The effects of bleomycin, mitomycin C, and cytoskeletal-disrupting drugs on angiogenesis in vitro and haemangioma development in vivo

Mabeta, Peaceful Lucy

22 January 2009

Angiogenesis, the process of new vessel formation, appears to be a central mechanism that underlies the development of haemangiomas. Recently, intralesional bleomycin injection was used to treat paediatric haemangiomas with very good results. The purpose of this study was to determine whether there was significant systemic circulatory spill-over of bleomycin in haemangioma patients treated with intralesional bleomycin to determine safety of use. Furthermore, in order to elucidate bleomycin’s mechanism of action in inducing haemangioma regression, this study aimed at determining the effects of bleomycin on aspects of angiogenesis, namely, endothelial cell migration, growth and apoptosis, and comparing these effects with those of drugs previously reported to inhibit various aspects of the angiogenic process (mitomycin C, 2-methoxyestradiol, taxol, vincristine, vinblastine, colchicine, nocodazole and cytochalasin D). Lastly, the effects of bleomycin, mitomycin C, 2-methoxyestradiol, taxol, vincristine, vinblastine, colchicine, nocodazole and cytochalasin D were studied in an animal haemangioma model. A rapid and highly sensitive high performance liquid chromatographic (HPLC) method was developed. Blood samples were collected from four haemangioma patients before and after (over a 24 hour period) intralesional bleomycin (IB) therapy. As a control, blood samples were also collected at identical time intervals from four patients undergoing intravenous (IV) bleomycin chemotherapy for various malignant tumours. The HPLC method was used to quantitate bleomycin fractions in patient samples. The mean bleomycin concentration detected in plasma samples obtained from IB treated patients was 0.00 ìg/ml for both bleomycin A<Sub>2 and B2 over the 24-hour period following therapy. Plasma bleomycin A2 and B2 levels of 360.79 and 158.85 ìg/ml respectively were detected in samples obtained from cancer patients treated with bleomycin IV. These findings indicate that the low levels detected may translate to a significantly lesser risk of pulmonary fibrosis following IBI. The effect of drugs on endothelial cell migration was analyzed by wounding a confluent monolayer of cells and determining the number of cells that had migrated from the wound edge. Endothelial cell growth was determined in cells treated with various drug concentrations while apoptosis was examined using hematoxylin and eosin staining, DNA fragmentation assay and acridine orange staining. The effect of test drugs on in vitro angiogenesis was determined on endothelial cells induced to form capillary-like tubes in collagen gel. Test drugs were then evaluated for antitumour activity in an animal haemangioma model. Data demonstrated that test drugs inhibited endothelial cell migration, with the exception of mitomycin C. All test drugs induced a reduction in the percentage of viable endothelial cell in a dose-dependant manner, and also induced endothelial cell apoptosis. The drugs inhibited angiogenesis in vitro and inhibited tumour development in vivo with varying potency. In general, results from this study indicated that there was negligible systemic spill-over of bleomycin following IB administration in patients with haemangiomas, suggesting a much lesser risk of developing bleomycin-induced pulmonary fibrosis. This study also showed that test drugs inhibited angiogenesis in vitro and haemangioma development in vivo in a mouse model. Taken together, these observations demonstrate that bleomycin may inhibit haemangioma growth by inhibiting angiogenesis. In addition, mitomycin C, 2-methoxyestradiol, taxol, vincristine, vinblastine, colchicine, nocodazole and cytochalasin D may have potential in the treatment of haemangiomas of infancy, and should be investigated further in a murine haemangioma model to determine effective dose schedules. / Thesis (PhD)--University of Pretoria, 2009. / Physiology / unrestricted

