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- All Subjects: Molecular Biology
- Genre: Masters Thesis
Description
Recombinases are powerful tools for genome engineering and synthetic biology, however recombinases are limited by a lack of user-programmability and often require complex directed-evolution experiments to retarget specificity. Conversely, CRISPR systems have extreme versatility yet can induce off-target mutations and karyotypic destabilization. To address these constraints we developed an RNA-guided recombinase protein by fusing a hyperactive mutant resolvase from transposon TN3 to catalytically inactive Cas9. We validated recombinase-Cas9 (rCas9) function in model eukaryote Saccharomyces cerevisiae using a chromosomally integrated fluorescent reporter. Moreover, we demonstrated cooperative targeting by CRISPR RNAs at spacings of 22 or 40bps is necessary for directing recombination. Using PCR and Sanger sequencing, we confirmed rCas9 targets DNA recombination. With further development we envision rCas9 becoming useful in the development of RNA-programmed genetic circuitry as well as high-specificity genome engineering.
ContributorsStandage-Beier, Kylie S (Author) / Wang, Xiao (Thesis advisor) / Brafman, David A (Committee member) / Tian, Xiao-jun (Committee member) / Arizona State University (Publisher)
Created2018
Description
Extrachromosomal circular DNA (eccDNA) has become an increasingly popular subject of study in eukaryotic cell biology due to its prevalence in human cancer. Though the literature reports a consensus regarding DNA break repair as a driver of eccDNA formation, there remains a lack of knowledge surrounding the exact mechanisms for eccDNA formation and the selective dynamics that promote their retainment in a cell or population. A central issue to studying eccDNA is the inability to distinguish between linear and circular DNA of homologous sequence. The work presented here describes an adapted eccDNA enrichment and detection assay, specifically for investigating the effects of manipulating a known eccDNA-forming locus in the budding yeast Saccharomyces cerevisiae. First, a galactose inducible GFP reporter was integrated within the copper inducible CUP1 tandem repeat locus of yeast cells. The eccDNA enrichment and detection assay was first applied to wildtype yeast to demonstrate the presence of CUP1 eccDNA in copper induced cells by qPCR. Although subsequent sequencing analysis failed to validate this result, it indicated the presence of various other known and previously un-reported eccDNA species. Finally, application of the enrichment protocol and qPCR detection assay to CUP1-GFP reporter cells yielded inconclusive results, suggesting the assay requires further optimization to sensitively detect eccDNA from this altered locus. While more work is necessary to draw conclusions regarding the limits of eccDNA production at a manipulated eccDNA-forming locus, this knowledge will lend to the potential for therapeutically targeting eccDNA at the point of de novo formation.
ContributorsKeal, Tula (Author) / Wang, Xiao (Thesis advisor) / Tian, Xiaojun (Committee member) / Plaisier, Christopher (Committee member) / Arizona State University (Publisher)
Created2022