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dc.contributor.authorLarsson Berglund, Lisa
dc.date.accessioned2016-04-25T09:04:34Z
dc.date.available2016-04-25T09:04:34Z
dc.date.issued2016-04-25
dc.identifier.isbn978-91-628-9830-4
dc.identifier.urihttp://hdl.handle.net/2077/42358
dc.description.abstractEvery cell is equipped with a protein quality control system to ensure the proper function of proteins. This is essential for both cell maintenance and the generation of new and healthy cells. In this thesis, the budding yeast Saccharomyces cerevisiae is used as a model to study both spatial quality control and the management of the protein involved in Huntington’s disease. The role of the actin cytoskeleton in both these processes has been the special focus of the thesis. Earlier studies established a role for the histone deacetylase Sir2 and the actin cytoskeleton in the asymmetrical inheritance of damaged proteins by the mother cell, as cells either lacking SIR2 or subjected to a transient collapse of the actin cytoskeleton, fail in this segregation process. In this thesis the protein disaggregase Hsp104, the polarisome complex, and the molecular chaperone CCT were identified as additional factors having important functions in the asymmetric segregation of damaged proteins. CCT is an essential, cytosolic folding machine, vital for the production of native actin. The actin folding capacity of CCT appears to be regulated by Sir2. Without this regulation the cell suffers from a reduction in native actin molecules, which could affect the integrity of actin cytoskeletal structures. The polarisome complex ensures actin polymerization at the bud tip and the establishment of a retrograde actin cable flow from the bud to the mother. Our data show that the presence of a functional actin cytoskeleton allows for Hsp104, associated with protein aggregates, to use the actin cytoskeleton as a scaffold and prevent the inheritance of damaged and aggregated proteins by the daughter. The retention of damaged protein within the mother cell is important for the rejuvenation of the daughter cell, as a daughter being born with increased damage suffer from a reduced life span.sv
dc.language.isoengsv
dc.relation.haspartI. Erjavec N, Larsson L, Grantham J, Nyström T (2007) Accelerated aging and failure to segregate damaged proteins in Sir2 mutants can be suppressed by overproducing the protein aggregation-remodeling factor Hsp104p. Genes & Development 21: 2410-21. ::PMID::17908928sv
dc.relation.haspartII. Liu B, Larsson L, Caballero A, Hao X, Oling D, Grantham J, Nyström T (2010) The polarisome is required for segregation and retrograde transport of protein aggregates. Cell 140: 257-67. ::PMID::20141839sv
dc.relation.haspartIII. Liu B, Larsson L, Franssens V, Hao X, Hill SM, Andersson V, Höglund D, Song J, Yang X, Öling D, Grantham J, Winderickx J, Nyström T (2011) Segregation of protein aggregates involves actin and the polarity machinery. Cell 147: 959-61. ::PMID::22118450sv
dc.relation.haspartIV. Song J, Yang Q, Yang J, Larsson L, Hao X, Zhu X, Malmgren-Hill S, Cvijovic M, Fernandez-Rodriguez J, Grantham J, Gustafsson CM, Liu B, Nyström T (2014) Essential genetic interactors of SIR2 required for spatial sequestration and asymmetrical inheritance of protein aggregates. PLoS Genetics 10 e1004539. ::PMID::25079602sv
dc.subjectProtein quality controlsv
dc.subjectActinsv
dc.subjectProtein aggregatesv
dc.subjectSegregationsv
dc.subjectPolarisomesv
dc.subjectCCTsv
dc.subjectHuntingtinsv
dc.titleOn the role of actin in yeast protein quality controlsv
dc.typeTextswe
dc.type.svepDoctoral thesiseng
dc.gup.maillisa.larsson@cmb.gu.sesv
dc.type.degreeDoctor of Philosophysv
dc.gup.originUniversity of Gothenburg. Faculty of Sciencesv
dc.gup.departmentDepartment of Chemistry and Molecular Biology ; Institutionen för kemi och molekylärbiologisv
dc.gup.defenceplaceFredagen den 13:e maj 2016, kl. 9.00, Carl Kylberg, Medicinaregatan 7, Göteborgsv
dc.gup.defencedate2016-05-13
dc.gup.dissdb-fakultetMNF


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