Cell growth

Angiogenesis

Cell migration

Basic fibroblast growth factor

Polyoma middle t oncogene

Vascular endothelial growth factor

Cytoskeletal-disrupting agents

Vascular tumour

Haemangioma

Bleomycin

Haemangioma

Endothelial cells

UCTD

Host-parasite interactions in the dissemination of Toxoplasma gondii

Kanatani, Sachie

January 2017

Toxoplasma gondii is an obligate intracellular parasite that infects virtually all warm-blooded organisms. Systemic dissemination of T. gondii in the organism can cause life-threatening infection that manifests as Toxoplasma encephalitis in immune-compromised patients. In addition, mounting evidence from epidemiological studies indicates a link between chronic Toxoplasma infection and mental disorders. To better understand the pathogenesis of toxoplasmosis, basic knowledge on the host-parasite interactions and the dissemination mechanisms are essential. Previous findings have established that, upon infection with T. gondii, dendritic cells (DCs) and microglia exhibit enhanced migration, which was termed the hypermigratory phenotype. As a result of this enhanced migration, DCs and microglia are used as vehicle cells for dissemination (‘Trojan horse’) which potentiates dissemination of T. gondii in mice. However, the precise mechanisms behind the hypermigratory phenotype remained unknown. In this thesis, we characterized host-parasite interactions upon infection with T. gondii and investigated the basic mechanisms behind the hypermigratory phenotype of T. gondii-infected DCs and microglia. In paper I, we observed that upon infection with T. gondii, DCs underwent rapid morphological changes such as loss of adhesiveness and podosomes, with integrin redistribution. These rapid morphological changes were linked to hypermotility and were induced by active invasion of T. gondii within minutes. T. gondii-infected DCs exhibited up-regulation of the C-C chemokine receptor CCR7 and chemotaxis towards the CCR7 chemotactic cue, CCL19. In paper II, we developed a 3-dimensional migration assay in a collagen matrix, which allowed us to characterize the hypermigratory phenotype in a more in vivo-like environment. The migration of T. gondii-infected DCs exhibited features consistent with integrin-independent amoeboid type of migration. T. gondii-induced hypermigration of DCs was further potentiated in the presence of CCL19 in a 3D migration assay. In paper III, we identified a parasite effector molecule, a Tg14-3-3 protein derived from parasite secretory organelles. Tg14-3-3 was sufficient to induce the hypermigratory phenotype. Transfection with Tg14-3-3-containing fractions or recombinant Tg14-3-3 protein induced the hypermigratory phenotype in primary DCs and in a microglial cell line. In addition, Tg14-3-3 localized in the parasitophorous vacuolar space and host 14-3-3 proteins were rapidly recruited around the parasitophorous vacuole. In paper IV, we found that mouse DCs dominantly express the L-type voltage-dependent calcium channel, Cav1.3. Cav1.3 was linked to the GABAergic signaling-induced hypermigratory phenotype. Pharmacological inhibition of Cav1.3 and knockdown of Cav1.3 abolished the hypermigratory phenotype in T. gondii infected DCs. Blockade of voltage-dependent calcium channels reduced the dissemination of T. gondii in a mouse model. In paper V, we showed that microglia, resident immune cells in the brain, also exhibited rapid morphological changes and hypermotility upon infection with T. gondii. However, an alternative GABA synthesis pathway was shown to be involved in the hypermigratory phenotype in microglia. In summary, this thesis describes novel host-parasite interactions, including host cell migratory responses and key molecular mechanisms that mediate the hypermigratory phenotype. The findings define a novel motility-related signaling axis in DCs. Thus, T. gondii employs GABAergic non-canonical pathways to hijack host cell migration and facilitate dissemination. We believe that these findings represent a significant step forward towards a better understanding of the pathogenesis of T. gondii infection. / <p>At the time of the doctoral defense, the following papers were unpublished and had a status as follows: Paper 4: Manuscript. Paper 5: Manuscript.</p>

Apicomplexa

dendritic cells

microglia

cell migration

14-3-3 proteins

GABAergic signaling

voltage-dependent calcium channel

host-parasite interaction

Biological Sciences

Biologiska vetenskaper

Caractérisation des différents mouvements collectifs au cours de la migration des cellules de bordure chez la drosophile / Characterisation of different collective movements during Drosophila border cell migration

