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Please use this identifier to cite or link to this item: http://arks.princeton.edu/ark:/88435/dsp016d56zz92g
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dc.contributor.advisorKorennykh, Alexei-
dc.contributor.authorChu, Jacqueline-
dc.date.accessioned2015-06-22T18:22:35Z-
dc.date.available2015-06-22T18:22:35Z-
dc.date.created2015-04-24-
dc.date.issued2015-06-22-
dc.identifier.urihttp://arks.princeton.edu/ark:/88435/dsp016d56zz92g-
dc.description.abstractRibonuclease L is an important effector of the type I IFN pathway in response to viral RNAs. In response to activation by 2-5As, RNase L cleaves both viral and cellular mRNAs. However, there is increasing interest in the roles of RNase L under homeostatic conditions. RNase L has been shown to cleave specific cellular mRNAs that have functions in proliferation and differentiation, but it is still unclear as to how RNase L is able to specifically target these RNAs. In order to elucidate the mechanism of RNase L substrate targeting, this study focused on determining the mechanism through which RNase L is localized. Deep sequencing, immunoblots, and a new localization assay developed for this study, all reveal a nuclear/cytoskeletal enrichment of both RNase L mRNA and protein. In addition, deep sequencing revealed an association of RNase L with RNAs of membrane-bound proteins. Based on this data, it is evident that studying the mechanism of RNase L mRNA localization can reveal how RNase L protein is localized, which has implications for how RNase L targets is substrates. In order to further study the connection between RNase L mRNA and localization of RNase L protein, two RNase L mutants were designed that study different possible mechanisms of RNase L mRNA spatial control of translation.en_US
dc.format.extent79 pages*
dc.language.isoen_USen_US
dc.titleRNase L localization studies in human cells and potential applications of RNase L modulation in cancer immunotherapyen_US
dc.typePrinceton University Senior Theses-
pu.date.classyear2015en_US
pu.departmentMolecular Biologyen_US
pu.pdf.coverpageSeniorThesisCoverPage-
Appears in Collections:Molecular Biology, 1954-2020

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