Global ETD Search

151	Role of Inner Arm Dyneins and Hydin in Ciliary Motility in Tetrahymena thermophila KABI, AMRITA 23 April 2010 (has links) No description available. Cellular Biology cilia axoneme dynein hydin hydrocephalus Tetrahymena thermophila LC-MS/MS
152	Genetic Modifiers of <i>CEP290</i>-Dependent Retinal Pathology Lessieur Contreras, Emma Mercedes 01 June 2018 (has links) No description available. Genetics Health Sciences Medicine Ophthalmology Molecular Biology photoreceptor cilia ciliopathies zebrafish CEP290
153	Mechanosensory Role of Vascular Endothelial Primary Cilia in the Development of Hypertension in Polycystic Kidney Disease Hossain Saad, Md Zubayer January 2016 (has links) No description available. Pharmacology Cellular Biology Molecular Biology
154	Investigations into Neuronal Cilia Utilizing Mouse Models of Bardet-Biedl Syndrome Berbari, Nicolas F. 18 March 2008 (has links) No description available. Biomedical Research Cellular Biology Genetics Molecular Biology cilia Bardet-Biedl Syndrome
155	The evolution of eukaryotic cilia Hodges, Matthew Edmiston January 2011 (has links) Eukaryotic cilia are complex, highly conserved microtubule-based organelles with a broad phylogenetic distribution. Cilia were present in the last eukaryotic common ancestor and many proteins involved in cilia function have been conserved through eukaryotic diversification. The evolution of these ciliary functions may be inferred from the distribution of the molecular components from which these organelles are composed. By linking protein distribution in 45 diverse eukaryotes with organismal biology, I define an ancestral ciliary inventory. Analysis of these core proteins allows the inference that the cenancestor of the eukaryotes possessed a cilium for motility and sensory function. I show that the centriolar basal body function is ancestral, whereas the centrosome is specific to the Holozoa, and I use this information to predict a number of roles for proteins based on their phylogenetic profile. I also show that while remarkably conserved, significant divergence in ciliary protein composition has occurred in many lineages, such as the unusual centriole of Caenorhabditis elegans and the transitional changes throughout the land plants. I exemplify this divergence through ultrastructural studies of the fern Ceratopteris richardii and the liverwort Marchantia polymorpha both of which have cilia that exhibit a number of distinctive morphological features, the most conspicuous of which is a general breakdown of canonical microtubule arrangements. Cilia have also been lost multiple times in different lineages: at least twice within the land plants. During these evolutionary transitions proteins with ancestral ciliary functions may be lost or co-opted into different functions. I have interrogated genomic data to identify proteins that I predict had an ancestral ciliary role, but which have been maintained in non-ciliated land plants. I demonstrate that several of these proteins have a flagellar localisation in protozoan trypanosomes and I use expression data correlation to predict potential non-ciliary plant roles. 571.65
156	Études fonctionnelles de deux nouvelles protéines centrosomales, NPHP5 et Cep76, et leurs implications dans les maladies humaines Barbelanne, Marine 08 1900 (has links) Les centrosomes sont de petits organites qui régulent divers processus cellulaires comme la polarité ou la mitose dans les cellules de mammifères. Ils sont composés de deux centrioles entourés par une matrice péricentriolaire. Ces centrosomes sont les principaux centres organisateurs de microtubules. De plus, ils favorisent la formation de cils, des protubérances sur la surface des cellules quiescentes qui sont critiques pour la transduction du signal. Une grande variété de maladies humaines telles que les cancers ou les ciliopathies sont liées à un mauvais fonctionnement des centrosomes et des cils. C’est pourquoi le but de mes projets de recherche est de comprendre les mécanismes nécessaires à la biogénèse et au fonctionnement des centrosomes et des cils. Tout d'abord, j’ai caractérisé une nouvelle protéine centrosomale nommée nephrocystine - 5 (NPHP5). Cette protéine est localisée dans les cellules en interphase au niveau de la région distale des centrioles. Sa déplétion inhibe la migration des centrosomes à la surface cellulaire lors de l’étape précoce de la formation des cils. NPHP5 interagit avec la protéine CEP290 via sa région C-terminale qui est essentielle pour la ciliogenèse. Elle interagit également avec la calmoduline ce qui empêche son auto-agrégation. J’ai démontré que les domaines de liaison de NHPH5 à CEP290 et à la calmoduline, ainsi que son domaine de localisation centrosomale sont séparables. De plus, j’ai démontré que les protéines NPHP5 présentant des mutations pathogènes ne peuvent plus interagir avec CEP290 et ne sont plus localisées aux centrosomes, rendant ainsi ces protéines non fonctionnelles. Enfin, en utilisant une approche pharmacologique pour moduler les événements en aval dans la voie ciliogénique, j’ai montré que la formation des cils peut être restaurée même en absence de NPHP5. D’autre part, j’ai étudié le rôle de NPHP5 dans l'assemblage et le trafic du complexe BBSome dans le cil. Le BBSome est composé de huit