Combedazou, Anne

18 November 2016

La migration cellulaire concerne des cellules individuelles ou bien des groupes de cellules migrant de manière collective et coordonnée. De nombreux processus physiologiques, notamment au cours du développement embryonnaire, ainsi que pathologiques, notamment lors de maladies inflammatoires ou de la formation de métastases nécessitent des mouvements cellulaire collectifs. Au cours de l'ovogénèse chez la Drosophile, un groupe de cellules, appelés cellules de bordure, migrent entre les cellules nourricières, collectivement, au sein du follicule ovarien. Ces cellules de bordure constituent un modèle de choix pour étudier les mécanismes régulant la migration collective in vivo. La migration de ce groupe de cellules est divisée en deux phases. Lors de la première moitié de migration, du début de la migration à la moitié du parcours, les cellules de bordure adoptent un mouvement linéaire, au cours duquel chaque cellule maintient sa position au sein de l'entité, et une seule et même cellule conduit le groupe vers l'avant. Ensuite, à mi-chemin, ces groupes commencent à effectuer des mouvements de rotation sur eux-mêmes pour aller atteindre l'ovocyte, permettant à n'importe quelle cellule de pouvoir mener la migration. L'objectif de ma thèse a été d'élucider les mécanismes régulant le choix entre ces deux modes de migration (linéaire et rotationnel). Le cytosquelette d'acto-myosine est un des acteurs principaux régulant la contraction cellulaire nécessaire à la motilité des cellules. Au cours de ma thèse, nous avons mis en évidence le rôle de la myosine non musculaire de type II dans le contrôle du passage d'un mouvement linéaire à rotationnel. Nos travaux démontrent que l'apparition des mouvements de rotation effectués par les cohortes de cellules de bordure est corrélée à une augmentation de l'activité de la myosine non musculaire de type II. De plus, nous avons montré que l'activité de la myosine non musculaire de type II pouvait être régulée de manière antagoniste par les récepteurs de guidance. En conclusion, mes travaux de thèse nous ont permis de démontré le rôle clé de la myosine non musculaire de type II dans l'adaptation du mode de migration au cours de mouvements collectifs des cellules de bordure. De plus nous avons identifié les facteurs régulant l'activité de la myosine non musculaire de type II. En effet, cette dernière est régulée positivement par EGFR. / In many biological processes, cells can move individually or in a coordinated and collective manner. Collective migrations are necessary during several embryo developmental processes, and pathologies such as inflammatory diseases or metastasis formation. During Drosophila oogenesis, border cells, a group of 6-10 cells, migrate in between nurse cell until the oocyte, within the egg chamber and provide a good model to study collective cell migration in vivo. Border cell migration is divided in to two phases. From the anterior pole of the egg chamber to the half of migrated distance, border cell adopt a linear movement, in which each cell maintain its position within the cluster and one leader cell drive the migration. Midway of the migration path, border cell clusters rotate to reach the oocyte. During this second phase, any cell can take the lead of the migration. The aim of my PhD research works was to identify mechanisms regulating the choice between linear and rotational movements. Acto-myosin cytoskeleton is one of the main regulators of cell contraction necessary for cell motility. Through our research, we demonstrated that non-muscle myosin II (NMII) regulate the switch between linear and rotational behaviour. These results led us to identify mechanisms regulating NMII activity during border cell migration. Border cells express two guidance receptors: PVR (Platelet-derived growth factor receptor (PDGFR) and Vascular endothelial growth factor receptor (VEGFR) receptor Related) and EGFR (Epidermal Growth Factor Receptor). Recent studies shown that PVR play a crucial role in the first phase and EGFR predominantly regulate the second phase of migration. Our data shows that NMII is antagonistically regulated by PVR and EGFR. Indeed, the inhibition of NMII in border cell over expressing EGFR completely blocks the rotational movement To conclude, my PhD works allow us to demonstrate the key role of NMII for the regulation of border cell migration. Moreover, we found that EGFR positively regulates NMII activity.

