THE EXPRESSION AND PURIFICATION OF GERANYLGERANYLATED KRAS4B

dc.contributor.authorProcter, Lauren
dc.contributor.departmentHood College Biology
dc.contributor.programBiomedical and Environmental Science
dc.date.accessioned2024-03-13T14:11:23Z
dc.date.available2024-03-13T14:11:23Z
dc.date.issued2016-11
dc.description.abstractWildtype KRAS4b is post-translationally modified by cells to include a 15-carbon farnesyl lipid and a methyl group at its C-terminus. The modifications function to anchor KRAS4b on the inner leaflet of the plasma membrane where it serves as a molecular switch to regulate cellular signaling pathways. Mutations in KRAS4b are drivers for 95% of human pancreatic cancer cases, and significant percentages of lung, colorectal, and other types of cancer. In the 1990s, farnesyltransferase inhibitors (FTIs) were developed as a therapeutic to disrupt RAS localization to the cell membrane, and thus prevent its signaling. When it was discovered that KRAS4b localization was not affected due to alternative prenylation by geranylgeranyltransferase-I (GGTase-I), efforts to disrupt membrane localization were diminished. A renewed effort to target RAS-driven cancers, along with a recently published method for producing farnesylated and methylated KRAS4b, provide a strong foundation for generating geranylgeranylated KRAS4b. The expression and purification methods used to generate this alternate form of prenylated KRAS4b are described. Reagent-quality geranylgeranylated KRAS4b will be beneficial in the continued efforts to target RAS-driven cancers.
dc.format.extent46 pages
dc.genreThesis (M.S.)
dc.identifierdoi:10.13016/m2d0gk-2vwa
dc.identifier.urihttp://hdl.handle.net/11603/31960
dc.language.isoen_US
dc.titleTHE EXPRESSION AND PURIFICATION OF GERANYLGERANYLATED KRAS4B
dc.typeText

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