Global ETD Search

81	In vitro and ex vivo examination of topical Pomiferin treatment. Gruber, J.V., Holtz, R., Sikkink, Stephen, Tobin, Desmond J. January 2014 (has links) No / Pomiferin is a unique, prenylated isoflavonoid that can be isolated and purified from the fruits of Maclura pomifera (Osage Orange). The molecule typically is isolated with a small amount of a molecule called Osajin which is structurally similar to Pomiferin but lacks an aromatic hydroxyl group. As a consequence, Osajin has been shown to be a less effective antioxidant than Pomiferin. In vitro studies on Normal Human Dermal Fibroblasts demonstrate that Pomiferin is a potent extracellular matrix protein stimulant, showing increases in collagen, elastin and fibrillin expression comparable or superior to equivalent concentrations of retinol. Ex vivo hair follicle assays demonstrate comparable effects on expression of collagen and elastin at Pomiferin concentrations in the range of 0.05–5 ppm. Taken together, the results from the two assays conducted on different models indicate that Pomiferin may be a very interesting ingredient for topical skin and scalp treatments where modulation of the expression of extracellular matrix proteins is important. Maclura pomifera Osage Orange Pomiferin Antioxidant Matrix proteins Follicle Topical skin treatment Human hair Dermal treatment
82	The Screening of Biomaterials to Support Long-term Growth and Maintenance of Human Embryonic Stem Cells in Xeno- and Feeder-free System Pang, Justin Tse Wei 09 December 2013 (has links) Current feeder-free culture systems employing undefined Matrigel are still more effective in maintaining human embryonic stem (ES) cells than defined surfaces using extracellular matrix (ECM) proteins. While the role of substrate stiffness in stem cell fate is becoming increasingly evident, all previous culture systems use ECM proteins on rigid polystyrene surfaces. Here, we used factorial designs to screen and evaluate combinations ECM proteins and substrate stiffness for their effect on short-term pluripotency and self-renewal. Using optimal conditions determined from our screening experiments, defined and near xeno-free culture systems maintained CA1 human ES cells for over 10 passages in Essential 8 (E8) medium. Under these conditions, we found that human ES cell self-renewal was greater on soft polydimethylsiloxane (PDMS) substrates than on rigid polystyrene dishes. The culture systems and screening tools developed in this project will help develop robust and defined xeno-free culture systems that incorporate both biochemical and biomechanical factors. Human Embryonic Stem Cells Biomaterials Extracellular Matrix Proteins Design of Experiments 0541
83	The Screening of Biomaterials to Support Long-term Growth and Maintenance of Human Embryonic Stem Cells in Xeno- and Feeder-free System Pang, Justin Tse Wei 09 December 2013 (has links) Current feeder-free culture systems employing undefined Matrigel are still more effective in maintaining human embryonic stem (ES) cells than defined surfaces using extracellular matrix (ECM) proteins. While the role of substrate stiffness in stem cell fate is becoming increasingly evident, all previous culture systems use ECM proteins on rigid polystyrene surfaces. Here, we used factorial designs to screen and evaluate combinations ECM proteins and substrate stiffness for their effect on short-term pluripotency and self-renewal. Using optimal conditions determined from our screening experiments, defined and near xeno-free culture systems maintained CA1 human ES cells for over 10 passages in Essential 8 (E8) medium. Under these conditions, we found that human ES cell self-renewal was greater on soft polydimethylsiloxane (PDMS) substrates than on rigid polystyrene dishes. The culture systems and screening tools developed in this project will help develop robust and defined xeno-free culture systems that incorporate both biochemical and biomechanical factors. Human Embryonic Stem Cells Biomaterials Extracellular Matrix Proteins Design of Experiments 0541
