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Sensitive Liquid Crystal-based Sensor for Monitoring the Enzymatic Activities of Trypsin

机译:基于灵敏液晶的传感器,用于监测胰蛋白酶的酶活性

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摘要

In this study, a highly sensitive and label-free method was developed to monitor the enzymatic activities of trypsin via orientational transition of liquid crystals (LCs) coupled to the interactions between the polyelectrolyte and phospholipid monolayer. Generally, the positively charged polyelectrolyte interacted with the negatively charged phospholipid monolayer by electrostatic interaction, which caused reorganization of the phospholipid membrane and induced a homeotropic to planar orientational transition of LCs. Enzymatic cleavage of the polyelectrolyte, which was caused by trypsin, eliminated the electrostatic interaction that occurred at the aqueous/LC interface and restored the LC alignment. The optical response of the LC changed in a way that corresponded with the LC molecular arrangement, which enables naked-eye detection under polarized optical microscopy. A rather low detection limit, down to 10 ng/mL, was achieved for trypsin activity detection by applying the proposed method.
机译:在这项研究中,开发了一种高度灵敏且无标记的方法,以通过液晶(LC)的取向转变以及聚电解质和磷脂单层之间的相互作用来监测胰蛋白酶的酶活性。通常,带正电的聚电解质通过静电相互作用与带负电的磷脂单层相互作用,这引起磷脂膜的重组,并引起LC的垂直向平面取向转变。胰蛋白酶引起的聚电解质的酶切消除了在水/ LC界面发生的静电相互作用,并恢复了LC排列。 LC的光学响应以与LC分子排列相对应的方式发生了变化,从而可以在偏振光学显微镜下进行肉眼检测。通过应用所提出的方法,对于胰蛋白酶活性的检测达到了相当低的检测限,低至10 ng / mL。

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