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The URI for Ph,D. , Biochemistry could not be found
To fix, comment below in the following format: MSc http://purl.org/ontology/bibo/degrees/ms
MSc http://purl.org/ontology/bibo/degrees/ms
Record: =LDR 04104cam a2200397 a 4500 =001 2663984 =005 20160321141917.0 =006 m\\f\\d\\\\ =007 he\amu\\bucu =008 070918t20072007kina\\sm\\000\0\eng\d =020 \$a9780494372272 =035 \$a2663984 =040 \$aCaOKQ$beng$cCaOKQ =100 1\$aParsons, Sean Allan. =245 10$aRegulation of inflammation by the Fps/Fes protein tyrosine kinase /$cby Sean Allan Parsons. =264 \1$aKingston, Ont. :$b[publisher not identified],$c[2007] =264 \4$c©2007 =300 \$axv, 109 leaves, :$billustrations (some color) =336 \$atext$btxt$2rdacontent =337 \$acomputer$bc$2rdamedia =338 \$aonline resource$bcr$2rdacarrier =502 \$bPh,D. , Biochemistry$cQueen's University$d2007 =504 \$aIncludes bibliographical references (leaves 93-108) =520 3\$aFps/Fes and Fer are members of a distinct subfamily of cytoplasmic protein tyrosine kinases that have recently been implicated in the regulation of innate immunity. Previous studies showed that mice lacking Fps/Fes are hyper-sensitive to systemic lipopolysaccharide (LPS) challenge. This study identifies physiological, cellular and molecular defects that contribute to the hyper-inflammatory phenotype in Fps/Fes-null mice. We showed that plasma tumour necrosis factor (TNF) -α levels were elevated in LPS challenged Fps/Fes-null mice as compared to wild type mice, and cultured Fps/Fes-null peritoneal macrophages treated with LPS showed increased TNF-α production. Cultured Fps/Fes-null macrophages also displayed prolonged LPS-induced degradation of IkappaB-α, increased phosphorylation of the p65 subunit of NF-kappaB, and defective TLR4 internalization. Next, we showed a role for Fps in the regulation of recruitment of inflammatory leukocytes. Using the cremaster muscle intravital microscopy model, we observed increased leukocyte adherence to venules, and increased rates and degrees of transendothelial migration in Fps/Fes-null mice, compared to wild type. There was also increased neutrophil migration into the peritoneal cavity subsequent to thioglycollate challenge. Using flow cytometry, we observed prolonged expression of the selectin ligand PSGL-1 on peripheral blood neutrophils from Fps/Fes-knockout mice stimulated ex-vivo with LPS. Finally, we examined the role of Fps/Fes in regulating apoptosis in response to inflammation. Upon intra-peritoneal challenge with LPS, Fps/Fes-null mice displayed a decreased depletion of macrophages from the peritoneal cavity. In response to ex-vivo TNF-α stimulation, macrophages from Fps/Fes-null mice underwent decreased apoptosis and necrosis as assessed by flow cytometry. Immunoblot analysis revealed that Fps/Fes-null macrophages displayed more TNF-α-induced degradation of IkappaB-α in Fps/Fes-null cells, with corresponding increases in the phosphorylation of the p65 subunit of NF-kappaB. In addition, stimulation of macrophages with TNF-α up-regulated PARP expression in wild-type macrophages; this up-regulation was not observed in Fps/Fes-null macrophages. Finally we observed a decreased recruitment of macrophages to the peritoneal cavities of Fps/Fes-null mice, with a corresponding increase in neutrophil recruitment, 5 days after thioglycollate challenge. Overall, we show that there is a role for Fps/Fes in regulating inflammation at the physiological, cellular, and molecular levels, and that this might be relevant in inflammatory disease. =533 \$aCopy 2, microfiche.$bOttawa :$cNational Library of Canada,$d[2007] --$e2 microfiches ; 11 x 15 cm. --$f(Canadian theses = Thèses canadiennes) =538 \$aMode of access: World Wide Web. =500 \$aGMD: electronic resource. =653 \$aLipopolysaccharide =653 \$aSepsis =653 \$aTyrosine kinase =653 \$aInflammation =710 2\$aQueen's University (Kingston, Ont.).$tTheses (Queen's University (Kingston, Ont.)) =710 2\$aQueen's University (Kingston, Ont.).$bDepartment of Biochemistry. =830 \0$aCanadian theses. =948 \$ac:sb =902 \$aMARCIVE2013
