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Creation and Characterization of a Fluorescence Signalling DNA Enzyme

dc.contributor.advisorLi, Yingfu
dc.contributor.authorMei, Shirley
dc.contributor.departmentBiochemistryen_US
dc.date.accessioned2018-05-02T15:56:12Z
dc.date.available2018-05-02T15:56:12Z
dc.date.issued2003-09
dc.description.abstract𝘐𝘯 𝘷𝘪𝘵𝘳𝘰 selection has been widely used to isolate single-stranded DNA molecules from large random-sequence pools that are able to perform a desired catalytic reaction, or bind to a target molecule. Using this technique, we have created a DNA enzyme, named DET22-18, which has a uniquely linked chemical catalysis/real-time signaling capability. It is a true enzyme with a 𝘬cₐₜ of~7 min⁻¹ -the second fastest rate ever reported for a DNA enzyme. The DNA enzyme cleaves a substrate containing a single ribonucleotide linkage embedded in a DNA chain and sandwiched between a fluorophore-labeled deoxyribonucleotide and a quencher-modified deoxyribonucleotide. The ability of DET22-18 to generate a large fluorescence signal provides a useful tool to engineer potential allosteric deoxyribozyme biosensors for real-time detection of important biological targets. To provide a proof of concept that a reporter system can be built from the above signaling DNA enzyme, the cis-acting version of this enzyme, DEC22-18A, was engineered into an allosterically regulated deoxyribozyme biosensor that can report ATP. A preliminary investigation was also conducted to determine a possible secondary structure of the DNA enzyme. This study lays a foundation for pursuing novel signaling DNA enzymes for biological detection directed applications.en_US
dc.description.degreeMaster of Science (MSc)en_US
dc.description.degreetypeThesisen_US
dc.identifier.urihttp://hdl.handle.net/11375/22784
dc.language.isoenen_US
dc.subjectfluorescenceen_US
dc.subjectDNAen_US
dc.subjectenzymeen_US
dc.subjectin vitroen_US
dc.titleCreation and Characterization of a Fluorescence Signalling DNA Enzymeen_US
dc.title.alternativeA Fluorescence Signalling DNA Enzymeen_US
dc.typeThesisen_US

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