Migration cellulaire collective

Myosine

ROCK

Récepteurs de guidance

Drosophila melanogaster

Cellules de bordure

Collective cell migration

Myosin

ROCK

Guidance receptors

Drosophila melanogaster

Border cells

The Role of LMO4 in the Regulation of SLK Localization & Activation within Migrating Cells and in Murine Mammary Tumorigenesis

Baron, Kyla Doreen

January 2016

The Ste20-like kinase SLK plays a pivotal role in cell migration and focal adhesion turnover. SLK activity is regulated by the LIM domain-binding proteins Ldb1/2. In addition to playing role in tumor initiation and progression, these proteins have been demonstrated to interact with LMO4. Therefore, this project assessed the ability of LMO4 to interact and regulate SLK activity. Results show that LMO4 can directly bind to SLK and activate its kinase activity. LMO4 can be co-precipitated with SLK following the induction of cell migration by scratch wounding. Cre deletion of LMO4 inhibits cell migration and SLK activation, and impairs Ldb1 and SLK recruitment to the leading edge of migrating cells. Src/Yes/Fyn-deficient cells (SYF) express very low levels of LMO4 and do not recruit SLK to the leading edge. Src-family kinase inhibition impairs SLK recruitment to the leading edge, suggesting that both expression of LMO4 and the recruitment of SLK to the leading edge require c-Src activity. In conclusion, cell migration and activation of SLK requires its recruitment to the leading edge by LMO4 in a Src-dependent manner. This study also investigated whether LMO4 deletion through MMTV-Cre-driven excision would impair mammary tumorigenesis in a PyMT mouse model of breast cancer. No difference in Overall Survival was observed between animals with and without LMO4 expression. Western blot analysis and IHC showed that tumors expressed LMO4 protein in animals genotyped as Cre-positive. This result suggests that expression of LMO4 is required for tumor initiation in the PyMT model of murine mammary carcinoma. This project has established a novel cytosolic role for the transcriptional co-activator LMO4 and validated it’s involvement in the regulation of SLK and cell migration. This pathway may provide a novel therapeutic strategy as LMO4 appears to be critical to the initiation and progression of breast cancer.

Ste20-Like Kinase

LIM-Only protein 4

LIM-domain binding protein 1/2

Src-Family Kinases

cell migration

cell signalling

mammary tumorigenesis

Dynamique de la fermeture des trous épithéliaux en utilisant des techniques de micromécanique et de microfabrication / Dynamics of epithelial gap closure using microfabrication and micromechanical approaches