Record File: 2da561c8ac6cc25c454f77dbf4784a91.mrc
The URI for Ph,D. , Biochemistry could not be found
To fix, comment below in the following format:
MSc http://purl.org/ontology/bibo/degrees/msRecord: =LDR 04104cam a2200397 a 4500 =001 2663984 =005 20160321141917.0 =006 m\\f\\d\\\\ =007 he\amu\\bucu =008 070918t20072007kina\\sm\\000\0\eng\d =020 \$a9780494372272 =035 \$a2663984 =040 \$aCaOKQ$beng$cCaOKQ =100 1\$aParsons, Sean Allan. =245 10$aRegulation of inflammation by the Fps/Fes protein tyrosine kinase /$cby Sean Allan Parsons. =264 \1$aKingston, Ont. :$b[publisher not identified],$c[2007] =264 \4$c©2007 =300 \$axv, 109 leaves, :$billustrations (some color) =336 \$atext$btxt$2rdacontent =337 \$acomputer$bc$2rdamedia =338 \$aonline resource$bcr$2rdacarrier =502 \$bPh,D. , Biochemistry$cQueen's University$d2007 =504 \$aIncludes bibliographical references (leaves 93-108) =520 3\$aFps/Fes and Fer are members of a distinct subfamily of cytoplasmic protein tyrosine kinases that have recently been implicated in the regulation of innate immunity. Previous studies showed that mice lacking Fps/Fes are hyper-sensitive to systemic lipopolysaccharide (LPS) challenge. This study identifies physiological, cellular and molecular defects that contribute to the hyper-inflammatory phenotype in Fps/Fes-null mice. We showed that plasma tumour necrosis factor (TNF) -α levels were elevated in LPS challenged Fps/Fes-null mice as compared to wild type mice, and cultured Fps/Fes-null peritoneal macrophages treated with LPS showed increased TNF-α production. Cultured Fps/Fes-null macrophages also displayed prolonged LPS-induced degradation of IkappaB-α, increased phosphorylation of the p65 subunit of NF-kappaB, and defective TLR4 internalization. Next, we showed a role for Fps in the regulation of recruitment of inflammatory leukocytes. Using the cremaster muscle intravital microscopy model, we observed increased leukocyte adherence to venules, and increased rates and degrees of transendothelial migration in Fps/Fes-null mice, compared to wild type. There was also increased neutrophil migration into the peritoneal cavity subsequent to thioglycollate challenge. Using flow cytometry, we observed prolonged expression of the selectin ligand PSGL-1 on peripheral blood neutrophils from Fps/Fes-knockout mice stimulated ex-vivo with LPS. Finally, we examined the role of Fps/Fes in regulating apoptosis in response to inflammation. Upon intra-peritoneal challenge with LPS, Fps/Fes-null mice displayed a decreased depletion of macrophages from the peritoneal cavity. In response to ex-vivo TNF-α stimulation, macrophages from Fps/Fes-null mice underwent decreased apoptosis and necrosis as assessed by flow cytometry. Immunoblot analysis revealed that Fps/Fes-null macrophages displayed more TNF-α-induced degradation of IkappaB-α in Fps/Fes-null cells, with corresponding increases in the phosphorylation of the p65 subunit of NF-kappaB. In addition, stimulation of macrophages with TNF-α up-regulated PARP expression in wild-type macrophages; this up-regulation was not observed in Fps/Fes-null macrophages. Finally we observed a decreased recruitment of macrophages to the peritoneal cavities of Fps/Fes-null mice, with a corresponding increase in neutrophil recruitment, 5 days after thioglycollate challenge. Overall, we show that there is a role for Fps/Fes in regulating inflammation at the physiological, cellular, and molecular levels, and that this might be relevant in inflammatory disease. =533 \$aCopy 2, microfiche.$bOttawa :$cNational Library of Canada,$d[2007] --$e2 microfiches ; 11 x 15 cm. --$f(Canadian theses = Thèses canadiennes) =538 \$aMode of access: World Wide Web. =500 \$aGMD: electronic resource. =653 \$aLipopolysaccharide =653 \$aSepsis =653 \$aTyrosine kinase =653 \$aInflammation =710 2\$aQueen's University (Kingston, Ont.).$tTheses (Queen's University (Kingston, Ont.)) =710 2\$aQueen's University (Kingston, Ont.).$bDepartment of Biochemistry. =830 \0$aCanadian theses. =948 \$ac:sb =902 \$aMARCIVE2013
Record File: 2da561c8ac6cc25c454f77dbf4784a91.mrc