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dc.contributor.advisorFlint, Janeen_US
dc.contributor.authorDeHart, Carolineen_US
dc.contributor.otherMolecular Biology Departmenten_US
dc.date.accessioned2013-09-16T17:25:47Z-
dc.date.available2013-09-16T17:25:47Z-
dc.date.issued2013en_US
dc.identifier.urihttp://arks.princeton.edu/ark:/88435/dsp01bv73c053r-
dc.description.abstractThe p53 tumor suppressor protein is a central component of numerous cellular signaling pathways and frequently mutated in human cancers. p53 undergoes extensive post-translational modification (PTM) in response to specific stressors and other cellular events, resulting in a combinatorial PTM code that may direct its stability, localization, and activity within the cell. p53 accumulates dramatically when normal or transformed cells are subjected to infection by a human adenovirus type 5 (Ad5) E1B 55 kDa-null mutant, which lacks the virus-specific ubiquitin ligase that targets p53 for proteasomal degradation. This population of p53 has been shown to localize normally, but is unable to activate transcription of p53 target genes. The mechanism by which this repression of p53 transcriptional activity occurs is unknown. One hypothesis was that the transcriptionally inert status of p53 might be due, in part, to PTM. The p53 protein that accumulates within adenoviral E1B 55 kDa null mutant-infected normal cells presented a unique opportunity to isolate an endogenous population of wild-type, transcriptionally inert p53 for analysis of PTM by mass spectrometry. In Chapter 2, this system was utilized to generate an expanded modification profile for transcriptionally inert human p53 and to compare this profile to one generated from an equivalent population of transcriptionally active human p53, in order to identify patterns of modifications potentially responsible for modulating p53 transcriptional function. While there were no significant differences in the PTM of transcriptionally inert and active p53, the wealth of PTMs identified suggested the possibility of a far greater degree of combinatorial regulation of p53 by PTM than previously anticipated. Additionally, p53 was recently reported to exhibit transcriptional activity in normal human cells infected by an E1B 55 kDa/E4orf3 double null mutant. In Chapter 3, an E1B 55 kDa/E4orf3 double null mutant was constructed for the purpose of clarifying the role of E4orf3 in the inhibition of p53-dependent target gene transcription, in addition to ascertaining whether the differences in p53 transcriptional activity or selectivity observed during infection with an E1B 55 kDa- or E1B 55 kDa/E4orf3-null mutant were in any way due to differential patterns of p53 PTM.en_US
dc.language.isoenen_US
dc.publisherPrinceton, NJ : Princeton Universityen_US
dc.relation.isformatofThe Mudd Manuscript Library retains one bound copy of each dissertation. Search for these copies in the <a href=http://catalog.princeton.edu> library's main catalog </a>en_US
dc.subjectAdenovirusen_US
dc.subjectMass spectrometryen_US
dc.subjectp53en_US
dc.subjectPTMen_US
dc.subject.classificationMolecular biologyen_US
dc.titleExtensive Post-Translational Modification of Endogenous Human p53en_US
dc.typeAcademic dissertations (Ph.D.)en_US
pu.projectgrantnumber690-2143en_US
Appears in Collections:Molecular Biology

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