Anon, Ester

05 October 2012

Les cellules peuvent migrer sous différentes conditions qui dépendent de l’environnement biochimique ou mécanique. Connaître les mécanismes de la migration, les protéines impliquées et leur régulation est essentiel pour comprendre les processus de morphogénèse ou certaines situations pathologiques. Dans ce contexte, la migration collective des cellules est un processus clé qui intervient pendant le développement ainsi que dans la vie adulte. Elle joue un rôle très important pour la formation et l’entretien des couches épithéliales, notamment au cours du développement embryonnaire et pendant la cicatrisation des trous épithéliaux résultant, par exemple, d’une blessure. Lorsque l’épithélium présente une discontinuité, des mécanismes actifs qui impliquent une migration coordonnée des cellules sont nécessaires pour préserver l’intégrité des tissus. Dans ce travail, nous avons étudié les mécanismes impliqués dans la fermeture des trous dans un épithélium. Pour des blessures de faible taille, le mode de fermeture dit de purse string est souvent évoqué, impliquant la contraction d’un anneau contractile d’acto-myosine qui ferme la blessure. Pour des blessures de tailles plus importantes, il est courant d’observer un mécanisme différent conduisant { la migration active des cellules du bord qui couvrent la surface “libre”.Pour étudier ces aspects de manière quantitative et reproductible, nous avons développé une nouvelle méthode basée sur des techniques de microfabrication et de lithographie dite « molle » qui permet de faire une étude quantitative de la fermeture des trous épithéliaux. Nous avons fabriqué des substrats de micropiliers de diamètre et de forme variés dans les quels les cellules sont libres de pousser entre les microstructures. Lorsqu’elles sont parvenues à confluence, on retire le substrat qui laisse apparaître des trous contrôlés.De cette manière, nous avons observé que les cellules épithéliales forment des lamellipodes pour la fermeture de ces trous. Le mécanisme de fermeture dépend de la taille des trous et nous avons pu observer différents régimes en fonction de diamètre des piliers. Les trous petits (de la taille d’une seule cellule) sont fermés par un mécanisme passif alors que la fermeture de trous plus larges nécessite un mécanisme actif de migration conduisant à la formation de lamellipodes et à des modes de migration collective. Par la suite, nous nous sommes intéressés à l’aspect mécanique de la fermeture des trous épithéliaux. Pour cela, nous avons utilisé un système d’ablation laser pour rompre quelques cellules dans une monocouche épithéliale. Nous avons alors mesuré les forces de traction que les cellules exercent au substrat et leur évolution temporelle et spatiale. Nous avons pu mettre en évidence différents modes de traction: au début, les cellules exercent des forces de traction importantes sur leur substrat pour laisser place à des contraintes mécaniques qui sont davantage issues d’un processus collectif au travers de la formation d’un câble multicellulaire qui les relie les cellules de bord entre elles. En conclusion, ce travail nous a permis d’obtenir des informations sur les mécanismes dynamiques de fermeture des tissus épithéliaux qui sont évidemment impliqués dans la cicatrisation des blessures mais aussi dans certains problèmes de malformations congénitales lors l’embryogenèse. / Most cells migrate under the appropriate conditions or stimuli; understanding the mechanisms of migration, the players involved, and their regulation, is pivotal to tackle the pathological situations where migration becomes an undesired effect. While largely overshadowed by the study of single cell migration, collective cell migration is a very relevant process that takes place during development as well as in adult life. Collective migration is very relevant for the formation and maintenance of epithelial layers: extensive migratory processes occur during the shape of the embryo, as well as during the healing of a skin incision in the adult. When openings or discontinuities appear in the epithelia, it is crucial that the appropriate mechanisms are activated.In the present work we attempt at deciphering what are the mechanisms involved in gap closure. Until now, most of the literature concerning the subject has reported contradictory results, mainly arising from the complexity of the process and the lack of systematic analysis. We have designed a novel approach to address epithelial gap closure under well-defined and controlled conditions. By using our gap patterning method, we have observed that epithelial cells extend lamellipodia when exposed to a newly available space. Interestingly, we found that the closure of such gap depends on the size: small gaps are closed by a passive physical mechanism, while large gaps are closed through a Rac-dependent cell crawling mechanism, in a collective migration-like manner. 11Abstract (English)Most cells migrate under the appropriate conditions or stimuli; understanding the mechanisms of migration, the players involved, and their regulation, is pivotal to tackle the pathological situations where migration becomes an undesired effect. While largely overshadowed by the study of single cell migration, collective cell migration is a very relevant process that takes place during development as well as in adult life. Collective migration is very relevant for the formation and maintenance of epithelial layers: extensive migratory processes occur during the shape of the embryo, as well as during the healing of a skin incision in the adult. When openings or discontinuities appear in the epithelia, it is crucial that the appropriate mechanisms are activated.In the present work we attempt at deciphering what are the mechanisms involved in gap closure. Until now, most of the literature concerning the subject has reported contradictory results, mainly arising from the complexity of the process and the lack of systematic analysis. We have designed a novel approach to address epithelial gap closure under well-defined and controlled conditions. By using our gap patterning method, we have observed that epithelial cells extend lamellipodia when exposed to a newly available space. Interestingly, we found that the closure of such gap depends on the size: small gaps are closed by a passive physical mechanism, while large gaps are closed through a Rac-dependent cell crawling mechanism, in a collective migration-like manner. Next, we also addressed the mechanical component of epithelial gap closure. In this study, we took advantage of a laser-ablation system to disrupt some cells within an epithelial monolayer, and study how the remaining cells sealed that gap. By measuring the traction forces that cells exert on the substrate along the closure, we observed that cells first pulled on the substrate to propel themselves. By the last steps of closure, there is a transition in the direction of the force, so that cells are pulled to the center of the gap due to the assembly of a supracellular actin cable. Altogether, this work provides valuable knowledge on the current understanding of the mechanisms accounting for epithelial gap closure. We believe that a better comprehension of these mechanisms can help to shed light in clinically relevant situations where epithelial gap closure is impaired.