84	Estudo da expressão do colágeno tipo V e sua relação com a proteína 1 da matriz extracelular no remodelamento da pele de pacientes com líquen escleroso / Study the expression of type V collagen and its relation to extracellular matrix protein 1 remodeling the skin of patients with lichen sclerosus Godoy, Charles Antonio Pires de 16 May 2013 (has links) Introdução: O remodelamento da matriz extracelular no líquen escleroso (LS) caracteriza-se histologicamente por uma faixa hialinizada situada predominantemente na derme superficial, semelhante ao que ocorre na lipoidoproteinose (LPE), uma genodermatose rara, na qual ocorre deficiência na produção da proteína 1 da matriz extracelular (ECM-1). Recentemente, em casos de LS foram descobertos auto-anticorpos contra a ECM-1 e um novo caminho foi proposto para desvendar a sua etiopatologia. O LS também é freqüentemente comparado com a Esclerodermia, visto que alguns autores consideram que são espectros de uma mesma doença. Na Esclerodermia e na LPE há aumento do colágeno tipo V (COL V), mas pouco se sabe sobre este tipo de colágeno no LS. Assim, o objetivo do presente trabalho foi demonstrar a localização e a quantidade de COL V e ECM-1 nas vulvas de pacientes com LS. Materiais e métodos: foram estudadas 21 biópsias de pacientes com LS vulvar e 21 biópsias de vulvas normais. A morfometria foi realizada nas imagens geradas através da imunofluorescência marcada com anticorpos contra os colágenos I (COL I), III (COL III) e V, e também nas de imunoistoquímica para ECM-1. Ademais, utilizou-se microscopia confocal a laser para visualizar o COL V e a ECM-1 na mesma lâmina. Resultados: Peles do grupo controle mostraram fraca e homogênea distribuição das fibras de COL I, III e V na imunofluorescência. Em contraste, peles com LS exibiram desarranjo da arquitetura da derme superficial e difuso aumento da fluorescência das fibras de COL I, III e V na faixa hialina. A fração de área das fibras de COL I, III, e V foram significativamente maiores nas peles de pacientes com LS em relação ao controle (p<0,05). Peles controles mostraram co-localização da ECM-1 e do COL V na parede de pequenos vasos e ao longo da membrana basal. Entretanto, no LS houve perda de expressão da ECM-1 na parede dos vasos sanguíneos (p<0,001) e difuso aumento da fluorescência verde do COL V (p<0,001). Conclusão: Houve inversa relação entre o COL V e a proteína ECe constatado pela histomorfometria, imunofluorescência, imunoistoquímica e reconstrução tridimensional, sugerindo que estratégias terapêuticas para prevenir o aumento da síntese de COL V e a diminuição da ECM-1 poderão ser promissoras no prognóstico e tratamento do LS / Background: The extracellular matrix remodeling in lichen sclerosus (LS) is characterized in routine light microscopy by a hyalinized band predominantly located in the superficial dermis. The same pattern occurs in the lipoid proteinosis (LPE), a rare genodermatosis, in which the production deficiency of extracellular matrix protein 1 (ECM-1) is responsible for triggering the disease. Recently, in cases of LS, autoantibodies were discovered against ECM-1 and a new way to unravel their aetiopathology was proposed. LS is also frequently compared with Scleroderma, since some authors consider that they are spectra of a similar disease. In Scleroderma and LPE there is an increase of type V collagen (COL V), but little is known about this type of collagen in LS. Thus, the objective of the current study was to demonstrate the location and quantity of COL V and ECM-1 on the vulvas of patients with LS. Materials and methods: Twenty one biopsies from patients with vulvar LS matched with 21 biopsies from normal vulvas were included in this study. Immunofluorescence against type I (COL I), (COL III) and V collagen and immunohistochemistry for ECM-1 was performed and the slides were analysed by morphometry. Furthermore, laser confocal microscopy was used to visualize the COL V fibers and the ECM-1 protein on the same slide. Results: Skins of the control group showed low and homogeneous distribution of fibers COL I, III and V in immunofluorescence. In contrast, skins with LS exhibited disruption of the architecture of the superficial dermis and diffuse increase in fluorescence fibers COL I, III and V in the range hyaline. The area fraction of fibers COL I, III, and V were significantly higher in the skin of patients with LS compared to control (p <0.05). Skins controls showed colocalization of ECM-1 and COL V the wall of small vessels and along the basement membrane. However, the LS had loss of expression of ECM-1 the wall of blood vessels (p <0.001) increase the fluorescence and diffuse green COL V (p <0.001). Conclusion: There was an inverse relationship between COL V and ECM-1 protein in LS as demonstrated by histomorphometry, immunofluorescence, immunohistochemistry and three-dimensional reconstruction, suggesting that therapeutic strategies to prevent the increased synthesis COL V and ECM-1 protein in LS as demonstrated by histomorphometry, immunofluorescence, immunohistochemistry and three-dimensional reconstruction, suggesting that therapeutic strategies to prevent the increased synthesis COL V and decreased ECM-1 may be promising in the prognosis and treatment of the LS Colágeno Collagen Confocal microscopy Extracellular matrix proteins Hialina Hyalin Imunofluorescence Imunofluorescência Lichen sclerosus Líquen escleroso Microscopia confocal Proteínas da matriz extracelular
