Gold nanodome SERS platform for label-free detection of protease activity

Author:

Wuytens Pieter C.12345ORCID,Demol Hans64784,Turk Nina12349ORCID,Gevaert Kris64784,Skirtach Andre G.58498,Lamkanfi Mohamed10114128,Baets Roel12349

Affiliation:

1. Photonics Research Group

2. INTEC

3. Ghent University – imec

4. Belgium

5. Department of Molecular Biotechnology

6. VIB-UGent Center for Medical Biotechnology

7. Department of Biochemistry

8. Ghent University

9. Center for Nano- and BioPhotonics

10. Center for Inflammation Research

11. VIB

12. Department of Internal Medicine

Abstract

Surface-enhanced Raman scattering provides a promising technology for sensitive and selective detection of protease activity by monitoring peptide cleavage. Not only are peptides and plasmonic hotspots similarly sized, Raman fingerprints also hold large potential for spectral multiplexing. Here, we use a gold-nanodome platform for real-time detection of trypsin activity on a CALNNYGGGGVRGNF substrate peptide. First, we investigate the spectral changes upon cleavage through the SERS signal of liquid-chromatography separated products. Next, we show that similar patterns are detected upon digesting surface-bound peptides. We demonstrate that the relative intensity of the fingerprints from aromatic amino acids before and after the cleavage site provides a robust figure of merit for the turnover rate. The presented method offers a generic approach for measuring protease activity, which is illustrated by developing an analogous substrate for endoproteinase Glu-C.

Funder

Fonds Wetenschappelijk Onderzoek

Bijzonder Onderzoeksfonds

FP7 Ideas: European Research Council

Publisher

Royal Society of Chemistry (RSC)

Subject

Physical and Theoretical Chemistry

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