Microfabrication

Cicatrisation

Migration cellulaire

Lamellipodia

Épithelium

Mécanique cellulaire

Sustrats mous

Microfabrication

Wound healing

Cell migration

Lamellipodia

Epithelia

Cell mechanics

Soft substrates

Mathematical models of transport phenomena in biological tissues

Grau Ribes, Alexis

13 March 2020

Cette thèse est consacrée à l’élaboration et l’étude théorique de modèles de transport décrivant les dynamiques cellulaires et la communication intercellulaire dans les tissus épithéliaux. Nous nous intéressons d’abord à l’influence du transport de microARNs (miRNAs) sur la dynamique spatiotemporelle de réseaux de régulation génétique. Ces courtes séquences d’ARN régulent la synthèse des protéines en bloquant l’activité des ARN messagers et leur sécrétion via des vesicules extracellulaires en font des agents de communication intercellulaire. Différents modèles faisant intervenir des miRNAs extracellulaires ont été construits et étudiés numériquement. Les premiers sont des modèles génériques destinés à mettre en évidence l'effet d'une cellule ayant une production de miRNAs anormale sur l'expression génétique dans les cellules voisines. Nous abordons ensuite des modèles plus complexes et réalistes dans lesquels des oscillations (liées à des rythmes biologiques) et de la bistabilité (liée à une différenciation cellulaire) sont observées. Ces modèles permettent d’étudier des dynamiques de communication complexes observées en biologie, comme la synchronisation de cellules couplées ou la propagation d'un changement de phénotype. Nous mettons également en évidence le rôle de défauts, tels que des mutations génétiques ou encore des variations de densité cellulaire dans les tissus, sur ces phénomènes de propagation. La deuxième partie de la thèse est dédiée à la construction de modèles de réaction-diffusion dans lesquels la dynamique des cellules dépend de leur état interne. Sur base d’études expérimentales montrant l’influence de protéines et de miRNAs sur la mobilité et la prolifération des cellules, nous établissons un modèle multi-échelle dans lequel la dynamique intracellulaire et le mouvement des cellules interagissent. En effet, certaines protéines sont responsables de l’adhésion cellulaire ou régulent la vitesse de prolifération. Dans notre modèle, chaque cellule synthétise ces espèces d’intérêt et les processus cellulaires (migration, prolifération) dépendent de la concentration de ces espèces biochimiques. Ce modèle permet de reproduire des expériences de migration cellulaire et de prédire, notamment, l'influence d'E-cadherin, une protéine clé dans l'adhesion cellulaire, sur la dynamique de régénération d'un tissu. / Doctorat en Sciences / info:eu-repo/semantics/nonPublished

Biologie théorique

Mathematical models

Modèles mathématiques

Transport phenomena

Phénomènes de transport

MicroRNA

MicroARN

Cell migration

Cell proliferation

Rôle des Arfs et de leurs régulateurs dans la migration des cellules de bordure chez la drosophile