85	O papel de Aae na adesão às proteínas de matriz extracelular e sua influência nas propriedades hidrofóbicas e formação de biofilme por Aggregatibacter actinomycetemcomitans. / The role of Aae in mediating adhesion to extracellular matrix proteins and its influence on hydrophobic properties and biofilm formation by Aggregatibacter actinomycetemcomitans. Nunes, Ana Carla Robatto 09 September 2009 (has links) O microrganismo gram-negativo Aggregatibacter actinomycetemcomitans, fortemente associado a quadros de periodontite agressiva, coloniza a cavidade oral, aderindo e invadindo as células epiteliais e participando da formação de biofilme nas superfícies do hospedeiro. A. actinomycetemcomitans expressa Aae, uma proteína de superfície, relacionada com a adesão às células epiteliais. Este estudo avaliou o papel de Aae na adesão a outros substratos tais como proteínas extracelulares colagenosas e não-colagenosas, hidroxiapatita recoberta por saliva (SHA) e na formação de biofilme. Um mutante nulo em aae foi construído e o fenótipo comparado com o da linhagem selvagem (VT1169). O mutante nulo exibiu significativa redução na adesão às células epiteliais e a SHA, na formação de biofilme, além de apresentar-se menos hidrofóbico que a linhagem parental. A capacidade de adesão ao colágeno V e a fibronectina foi fracamente afetada pela interrupção do gene aae. Entretanto, o mutante nulo em aae exibiu uma capacidade diminuída na adesão à laminina e colágenos I, III e IV. Estes dados sugerem que Aae desempenha um importante papel na colonização da cavidade oral, não somente promovendo sua adesão às células epiteliais, mas também a outros substratos. / The gram-negative organism Aggregatibacter actinomycetemcomitans, associated with aggressive periodontitis, colonizes the oral cavity by binding to and invading epithelial cells and by participating in biofilms formed in host surfaces. A. actinomycetemcomitans express Aae, a surface protein, implicated in the adhesion to epithelial cells. This study evaluated the role of Aae in adhesion to other substrates such as collagen and non-collagen extracellular matrix proteins and saliva coated hydroxyapatite (SHA) and in biofilm formation. A null mutant in aae was constructed and its behavior was compared with the wild type strain VT1169. The null mutant exhibited a decreased ability to bind to epithelial cells and to SHA, formed less biofilm and was less hydrophobic than the parental strain. The abilities to bind to collagen V and fibronectin were very poorly affected by aae interruption. However, the null aae mutant exhibited a decreased ability to adhere to laminin, collagen I, III and IV. These data suggest that Aae may play an important role in the colonization of the oral cavity by A. actinomycetemcomitans, not only by promoting its adhesion to epithelial cells, but by mediating adhesion to other substrates. Aggregatibacter actinomycetemcomitans Aggregatibacter actinomycetemcomitans Aae Aae Adesão Adhesion Extracellular matrix proteins Hidrofobicidade Hydrophobicity Microbiologia Microbiology Proteínas de matriz extracelular
86	Epstein-Barr virus (EBV) genotyping in EBV-associated lesions. / CUHK electronic theses & dissertations collection January 2004 (has links) Tong Hung Man Joanna. / "June 2004." / Thesis (Ph.D.)--Chinese University of Hong Kong, 2004. / Includes bibliographical references (p. 137-149). / Electronic reproduction. Hong Kong : Chinese University of Hong Kong, [2012] System requirements: Adobe Acrobat Reader. Available via World Wide Web. / Mode of access: World Wide Web. / Abstracts in English and Chinese. Epstein-Barr virus Viral carcinogenesis Nasopharynx--Cancer Herpesvirus 4, Human Neoplasms--etiology Genotype Viral Matrix Proteins Nasopharyngeal Neoplasms--genetics
