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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
1

ANDROGENS SUPPRESS OSTEOCLAST FORMATION INDUCED BY RANK LIGAND AND M-CSF

Huber, Dustin Michael 11 October 2001 (has links)
No description available.
2

Mecanismos moleculares que regulan la activación clásica y alternativa en los macrófagos

Arpa Toribio, Luis 25 April 2008 (has links)
Los macrófagos son células fagocíticas pertenecientes al sistema inmunitario que participan tanto en la respuesta innata como en la adaptativa. En presencia de M-CSF, su estímulo mitogénico específico, proliferan, mientras que el tratamiento con estímulos activadores como el IFN-γ o el LPS hace que detengan su proliferación, se activen y pasen así a ejercer sus funciones específicas. En este contexto, existen dos tipos de citocinas con capacidad de activar al macrófago, las llamadas citocinas de tipo Th1 y las de tipo Th2. Las citocinas de tipo Th1 como el IFN-γ inducen en los macrófagos un patrón de activación llamado "clásico" cuya finalidad es provocar una respuesta de tipo proinflamatoria que acabará por eliminar la presencia de agentes patógenos. Por el contrario, las citocinas de tipo Th2 como la IL-4 inducen una activación "alternativa" en los macrófagos, cuya finalidad es la de llevar a cabo la reparación y remodelación tisular tras la respuesta proinflamatoria. En este estudio hemos observado, por primera vez, que la activación alternativa del macrófago cumple también la dicotomía proliferación/activación observada bajo estímulos clásicos e inhibe la proliferación del macrófago en el umbral entre las fases G1 y S del ciclo celular. En este sentido, hemos visto que tanto el IFN-γ como la IL-4 inducen un alargamiento en el tiempo de la cinética de activación de la MAPK ERK-1/2, encargada de regular la proliferación del macrófago en respuesta al M-CSF. Esta MAPK es regulada por la fosfatasa MKP-,1 quien se encarga de defosforilarla. Así, en presencia del M-CSF, MKP-1 se induce para regular a ERK-1/2 mientras que el IFN-γ y la IL-4 bloquean su expresión de forma dependiente de STAT. La inhibición directa de MKP-1 mediante tecnología de RNA de interferencia induce también un alargamiento de la actividad de ERK-1/2 y, en consecuencia, una parada de la proliferación, corroborando así los resultados obtenidos previamente. También hemos analizado el estado de activación de los complejos cdk2/cicE, encargados de la progresión del ciclo celular entre las fases G1 y S. Hemos visto que, mientras que el M-CSF induce la expresión de la ciclina E y, en consecuencia, la activación del complejo cdk2/cicE, tanto el IFN-γ como la IL-4 inhiben a ambos, explicando así el mecanismo utilizado por estas citocinas para mantener la parada en G1. Este bloqueo de la actividad cdk2/cicE es llevado a cabo gracias a la acción del inhibidor de cdk p21Waf1. Sin embargo, aunque ambas citocinas inducen la expresión de esta proteína, utilizando células knockout para p21Waf1 hemos demostrado que sólo la parada inducida por la IL-4 es dependiente de esta proteína, lo cual sugiere que el IFN-γ y la IL-4 utilizan vías de señalización distintas para ejercer funciones celulares similares. Por otro lado, hemos analizado también la implicación de la vía de las MAPK en la activación alternativa del macrófago. En este aspecto hemos demostrado que, aunque la expresión de los principales genes responsables de dicha activación es dependiente de STAT6, la acción de JNK1 ejerce un efecto sinérgico sobre su inducción, ya que la inhibición de esta quinasa resulta en una disminución de la expresión de dichos genes. El mecanismo mediante el cual JNK1 ejerce esta función no está aún del todo claro. Sin embargo, los resultados obtenidos mediante ensayos de inmunoprecipitacion de cromatina sugieren que JNK1 podría estar fosforilando a determinados cofactores en las zonas promotoras de algunos genes, colaborando así con la actividad del factor de transcripción STAT6. / Macrophages play a crucial role as regulators of immune response. They are originated from bone marrow stem cells and, in response of growth factors and particularly to macrophage colony-stimulating factor (M-CSF), they proliferate and differentiate. We have previously observed that activation of extracellularly regulated kinase (ERK) 1/2 is required for macrophage proliferation in response to growth factors. A short and early pattern of ERK activity correlated with the proliferative response. In contrast, slightly prolonged patterns of activity of these kinases were induced by signals that lead to macrophage activation and growth arrest. IFN-γ is the main endogenous Th1 type macrophage activator and IL-4 is the main Th2 type one. While M-CSF withdrawal arrested the cell cycle at early G1, treatment of macrophages with IFN-γ or IL-4 stopped the cell cycle later, at the G1/S boundary. IFN-γ and IL-4 induced the expression of the Cdk inhibitor p21Waf1. Using knockout mice and siRNA experiments, we found that p21Waf1 is required for IL-4- but not for IFN-γ-dependent inhibition of proliferation. Moreover, both IFN-γ and IL-4 elongate the activity pattern of the MAPK ERK-1/2 through the inhibition of the phosphatase MKP-1, which in fact results in a decrease of proliferation. Moreover, inhibition of MKP-1 expression using siRNA technology or synthetic inhibitors also led to elongated ERK activity and significant blockage of M-CSF-dependent proliferation. On the other hand, we have also analyzed the relationship between IL-4 and the MAPK pathway on the context of the alternative activation of macrophages. The IL-4 signaling pathway involves activation of STAT-6. However, IL-4 has also the capability to activate members of the MAPK family. In primary bone marrow-derived macrophages, we have observed strong activation of JNK-1 at early time points of IL-4 stimulation, whereas weak activation of ERK-1/2 and p38 were detected at a more delayed stage. By using selective inhibitors and knockout models, we have explored the contributions of MAPK activation to the macrophage response to IL-4. Our findings indicate that JNK-1 regulate IL-4-mediated expression of genes typically involved in alternative activation such as arginase 1.
3

