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Dive into the research topics where Garry C. King is active.

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Featured researches published by Garry C. King.


Nucleic Acids Research | 2005

Proximity extension of circular DNA aptamers with real-time protein detection

Daniel A. Di Giusto; Wjatschesslaw A. Wlassoff; J. Justin Gooding; Barbara A. Messerle; Garry C. King

Multivalent circular aptamers or ‘captamers’ have recently been introduced through the merger of aptameric recognition functions with the basic principles of DNA nanotechnology. Aptamers have strong utility as protein-binding motifs for diagnostic applications, where their ease of discovery, thermal stability and low cost make them ideal components for incorporation into targeted protein assays. Here we report upon a property specific to circular DNA aptamers: their intrinsic compatibility with a highly sensitive protein detection method termed the ‘proximity extension’ assay. The circular DNA architecture facilitates the integration of multiple functional elements into a single molecule: aptameric target recognition, nucleic acid hybridization specificity and rolling circle amplification. Successful exploitation of these properties is demonstrated for the molecular analysis of thrombin, with the assay delivering a detection limit nearly three orders of magnitude below the dissociation constants of the two contributing aptamer–thrombin interactions. Real-time signal amplification and detection under isothermal conditions points towards potential clinical applications, with both fluorescent and bioelectronic methods of detection achieved. This application elaborates the pleiotropic properties of circular DNA aptamers beyond the stability, potency and multitargeting characteristics described earlier.


ChemBioChem | 2006

Multitasking by multivalent circular DNA aptamers.

Daniel A. Di Giusto; Sarah M. Knox; Yuching Lai; Gregory D. Tyrelle; May T. Aung; Garry C. King

Nucleic acid aptamers are finding increasing applications in biology, especially as therapeutic candidates and diagnostic components. An important characteristic in meeting the needs of these applications is improved stability in physiological fluids, which is most often accomplished with chemical modification or unnatural nucleotides. In an alternative approach we have specified the design of a multivalent circular DNA aptamer topology that encompasses a number of properties relevant to nucleic acid therapeutic candidates, especially the ability to multitask by combining different activities together within a modular structure. Improved stability in blood products, greater conformational stability, antidoting by complementary circular antiaptamers, heterovalency, transcription factor decoy activity and minimal unintended effects upon the cellular innate immune response are desirable properties that are described here. Multitasking by circular DNA aptamers could similarly find applications in diagnostics and biomaterials, where the combination of interchangeable modules might generate new functions, such as anticoagulation coupled with reversible cell capture as, described here. These results provide a platform for further exploration of multivalent circular aptamer properties, especially in novel combinations of nucleic acid therapeutic modes.


Journal of Materials Chemistry | 2005

Nucleic acid biosensors based upon surface-assembled monolayers: exploiting and enhancing materials properties

J. Justin Gooding; Garry C. King

The use of self-assembled monolayers for the fabrication of nucleic acid recognition interfaces has opened up a host of new opportunities for DNA biosensors with regard to (1) exploiting differences in the physical properties of single-stranded DNA probes relative to double-stranded nucleic acids for the development of hybridisation biosensors, and (2) tailoring the interface for the control of protein interactions such that biosensors can be developed, and also to permit access by nucleic acid modifying enzymes for the purposes of sensing and fabrication of nucleic acid nanostructures.


Nucleic Acids Research | 2004

Strong positional preference in the interaction of LNA oligonucleotides with DNA polymerase and proofreading exonuclease activities: implications for genotyping assays.

Daniel A. Di Giusto; Garry C. King


Structure | 1999

The crystal structure of plasminogen activator inhibitor 2 at 2.0 Å resolution: implications for serpin function

Stephen J. Harrop; Lucy Jankova; Murray Coles; Daniel Jardine; Jason S Whittaker; Alison R. Gould; Andreas Meister; Garry C. King; Bridget C. Mabbutt; Paul M. G. Curmi


Journal of the American Chemical Society | 2004

Multipotential electrochemical detection of primer extension reactions on DNA self-assembled monolayers

Daniel A. Di Giusto; Wjatschesslaw A. Wlassoff; Susanne Giesebrecht; J. Justin Gooding; Garry C. King


Journal of Biological Chemistry | 2004

Construction, Stability, and Activity of Multivalent Circular Anticoagulant Aptamers

Daniel A. Di Giusto; Garry C. King


Nucleic Acids Research | 2003

Single base extension (SBE) with proofreading polymerases and phosphorothioate primers: improved fidelity in single‐substrate assays

Daniel A. Di Giusto; Garry C. King


Nucleic Acids Research | 2002

Ferrocene conjugates of dUTP for enzymatic redox labelling of DNA

Wjatschesslaw A. Wlassoff; Garry C. King


Angewandte Chemie | 2004

Enzymatic Synthesis of Redox-Labeled RNA and Dual-Potential Detection at DNA-Modified Electrodes†

Daniel A. Di Giusto; Wjatschesslaw A. Wlassoff; Susanne Giesebrecht; J. Justin Gooding; Garry C. King

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Daniel A. Di Giusto

University of New South Wales

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J. Justin Gooding

University of New South Wales

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Susanne Giesebrecht

University of New South Wales

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Paul M. G. Curmi

University of New South Wales

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Stephen J. Harrop

University of New South Wales

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Alison R. Gould

University of New South Wales

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Andrew P. R. Sutherland

Garvan Institute of Medical Research

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Barbara A. Messerle

University of New South Wales

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