87	Estudo da expressão do colágeno tipo V e sua relação com a proteína 1 da matriz extracelular no remodelamento da pele de pacientes com líquen escleroso / Study the expression of type V collagen and its relation to extracellular matrix protein 1 remodeling the skin of patients with lichen sclerosus Charles Antonio Pires de Godoy 16 May 2013 (has links) Introdução: O remodelamento da matriz extracelular no líquen escleroso (LS) caracteriza-se histologicamente por uma faixa hialinizada situada predominantemente na derme superficial, semelhante ao que ocorre na lipoidoproteinose (LPE), uma genodermatose rara, na qual ocorre deficiência na produção da proteína 1 da matriz extracelular (ECM-1). Recentemente, em casos de LS foram descobertos auto-anticorpos contra a ECM-1 e um novo caminho foi proposto para desvendar a sua etiopatologia. O LS também é freqüentemente comparado com a Esclerodermia, visto que alguns autores consideram que são espectros de uma mesma doença. Na Esclerodermia e na LPE há aumento do colágeno tipo V (COL V), mas pouco se sabe sobre este tipo de colágeno no LS. Assim, o objetivo do presente trabalho foi demonstrar a localização e a quantidade de COL V e ECM-1 nas vulvas de pacientes com LS. Materiais e métodos: foram estudadas 21 biópsias de pacientes com LS vulvar e 21 biópsias de vulvas normais. A morfometria foi realizada nas imagens geradas através da imunofluorescência marcada com anticorpos contra os colágenos I (COL I), III (COL III) e V, e também nas de imunoistoquímica para ECM-1. Ademais, utilizou-se microscopia confocal a laser para visualizar o COL V e a ECM-1 na mesma lâmina. Resultados: Peles do grupo controle mostraram fraca e homogênea distribuição das fibras de COL I, III e V na imunofluorescência. Em contraste, peles com LS exibiram desarranjo da arquitetura da derme superficial e difuso aumento da fluorescência das fibras de COL I, III e V na faixa hialina. A fração de área das fibras de COL I, III, e V foram significativamente maiores nas peles de pacientes com LS em relação ao controle (p<0,05). Peles controles mostraram co-localização da ECM-1 e do COL V na parede de pequenos vasos e ao longo da membrana basal. Entretanto, no LS houve perda de expressão da ECM-1 na parede dos vasos sanguíneos (p<0,001) e difuso aumento da fluorescência verde do COL V (p<0,001). Conclusão: Houve inversa relação entre o COL V e a proteína ECe constatado pela histomorfometria, imunofluorescência, imunoistoquímica e reconstrução tridimensional, sugerindo que estratégias terapêuticas para prevenir o aumento da síntese de COL V e a diminuição da ECM-1 poderão ser promissoras no prognóstico e tratamento do LS / Background: The extracellular matrix remodeling in lichen sclerosus (LS) is characterized in routine light microscopy by a hyalinized band predominantly located in the superficial dermis. The same pattern occurs in the lipoid proteinosis (LPE), a rare genodermatosis, in which the production deficiency of extracellular matrix protein 1 (ECM-1) is responsible for triggering the disease. Recently, in cases of LS, autoantibodies were discovered against ECM-1 and a new way to unravel their aetiopathology was proposed. LS is also frequently compared with Scleroderma, since some authors consider that they are spectra of a similar disease. In Scleroderma and LPE there is an increase of type V collagen (COL V), but little is known about this type of collagen in LS. Thus, the objective of the current study was to demonstrate the location and quantity of COL V and ECM-1 on the vulvas of patients with LS. Materials and methods: Twenty one biopsies from patients with vulvar LS matched with 21 biopsies from normal vulvas were included in this study. Immunofluorescence against type I (COL I), (COL III) and V collagen and immunohistochemistry for ECM-1 was performed and the slides were analysed by morphometry. Furthermore, laser confocal microscopy was used to visualize the COL V fibers and the ECM-1 protein on the same slide. Results: Skins of the control group showed low and homogeneous distribution of fibers COL I, III and V in immunofluorescence. In contrast, skins with LS exhibited disruption of the architecture of the superficial dermis and diffuse increase in fluorescence fibers COL I, III and V in the range hyaline. The area fraction of fibers COL I, III, and V were significantly higher in the skin of patients with LS compared to control (p <0.05). Skins controls showed colocalization of ECM-1 and COL V the wall of small vessels and along the basement membrane. However, the LS had loss of expression of ECM-1 the wall of blood vessels (p <0.001) increase the fluorescence and diffuse green COL V (p <0.001). Conclusion: There was an inverse relationship between COL