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dc.contributor.authorJohansson, Helena
dc.date.accessioned2010-09-10T10:54:23Z
dc.date.available2010-09-10T10:54:23Z
dc.date.issued2010-09-10
dc.identifier.isbn978-91-628-8135-1
dc.identifier.urihttp://hdl.handle.net/2077/23135
dc.description.abstractEmbryonic stem (ES) cells provide an unlimited source of cells potentially useful for regenerative medicine, however, prior to clinical implementation, additional basic research is needed. This thesis is focused upon different molecular aspects regarding ES cells, primarily by finding novel stem cell protein-protein interactions and their functions. As functions of a specific protein may be dependent on its interacting partner, identification of such protein-protein interactions is important. Using several different methods, for example in situ proximity ligation assay and co-immunoprecipitation, numerous novel protein-protein interactions occurring in ES cells were found. The same proteins were shown to be involved in several different protein complexes, some of them likely to be part of bigger complexes. Tpt1 and Npm1 were two such proteins found in several different interactions. Tpt1/Npm1 interacted with a prominent peak during mitosis and were proven to be involved in cell proliferation. Individual depletion of Tpt1 and Npm1 resulted in increased levels of markers of the neural and mesodermal lineages, respectively. Further, Npm1 also associated with all three core transcription factors, namely Oct4, Sox2 and Nanog, signifying the importance of Npm1 in ES cells. The Npm1/Sox2 interaction was shown to remain while cells were induced to differentiate into neural lineage, while decreasing in the other differentiation pathways, indicating of an additional role of this protein complex during differentiation to ectoderm. Phosphorylated Ncl was found to interact individually with Tpt1 and Oct4 in a cell cycle dependent manner, speculatively involved in cell proliferation and transcription. In screening for factors binding to Oct4 proximal promoter, SAF-A was found and subsequently shown to be involved in the transcriptional regulation of Oct4. The binding occurred preferentially to unmethylated Oct4 promoter and was reduced when ES cells were induced to differentiate. SAF-A was also found to interact with RNA pol II as well as STAT3, Oct4 and Sox2. In conclusion: twelve novel protein-protein interactions, involved in cell proliferation, differentiation and transcriptional regulation, are presented in this thesis.sv
dc.language.isoengsv
dc.relation.haspartI. Johansson, H., Vizlin-Hodzic, D., Simonsson, T., Simonsson, S. (2010). Translationally controlled tumor protein interacts with nucleophosmin during mitosis in ES cells. Cell Cycle, 9, 2160-2169. ::doi::10.4161/cc.9.11.11841sv
dc.relation.haspartII. Johansson, H., Svensson, F., Simonsson, T., Simonsson, S. (2010). Phosphorylated nucleolin interacts with translationally controlled tumor protein during mitosis and with Oct4 during interphase in ES cells. Submitted manuscript, under revisionsv
dc.relation.haspartIII. Vizlin-Hodzic, D., Johansson, H., Simonsson, T., Simonsson, S. (2010). SAF-A has a role in transcriptional regulation of Oct4 in ES cells through promoter binding. Submitted manuscriptsv
dc.relation.haspartIV. Johansson, H., and Simonsson, S. (2010). Nucleophosmin is in complex with Oct4, Sox2 and Nanog in ES cells. Manuscriptsv
dc.subjectembryonic stem cellssv
dc.subjectTpt1sv
dc.subjectNpm1sv
dc.subjectNclsv
dc.subjectOct4sv
dc.subjectSox2sv
dc.subjectNanogsv
dc.subjectSAF-Asv
dc.subjectcell proliferationsv
dc.subjecttranscriptional regulationsv
dc.titleIdentification of stem cell factors - Novel protein-protein interactions and their functionssv
dc.typetexteng
dc.type.svepDoctoral thesiseng
dc.type.degreeDoctor of Philosophy (Medicine)sv
dc.gup.originUniversity of Gothenburg. Sahlgrenska Academysv
dc.gup.departmentInstitute of Biomedicine. Department of Medical Biochemistry and Cell Biologysv
dc.gup.defenceplaceFredagen den 1 oktober 2010, kl. 9.00, Hörsal Arvid Carlsson, Academicum, Medicinaregatan 3, Göteborgsv
dc.gup.defencedate2010-10-01
dc.gup.dissdb-fakultetSA


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