Endovascular trophoblast cell behavior in normal and abnormal pregnancy

Endo, Yasuhiro 06 June 2008 (has links)
Preeclampsia is an important disease during pregnancy and causes significant maternal and fetal mortality and morbidity. Despite intense research efforts, the etiology and pathogenesis of the disease remain largely unknown. Since placentas from preeclamptic patients are smaller than normal, and cytokine growth factors are suggested to be important in placental growth, the effects of macrophage-colony stimulating factor (M-CSF) on human trophoblast cells were examined. While term trophoblast cells did not respond to M-CSF, those from early trimester and choriocarcinoma cells showed enhanced growth after treatment. In addition, the serum level of M-CSF in hypertensive pregnant women at the second trimester were significantly lower than those of normal pregnant women. These data suggest possible roles of M-CSF in preeclampsia. When M-CSF was administered to pregnant rats on days 8-11, rats had smaller placentas at day 12 and increased fetal resorption rate at day 20. The effects of interleukin-12 (IL-12) was also examined on days 8-11. While placental development was normal at both days 12 and 20, fetuses were significantly smaller at day 20. To remedy the difficulties and dangers associated with obtaining human placentas, I characterized endovascular trophoblast cell behavior in pregnant rats. In normal pregnancy, rat trophoblast cells simulated all features of human endovascular trophoblast behavior including selective invasion into the spiral arteries, retrograde migration, embedding, and secretion of PAS-positive materials as well as IIphysiological changes," In pregnancy terminated with a certain type of spontaneous fetal resorption, defective endovascular trophoblast cell behavior was observed, which was similar to that reported in preeclamptic pregnancy. Finally, the roles of cytoskeleton on trophoblast cell locomotion were investigated in vivo with a cytoskeleton-disrupting agent, cytochalasin B. This treatment impaired trophoblast cell invasion at day 12 and induced smaller fetuses at day 20, suggesting the importance of cytoskeleton in trophoblast movement. In conclusion, the results suggest the importance of the use of appropriate specimens and endpoints in the study of pregnancy, and rats may serve as a suitable animal model for the study of endovascular trophoblast cell behavior with clinical relevance to preeclampsia. / Ph. D.
4

Impact de l’acide lactique sur le phénotype et le métabolisme des macrophages humains / Impact of lactic acidosis on the phenotype of human macrophages

Paolini, Léa 13 December 2018 (has links)
Les macrophages associés aux tumeurs (TAM) orchestrent l'inflammation nécessaire à la croissance tumorale (propriétés de type M1) et favorisent les métastases et l'angiogenèse (caractéristiques de type M2). Cependant, la nature des facteurs capables de conférer des propriétés M1 et M2 aux macrophages humains demeure inconnue. L'acide lactique (AL) est un métabolite produit par les cellules tumorales connu pour moduler les fonctions des cellules présentes dans le microenvironnement tumoral. Dans cette étude, nous avons analysé son impact sur la différenciation des monocytes humains. Les résultats montrent que l’AL induit la différentiation des monocytes (cultivées en présence de GM-CSF) en macrophages présentant un phénotype atypique (CD14high CD163high IL-10low IL-12low) et, de manière intéressante, des caractéristiques phénotypiques M1 (production de cytokines inflammatoires) et M2 (production de facteurs de croissance, expression de gènes prototypiques M2). Un profil similaire est obtenu lorsque les monocytes sont cultivés avec des cellules cancéreuses primaires glycolytiques. Ces effets de l'AL sur la polarisation des macrophages nécessitent l'entrée du lactate dans les cellules (via le transporteur MCT-1) et son oxydation en pyruvate et sont médiés par une stabilisation de HIF-1α et une consommation autocrine de M-CSF.Ces résultats (i) identifient l'AL comme un médiateur induisant la génération de macrophages humains présentant des caractéristiques M2 et des propriétés inflammatoires et (ii) renforcent l'intérêt de l’utilisation des inhibiteurs de la glycolyse aérobie pour moduler les fonctions des TAM. / In established tumors, tumor-associated macrophages (TAM) orchestrate unresolving cancer-related inflammation (M1-related properties) and favor tumor development, metastasis and angiogenesis (M2-like properties). However, to date, the nature of the polarization factor(s) able to confer M1 and M2 functional properties to human macrophages remains unknown.Lactic acid (LA), a metabolite produced at high levels in most established tumors, can impact the phenotype and functions of cells present in the tumor microenvironment. In this study, we analyzed the impact of LA on the human monocyte differentiation. Results showed that LA skews monocytes (differentiated in the presence of GM-CSF) into macrophages (GM+LA-Mφ) exhibiting an atypical CD14high CD163high IL-10low IL-12low phenotype. Interestingly they harbor M1 and M2 phenotypic features, as assessed the production of a wide variety of inflammatory and growth factors and the expression of prototypic M2-like genes. A similar profile is induced by culturing monocytes with glycolytic human primary cancer cells. These effects of LA on macrophage polarization require the entry of lactate into the cells (via the monocarboxylate transporter 1) and its oxidation into pyruvate and are mediated via HIF-1α stabilization and autocrine M-CSF consumption by differentiating cells. These results identify tumor-derived LA as a missing link reconciling the M2-like features of TAM with their inflammatory properties. They also reinforce the interest of aerobic glycolysis inhibitors to modulate the functions of TAM.
5