sous-unités différentes qui s’assemblent en un complexe fonctionnel dont on sait peu de chose sur la régulation spatiotemporelle de son processus d'assemblage. J’ai précédemment montré que NPHP5 favorisait la formation des cils et que son dysfonctionnement contribuait au développement de néphronophtise (NPHP). Bien que la NPHP et le syndrome de Bardet-Biedl (BBS) soient des ciliopathies qui partagent des caractéristiques cliniques communes, la base moléculaire de ces ressemblances phénotypiques n’est pas comprise. J’ai constaté que NPHP5, localisé à la base du cil, contient deux sites de liaison distincts pour le BBSome. De plus, j’ai démontré que NPHP5 et son partenaire CEP290 interagissent de façon dynamique avec le BBSome pendant la transition de la prolifération à la quiescence. La déplétion de NPHP5 ou CEP290 conduit à la dissociation d’au moins deux sous-unités du BBSome formant alors un sous-complexe dont la capacité de migration dans le cil n’est pas compromise. J’ai montré que le transport des cargos vers le compartiment ciliaire par ce sous-complexe n’est que partiellement altéré. Enfin, j’ai également concentré mes recherches sur une autre protéine centrosomale peu caractérisée. La protéine centrosomale de 76 kDa (Cep76) a été précédemment impliquée dans le maintien d’une duplication unique des centrioles par cycle cellulaire, et dans une interaction avec la kinase cycline-dépendante 2 (CDK2). Cep76 est préférentiellement phosphorylée par le complexe cycline A/CDK2 sur le site unique S83. Cet événement est essentiel pour supprimer l'amplification des centrioles en phase S. J’ai démontré que Cep76 inhibe cette amplification en bloquant la phosphorylation de Plk1 au niveau des centrosomes. D’autre part, Cep76 peut être acétylée au site K279 en phase G2, ce qui régule négativement son activité et sa phosphorylation sur le site S83. Ces études permettent d'améliorer notre compréhension de la biologie des centrosomes et des cils et pourraient conduire au développement de nouvelles applications diagnostiques et thérapeutiques. / Centrosomes are small organelles that regulate diverse cellular processes such as polarity or mitosis in mammalian cells. They are composed of two centrioles surrounded by a pericentriolar matrix. These centrosomes are the major microtubule organizing centers. Moreover, they promote the formation of cilia, protrusions on the surface of quiescent cells that are critical for signal transduction. A wide variety of human diseases such as cancers or ciliopathies are linked to a malfunction of centrosomes and cilia. Therefore the aim of my research is to understand the mechanisms necessary for the biogenesis and function of centrosomes and cilia. First, I have characterized a novel centrosomal protein called nephrocystin - 5 (NPHP5). This protein is localized, in interphase cells, in the distal region of centrioles. Its depletion inhibits the migration of centrosomes to the cell surface during the early stage of cilia formation. NPHP5 interacts with CEP290 via its C-terminal region that is essential for ciliogenesis. It also interacts with calmodulin, which prevents its self-aggregation. I have demonstrated that the Cep290- and CaM-binding domains as well as the centrosomal localization domain of NPHP5 are separable. Moreover, I have shown that NPHP5 proteins with pathogenic mutations can no longer interact with CEP290 and are not localized to centrosomes, rendering these proteins non-functional. Finally, using a pharmacological approach to modulate the downstream events in the ciliogenic pathway, I showed that cilia formation can be restored even without NPHP5. On the other hand, I studied the role of NPHP5 in the assembly and trafficking of the BBSome into the cilium. The BBSome consists of eight different subunits that assemble into a functional complex of which little is known about the spatiotemporal regulation of its assembly process. I have previously shown that NPHP5 favored the formation of cilia and its dysfunction contributes to the development of nephronophthisis (NPHP). Although the NPHP and BBS syndrome (BBS) are ciliopathies that share common clinical features, molecular basis of these phenotypic similarities is not understood. I found that NPHP5, located at the base of the cilium, contains two separate binding sites for BBSome. Furthermore, I demonstrated that NPHP5 and his partner CEP290 interact dynamically with the BBSome during the transition from quiescence to proliferation. Depletion NPHP5 or CEP290 leads to the dissociation of at least two subunits of BBSome forming a sub-complex that can still traffic into the cilium. I have shown that the transport of cargo to the ciliary compartment through this sub-complex is only partially altered. Finally, I have also focused my research on another centrosomal protein poorly characterized. The centrosomal protein of 76 kDa (Cep76) was previously involved in the maintenance of a single duplication of centrioles per cell cycle, and interacts with the cyclindependent kinase 2 (CDK2). Cep76 is preferentially phosphorylated by cyclin A/CDK2 on the single site S83. This event is essential to suppress centrioles amplification in S phase. I have demonstrated that Cep76 inhibits amplification by blocking the phosphorylation of Plk1 at the centrosome. Moreover, Cep76 can be acetylated at the K279 site in G2 phase, which negatively regulates its activity and phosphorylation on the site S83. These studies will improve our understanding of the biology of centrosomes and cilia and could lead to development of new diagnostic and therapeutic applications. Cil NPHP5 Cep76 cycle cellulaire Cep290 BBSome Cell cycle Cilia Centrosome
