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Enzyme-amplified array sensing of proteins in solution and in biofluids.


ABSTRACT: We have developed an enzyme-nanoparticle sensor array where the sensitivity is amplified through enzymatic catalysis. In this approach cationic gold nanoparticles are electrostatically bound to an enzyme (beta-galactosidase, beta-Gal), inhibiting enzyme activity. Analyte proteins release the beta-Gal, restoring activity and providing an amplified readout of the binding event. Using this strategy we have been able to identify proteins in buffer at a concentration of 1 nM, substantially lower than current strategies for array-based protein sensing. Moreover, we have obtained identical sensitivity in studies where the proteins are spiked into the complex protein matrix provided by desalted human urine ( approximately 1.5 muM total protein; spiked protein concentrations were 0.067% of the overall protein concentration), demonstrating the potential of the method for diagnostic applications.

SUBMITTER: Miranda OR 

PROVIDER: S-EPMC2855490 | biostudies-literature | 2010 Apr

REPOSITORIES: biostudies-literature

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Enzyme-amplified array sensing of proteins in solution and in biofluids.

Miranda Oscar R OR   Chen Hung-Ting HT   You Chang-Cheng CC   Mortenson David E DE   Yang Xiao-Chao XC   Bunz Uwe H F UH   Rotello Vincent M VM  

Journal of the American Chemical Society 20100401 14


We have developed an enzyme-nanoparticle sensor array where the sensitivity is amplified through enzymatic catalysis. In this approach cationic gold nanoparticles are electrostatically bound to an enzyme (beta-galactosidase, beta-Gal), inhibiting enzyme activity. Analyte proteins release the beta-Gal, restoring activity and providing an amplified readout of the binding event. Using this strategy we have been able to identify proteins in buffer at a concentration of 1 nM, substantially lower than  ...[more]

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