Peptide surfaces were obtained by the covalent immobilisation of fluorescently labelled pentapeptides carboxyfluorescein–glycine–arginine–methionine–leucine–glycine, either directly or through a poly(ethylene glycol) (PEG) linker on modified silicon wafers. Each step during the preparation of the peptide surfaces was confirmed by several surface characterisation techniques. Time-of-flight secondary ion mass spectrometry (ToF-SIMS) and X-ray photoelectron spectroscopy were used to determine the surface composition, the wafers philicity was measured by contact angle and atomic force microscopy was used to investigate the surface morphology. Exposure of the peptide surfaces to trypsin resulted in the release of a fluorescently labelled peptide product, which allowed the kinetics of the enzymatic reaction to be followed with the aid of fluorescence spectroscopy. The electrospray ionisation mass spectrometry analysis of the post-digestion solution confirmed that the pentapeptides attached to the solid support undergo specific trypsin hydrolysis at the C-terminus of the arginine residues. Detailed surface analyses before and after the enzyme action was performed using ToF-SIMS. Because of the limited accessibility of the short peptide directly attached to the surface, a quantitative yield of enzymatic hydrolysis was observed only in case when the peptide was bound through the PEG linker. The insertion of the PEG linker increased the number of immobilised peptides and the rate of enzymatic digestion which consequently improved the quality of the enzyme assays. The described approach may be used for different peptide sequences designed for other proteases.FigureMonitoring of trypsin hydrolysis on PEG-peptide surfaceElectronic supplementary materialThe online version of this article (doi:10.1007/s00216-013-7082-z) contains supplementary material, which is available to authorized users.
This study describes the synthesis and aggregation behavior of thermosensitive poly(di(ethylene glycol) monomethyl ether methacrylate) (P(DEGMA‐ME)) conjugated with the fluorescently labeled pentapeptide glycine‐arginine‐lysine‐phenylalanine‐glycine‐dansyl (GRKFG‐Dns). The GRKFG‐Dns was obtained using Fmoc solid‐phase peptide synthesis and was modified with 2‐bromopropionic acid to initiate an atom transfer radical polymerization of di(ethylene glycol) monomethyl ether methacrylate (DEGMA‐ME). The polymerization led to a well‐defined P(DEGMA‐ME)–GRKFG‐Dns conjugate with a number average molar mass of 108,000 g/mol. The pentapeptide acted as a hydrophilic moiety that increased the phase transition temperature compared to the P(DEGMA‐ME) homopolymer of similar molar mass. The bioconjugate macromolecules aggregated in dilute aqueous solution into spherical particles (mesoglobules). The sizes of aggregates were easily controlled by changing the concentration and heating rate of the P(DEGMA‐ME)‐GRKFG‐Dns solution. The weight average molar masses and sizes of mesoglobules were determined based on light scattering measurements. Enzymatic hydrolysis of the bioconjugate in dilute solution was performed at temperatures below and above the cloud point temperature of the bioconjugate. The peptides were fully accessible to enzymatic digestion even when the macromolecules were aggregated to mesoglobules, indicating that the peptide segments in mesoglobules formed the external shell of the nanoparticles and could be easily released by enzymes. © 2012 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem, 2012
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