Department of Chemistry, Zhejiang Sci-Tech University, Hangzhou 310018, P. R. China.
Analyst. 2014 Mar 7;139(5):1057-62. doi: 10.1039/c3an01724a. Epub 2014 Jan 14.
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 1 via 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.
已经开发出一种用于蛋白酶活性和抑制剂筛选的实时荧光开启策略。使用了带负电荷的苯并[ghi]菲衍生物(探针 1)。鱼精蛋白是一种阳离子蛋白,可通过强静电和疏水相互作用诱导探针 1 的聚集。探针 1 的荧光被有效地猝灭。在存在蛋白酶的情况下,鱼精蛋白被酶解,探针 1 解聚。可以检测到探针 1 单体荧光的恢复。可以实时监测蛋白酶的活性。此外,加入蛋白酶抑制剂后,抑制了蛋白酶催化的水解,导致荧光恢复减少。因此,荧光测定法也可用于筛选蛋白酶抑制剂。