Zeledon Orellana, José Carlos

03 1900

La migration cellulaire joue un rôle essentiel dans le développement des organismes multicellulaires et dans certaines pathologies comme le cancer, où elle permet la formation de métastases. Le trafic vésiculaire est un régulateur clé de la migration cellulaire, notamment en contrôlant la localisation de protéines impliquées dans la migration telles que les intégrines, les cadhérines et les récepteurs transmembranaires. En particulier, notre laboratoire a montré que l'endocytose contrôle l'orientation et la communication cellulaire durant la migration cellulaire collective. Notre hypothèse est que d'autres événements du trafic vésiculaire pourraient aussi être impliqués dans ce type de migration. Ainsi, le but de cette thèse a été de déterminer la fonction des petites GTPases Arf, importantes pour la formation de vésicules et le tri de cargo dans ces vésicules et de leurs régulateurs dans la migration cellulaire collective. Un modèle pour étudier la migration cellulaire collective est les chambres d’œufs de Drosophila melanogaster. En effet, lors de l’ovogénèse, des cellules folliculaires appelées cellules de bordure migrent à travers les cellules nourricières pour atteindre l’ovocyte. Conformément à notre hypothèse, un fort défaut de migration est observé lorsque les Arfs sont déplétées spécifiquement dans les cellules de bordure. De plus, un constat similaire est observé après la déplétion de certains régulateurs des Arfs (ArfGAPs et ArfGEFs). Notamment, nous avons démontré que l’ArfGAP Drongo et sa fonction d'activation de l’activité GTPase sont essentielles pour le détachement initial des cellules de bordure du tissu folliculaire. Drongo promeut le détachement en contrôlant la localisation de la myosine phosphatase afin de réguler l’activité de la myosine II à l’arrière des cellules. De plus, nous avons montré que Drongo agit sur l’Arf de classe III (Arf51F) de manière antagoniste à l’ArfGEF Steppke pour déplacer la myosine phosphatase de l’arrière du groupe de cellules. D’un autre côté, nous avons aussi démontré qu’une autre GAP, ArfGAP1, contrôle la directionnalité de migration. Cette ArfGAP agit potentiellement en régulant la localisation de certains déterminants de la migration tels que l’E-cadhérine et les récepteurs tyrosine kinase. Ainsi, nos recherches ont démontré un rôle essentiel des Arfs ainsi que des rôles spécifiques de deux ArfGAPs dans la migration cellulaire collective. / Cell migration is implicated in various important biological processes, notably it is central for the dissemination of cancer cells. Vesicular trafficking is a key regulator of cell migration, notably by controlling the localisation of proteins involved in migration such as integrins, cadherins and transmembrane receptors. In particular, our laboratory has shown that endocytosis controls orientation and cellular communication during collective cell migration. Our hypothesis is that other events of vesicular trafficking might be implicated in collective cell migration. Thus, the purpose of this thesis was to assess the function of small GTPases Arf, important for vesicle formation and cargo sorting into those vesicles, and their regulators in collective cell migration. A powerful model to study collective cell migration is the migration of follicular cells named border cells during oogenesis in Drosophila melanogaster. Border cells (BCs) detach from the follicle epithelium surrounding the egg chambers and form a small cluster of six to ten cells that migrates invasively between the giant nurse cells that compose the center of the egg chamber, toward the oocyte. Accordingly to our hypothesis, a strong migration defect is observed when the Arfs are depleted specifically in the border cells. Moreover, a similar finding is observed after depletion of some Arfs regulators (ArfGAPs and ArfGEFs). In particular, the ArfGAP Drongo and its GTPase-activating function are essential for the initial detachment of the border cell cluster from the basal lamina. We demonstrated through protein localization and genetic interactions that Drongo controls the localisation of the myosin phosphatase in order to regulate myosin II activity at the back of the cluster and promote border cells detachment. Moreover, we showed that Drongo acts on the class III Arf (Arf51F) antagonistically to the guanine exchange factor Steppke to displace myosin phosphatase from the back of the cluster. On the other hand, we have also demonstrated that the GAP ArfGAP1 controls the directionality of migration. This ArfGAP potentially acts by regulating the localization of certain determinants of migration such as E-cadherin and receptors tyrosine kinase. Thus, our research has demonstrated an essential role for Arfs in collective cell migration and specific contributions of two ArfGAPs in this migration process.

Migration cellulaire

Trafic vésiculaire

GTPases Arf

ArfGAPs

Drongo

ArfGAP1

Cellules de bordure

Drosophile

Cell migration

Vesicular trafficking

Arf GTPases

Border cells

Drosophila

Studium migrace mesenchymálních kmenových buněk na principu chemotaxe / Study of mesenchymal stem cell migration based on principles of chemotaxis

Pošustová, Veronika

January 2020

The purpose of this Master thesis is to verify migration of mesenchymal stem cells on the principle known as chemotaxis. First part of this study is focused on cell migration in order to explain the whole migration process. Next part describes various chemotaxis methods and selected studies dealing with clinical applications of mesenchymal stem cells in different medical and biomedical fields. The following step describes confocal microscopy, which is used for acquiring images of the cells. The experimental part is focused on cultivation of mesenchymal stem cells in a laboratory, which is necessary for cell vitality. Furthermore, there are designed two main experiments. Firstly there is a 2D experiment with adherent cells for chemotaxis using -Slide Chemotaxis. Secondly Transwell migration test is designed and executed. Finally, the acquired images from confocal microscope are used for image processing, which was done in Matlab R2020a programming environment. The result of this processing is evaluation of cell confluence and migration. In the end, experimental part of this study was optimized according to recommended studies. The results are summarized in the conclusion with proposal for improvements of those methods.