157	The Role of KRAS in Mechanosensing in Non-Small Cell Lung Cancer Powell, Krista M 01 January 2019 (has links) Lung cancer is the number one cause of cancer related death worldwide, with more than 1.6 million fatalities each year. Non-small cell lung cancer (NSCLC) accounts for 80-85% of all lung cancers, with KRAS being one of the most prevalent oncogenic driver mutations. Therapeutic approaches for KRAS-mutated NSCLC have been extensively explored due to the US National Cancer Institute RAS Initiative, but methods of directly targeting KRAS or downstream effectors, such as MEK, still have poor results. Previous reports have shown that KRAS-mutated NSCLC activate distinct receptor tyrosine kinases (RTKs) depending on the epithelial or mesenchymal state. Epithelial-to-mesenchymal transition (EMT) is known to play a role in the metastasis and poor prognosis of cancer, and is induced by extracellular matrix (ECM) stiffness. Hallmarks of EMT include loss of E-Cadherin and increase in Vimentin. This research investigates the role of KRAS in EMT transition due to increased ECM stiffness in KRAS mutant NSCLC, and how this affects the efficacy of KRAS and MEK inhibition. To understand how KRAS mutations in NSCLC play a role in this stiffness induced EMT, experiments were performed to detect the gene and protein expression of EMT markers, as well as possible sources of mechanosensing, including primary cilia and receptor tyrosine kinases. We hypothesized that KRAS plays a role in activation of mechanosensors and directly correlates to EMT induced by increased mechanical forces. Results show when KRAS was inhibited and there was increased mechanical forces, either from stretch or substrate stiffness, there was a decreased activation of mechanosensors. KRAS inhibition also prevented the cells from undergoing stiffness-induced EMT. This supports our hypothesis that KRAS plays a key role in ECM stiffness induced EMT. Future studies include examining the mechanism behind this phenomenon and in vivo studies. KRAS Non-Small Cell Lung Cancer Extracellular Matrix Stiffness Primary Cilia Receptor Tyrosine Kinase Mechano-receptors Biomechanics and Biotransport Cancer Biology
158	Spag17 Deficiency Impairs Neuronal Cell Differentiation in Developing Brain Choi, Olivia J 01 January 2019 (has links) The development of the nervous system is a multi-level, time-sensitive process that relies heavily on cell differentiation. However, the molecular mechanisms that control brain development remain poorly understood. We generated a knockout (KO) mouse for the cilia associated gene Spag17. These animals develop hydrocephalus and enlarged ventricles consistent with the role of Spag17 in the motility of ependymal cilia. However, other phenotypes that cannot be explained by this role were also present. Recently, a mutation in Spag17 has been associated with brain malformations and severe intellectual disability in humans. Therefore, we hypothesized that Spag17 plays a crucial role in nervous system development. To investigate this possibility, we first characterized the spatiotemporal expression of Spag17 in the developing brain by using Beta-galactosidase staining and immunohistochemistry. Results showed Spag17 expression in the spinal cord in embryonic E11. By E11.5-12.5 the expression extends to the rhombic lip from the developing hindbrain, as well as to the forebrain and midbrain regions. E14.5-15.5 embryos exhibit an intense expression in the developing ventricles as well as the cerebellum. From E17.5 to birth (P0), the gene is more broadly expressed. We then used a global Spag17 KO mouse model to characterize the function of Spag17 during brain development. Immunohistochemical studies performed in brain sections from E15.5 and P0 time points showed increased expression of the neural progenitor marker Nestin, and reduced expression of mature neuron marker NeuN, increasing positive trend with the young neuron marker Tuj1. Altogether, these findings reveal that Spag17 has a unique spatiotemporal distribution and may be critical for the maturation of neural progenitor cells. Cellular Differentiation Neural Stem Cells Neurons Neural Development Cilia Developmental Biology Embryonic Structures Molecular and Cellular Neuroscience Nervous System
159	Transport of lipid vesicles via the cilia logistic network in the brain of mice Günther, Ann-Kathrin 21 September 2018 (has links) No description available. 530 Physik (PPN621336750) ventral thrid ventricle cilia-generated flow liposomes extracellular vesicles ciliary logistic network CSF transport
160	Nitric Oxide in Primary Ciliary Dyskinesia : Missing in action? Inganni, Johan January 2008 (has links) No description available. Nitric oxide Primary ciliary dyskinesia cilia dynein axoneme Kartagener's situs inversus cilium iNOS inducible nitric oxide synthase Molecular biology Molekylärbiologi

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