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Photoactive hydrogels for pre-concentration, labelling, and controlled release of proteins.


ABSTRACT: We report a novel hydrogel for pre-concentration, fluorescent labelling, and light-triggered release of proteins for detection of low abundance biomarkers. The hydrogel was a co-polymer of acrylamide/bisacrylamide and methacrylamide attached to fluorescein isothiocyanate via a light cleavable bond and a poly(ethylene glycol) spacer arm of molecular weight of 3400 g mol-1. Unlike previous work, proteins were captured by an irreversible chemical reaction rather than by non-covalent affinity binding or physical entrapment. Because the protein-reactive group was attached to fluorescein, which in turn was coupled to the hydrogel by a photocleavable bond, on release the protein was labelled with fluorescein. Our hydrogel offered a pre-concentration factor of up to 236 for a model protein, streptavidin. Each protein molecule was labelled with 85 fluorescein molecules, and 50% of the proteins in the hydrogel were released after UV exposure for ∼100 s. The proteins released from the hydrogel were captured in biotinylated microtitre plates and detected by fluorescence, allowing measurement of at least 0.01 ppm (or ∼166 pM) of protein in sample solutions. The reported hydrogel is promising for detection of low abundance proteins while being less laborious than enzyme-linked immunosorbent assay and less affected by changes in environmental conditions than label-free biosensors.

SUBMITTER: Kellermann L 

PROVIDER: S-EPMC10440800 | biostudies-literature | 2023 Aug

REPOSITORIES: biostudies-literature

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Photoactive hydrogels for pre-concentration, labelling, and controlled release of proteins.

Kellermann Leanne L   Gupta Ruchi R  

The Analyst 20230821 17


We report a novel hydrogel for pre-concentration, fluorescent labelling, and light-triggered release of proteins for detection of low abundance biomarkers. The hydrogel was a co-polymer of acrylamide/bisacrylamide and methacrylamide attached to fluorescein isothiocyanate <i>via</i> a light cleavable bond and a poly(ethylene glycol) spacer arm of molecular weight of 3400 g mol<sup>-1</sup>. Unlike previous work, proteins were captured by an irreversible chemical reaction rather than by non-covale  ...[more]

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