Issue 5, 2014

Real-time fluorometric turn-on assay for protease activity and inhibitor screening with a benzoperylene probe

Abstract

A real-time fluorescence turn-on strategy for protease activity and inhibitor screening has been developed. A negatively charged benzo[ghi]perylene derivative (probe 1) was employed. Protamine is a cationic protein which can induce aggregation of probe 1via strong electrostatic and hydrophobic interactions. The fluorescence of probe 1 was efficiently quenched. In the presence of a protease, protamine was enzymatically hydrolyzed and probe 1 de-aggregated. The recovery of the probe 1 monomer fluorescence could be detected. The protease activity could be monitored in real-time. In addition, upon addition of a protease inhibitor, the protease-catalyzed hydrolysis was inhibited, which led to a decreased fluorescence recovery. The fluorometric assay thus could also be employed for screening protease inhibitors.

Graphical abstract: Real-time fluorometric turn-on assay for protease activity and inhibitor screening with a benzoperylene probe

Supplementary files

Article information

Article type
Paper
Submitted
10 Sep 2013
Accepted
05 Dec 2013
First published
05 Dec 2013

Analyst, 2014,139, 1057-1062

Real-time fluorometric turn-on assay for protease activity and inhibitor screening with a benzoperylene probe

C. Zhou, W. Li, J. Chen, M. Yang, Y. Li, J. Zhu and C. Yu, Analyst, 2014, 139, 1057 DOI: 10.1039/C3AN01724A

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