Cellular adhesion gene SELP is associated with rheumatoid arthritis and displays differential allelic expression

Burkhardt, Jana, Blume, Mechthild, Petit-Teixeira, Elisabeth, Teixeira, Vitor Hugo, Steiner, Anke, Quente, Elfi, Wolfram, Grit, Scholz, Markus, Pierlot, Céline, Migliorini, Paola, Bombardieri, Stefano, Balsa, Alejandro, Westhovens, René, Barrera, Pilar, Radstake, Timothy R. D. J., Alves, Helena, Bardin, Thomas, Prum, Bernard, Emmrich, Frank, Cornelis, Francois, Ahnert, Peter, Kirsten, Holger

January 2014

In rheumatoid arthritis (RA), a key event is infiltration of inflammatory immune cells into the synovial lining, possibly aggravated by dysregulation of cellular adhesion molecules. Therefore, single nucleotide polymorphisms of 14 genes involved in cellular adhesion processes (CAST, ITGA4, ITGB1, ITGB2, PECAM1, PTEN, PTPN11, PTPRC, PXN, SELE, SELP, SRC, TYK2, and VCAM1) were analyzed for association with RA. Association analysis was performed consecutively in three European RA family sample groups (Nfamilies = 407). Additionally, we investigated differential allelic expression, a possible functional consequence of genetic variants. SELP (selectin P, CD62P) SNP-allele rs6136-T was associated with risk for RA in two RA family sample groups as well as in global analysis of all three groups (ptotal = 0.003). This allele was also expressed preferentially (p,1026) with a two- fold average increase in regulated samples. Differential expression is supported by data from Genevar MuTHER (p1 = 0.004; p2 = 0.0177). Evidence for influence of rs6136 on transcription factor binding was also found in silico and in public datasets reporting in vitro data. In summary, we found SELP rs6136-T to be associated with RA and with increased expression of SELP mRNA. SELP is located on the surface of endothelial cells and crucial for recruitment, adhesion, and migration of inflammatory cells into the joint. Genetically determined increased SELP expression levels might thus be a novel additional risk factor for RA.

info:eu-repo/classification/ddc/610

ddc:610

New Insights into the Cell Biology of Hematopoietic Progenitors by Studying Prominin-1 (CD133)

Bauer, Nicola, Fonseca, Ana-Violeta, Florek, Mareike, Freund, Daniel, Jászai, József, Bornhäuser, Martin, Fargeas, Christine A., Corbeil, Denis

January 2008

Prominin-1 (alias CD133) has received considerable interest because of its expression by several stem and progenitor cells originating from various sources, including the neural and hematopoietic systems. As a cell surface marker, prominin-1 is now used for somatic stem cell isolation. Its expression in cancer stem cells has broadened its clinical value, as it might be useful to outline new prospects for more effective cancer therapies by targeting tumor-initiating cells. Cell biological studies of this molecule have demonstrated that it is specifically concentrated in various membrane structures that protrude from the planar areas of the plasmalemma. Prominin-1 binds to the plasma membrane cholesterol and is associated with a particular membrane microdomain in a cholesterol-dependent manner. Although its physiological function is not yet determined, it is becoming clear that this cell surface protein, as a unique marker of both plasma membrane protrusions and membrane microdomains, might reveal new aspects of the cell biology of rare stem and cancer stem cells. The aim of this review is to outline the recent discoveries regarding the dynamic reorganization of the plasma membrane of rare CD133+ hematopoietic progenitor cells during cell migration and division. / Dieser Beitrag ist mit Zustimmung des Rechteinhabers aufgrund einer (DFG-geförderten) Allianz- bzw. Nationallizenz frei zugänglich.

info:eu-repo/classification/ddc/610

ddc:610