V and ECM-1 protein in LS as demonstrated by histomorphometry, immunofluorescence, immunohistochemistry and three-dimensional reconstruction, suggesting that therapeutic strategies to prevent the increased synthesis COL V and ECM-1 protein in LS as demonstrated by histomorphometry, immunofluorescence, immunohistochemistry and three-dimensional reconstruction, suggesting that therapeutic strategies to prevent the increased synthesis COL V and decreased ECM-1 may be promising in the prognosis and treatment of the LS Colágeno Hialina Imunofluorescência Líquen escleroso Microscopia confocal Proteínas da matriz extracelular Collagen Confocal microscopy Extracellular matrix proteins Hyalin Imunofluorescence Lichen sclerosus
88	Elastin synthesis in the fetal sheep lung in vivo : effects of physical, metabolic and endocrine factors Joyce, Belinda Jane January 2004 (has links) Abstract not available Elastin -- Synthesis Lungs -- Growth Sheep -- Fetuses -- Physiology Fetus -- Growth Fetal growth retardation
89	The role of connective tissue growth factor (ctgf) in oval cell aided liver regeneration in the 2-aaf/phx model Pi, Liya, January 2005 (has links) Thesis (Ph.D.)--University of Florida, 2005. / Typescript. Title from title page of source document. Document formatted into pages; contains 162 pages. Includes Vita. Includes bibliographical references.
90	O papel de Aae na adesão às proteínas de matriz extracelular e sua influência nas propriedades hidrofóbicas e formação de biofilme por Aggregatibacter actinomycetemcomitans. / The role of Aae in mediating adhesion to extracellular matrix proteins and its influence on hydrophobic properties and biofilm formation by Aggregatibacter actinomycetemcomitans. Ana Carla Robatto Nunes 09 September 2009 (has links) O microrganismo gram-negativo Aggregatibacter actinomycetemcomitans, fortemente associado a quadros de periodontite agressiva, coloniza a cavidade oral, aderindo e invadindo as células epiteliais e participando da formação de biofilme nas superfícies do hospedeiro. A. actinomycetemcomitans expressa Aae, uma proteína de superfície, relacionada com a adesão às células epiteliais. Este estudo avaliou o papel de Aae na adesão a outros substratos tais como proteínas extracelulares colagenosas e não-colagenosas, hidroxiapatita recoberta por saliva (SHA) e na formação de biofilme. Um mutante nulo em aae foi construído e o fenótipo comparado com o da linhagem selvagem (VT1169). O mutante nulo exibiu significativa redução na adesão às células epiteliais e a SHA, na formação de biofilme, além de apresentar-se menos hidrofóbico que a linhagem parental. A capacidade de adesão ao colágeno V e a fibronectina foi fracamente afetada pela interrupção do gene aae. Entretanto, o mutante nulo em aae exibiu uma capacidade diminuída na adesão à laminina e colágenos I, III e IV. Estes dados sugerem que Aae desempenha um importante papel na colonização da cavidade oral, não somente promovendo sua adesão às células epiteliais, mas também a outros substratos. / The gram-negative organism Aggregatibacter actinomycetemcomitans, associated with aggressive periodontitis, colonizes the oral cavity by binding to and invading epithelial cells and by participating in biofilms formed in host surfaces. A. actinomycetemcomitans express Aae, a surface protein, implicated in the adhesion to epithelial cells. This study evaluated the role of Aae in adhesion to other substrates such as collagen and non-collagen extracellular matrix proteins and saliva coated hydroxyapatite (SHA) and in biofilm formation. A null mutant in aae was constructed and its behavior was compared with the wild type strain VT1169. The null mutant exhibited a decreased ability to bind to epithelial cells and to SHA, formed less biofilm and was less hydrophobic than the parental strain. The abilities to bind to collagen V and fibronectin were very poorly affected by aae interruption. However, the null aae mutant exhibited a decreased ability to adhere to laminin, collagen I, III and IV. These data suggest that Aae may play an important role in the colonization of the oral cavity by A. actinomycetemcomitans, not only by promoting its adhesion to epithelial cells, but by mediating adhesion to other substrates. Aggregatibacter actinomycetemcomitans Aae Adesão Hidrofobicidade Microbiologia Proteínas de matriz extracelular Aggregatibacter actinomycetemcomitans Aae Adhesion Extracellular matrix proteins Hydrophobicity Microbiology

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