Mutational analysis of the proto-oncogenes c-fms and c-kit

Baker, David Alan January 1995 (has links)
No description available.
6

The Role of Colony-stimulating Factor 1 and its Receptor on Acute Myeloid Leukemia

Fateen, Mohammed 25 July 2012 (has links)
Colony-stimulating factor 1 receptor (CSF1R, Fms) is an integral transmembrane glycoprotein with tyrosine specific protein kinase activity that it is found on the mononuclear phagocytes to promote their survival, proliferation and differentiation. Colony-stimulating factor 1 (CSF-1), also known as M-CSF, is a protein ligand that acts on the CSF1R. There is a variable association of Fms with the stem cell marker CD34 on acute myeloid leukemia (AML) cells and this suggests different structures of the AML hierarchy in different patients. Mouse stromal cells (MS-5) were transduced with a plasmid containing human CSF-1 because mouse CSF-1 is inactive on human CSF1R. Results show that AML cells cultured with CSF-1-expressing stroma had a much better growth and survival than the control stroma, suggesting that CSF-1 might be a stimulating factor for the growth of leukemic stem cells.
7

The Role of Colony-stimulating Factor 1 and its Receptor on Acute Myeloid Leukemia

Fateen, Mohammed 25 July 2012 (has links)
Colony-stimulating factor 1 receptor (CSF1R, Fms) is an integral transmembrane glycoprotein with tyrosine specific protein kinase activity that it is found on the mononuclear phagocytes to promote their survival, proliferation and differentiation. Colony-stimulating factor 1 (CSF-1), also known as M-CSF, is a protein ligand that acts on the CSF1R. There is a variable association of Fms with the stem cell marker CD34 on acute myeloid leukemia (AML) cells and this suggests different structures of the AML hierarchy in different patients. Mouse stromal cells (MS-5) were transduced with a plasmid containing human CSF-1 because mouse CSF-1 is inactive on human CSF1R. Results show that AML cells cultured with CSF-1-expressing stroma had a much better growth and survival than the control stroma, suggesting that CSF-1 might be a stimulating factor for the growth of leukemic stem cells.
8

Osteoclasts and Microgravity

Smith, John Kelly 01 September 2020 (has links)
Astronauts are at risk of losing 1.0% to 1.5% of their bone mass for every month they spend in space despite their adherence to diets and exercise regimens designed to protect their musculoskeletal systems. This loss is the result of microgravity-related impairment of osteocyte and osteoblast function and the consequent upregulation of osteoclast-mediated bone resorption. This review describes the ontogeny of osteoclast hematopoietic stem cells and the contributions macrophage colony stimulating factor, receptor activator of the nuclear factor-kappa B ligand, and the calcineurin pathways make in osteoclast differentiation and provides details of bone formation, the osteoclast cytoskeleton, the immune regulation of osteoclasts, and osteoclast mechanotransduction on Earth, in space, and under conditions of simulated microgravity. The article discusses the need to better understand how osteoclasts are able to function in zero gravity and reviews current and prospective therapies that may be used to treat osteoclast-mediated bone disease.
9

Lysosomal Regulation of Gene Expression

Heur, J. Martin 27 September 2002 (has links)
No description available.
10

The Involvement of Lyn and the SH2-domain-containing Inositol 5’-Phosphatase 1 (SHIP1) in the Negative Regulation of M-CSF-induced Cellular Signaling Events

Baran, Christopher Phillip 12 May 2003 (has links)
No description available.

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