of endothelial cell differentiation and proliferation for vascular tissue engineering /

Nourse, Marilyn Brower,

January 2007

Thesis (Ph. D.)--University of Washington, 2007. / Vita. Includes bibliographical references (leaves 117-139).