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Label-Free Fluorescent Detection of Trypsin Activity Based on DNA-Stabilized Silver Nanocluster-Peptide Conjugates

机译:基于DNA稳定化的银纳米簇-肽缀合物的胰蛋白酶活性的无标记荧光检测。

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摘要

Trypsin is important during the regulation of pancreatic exocrine function. The detection of trypsin activity is currently limited because of the need for the substrate to be labeled with a fluorescent tag. A label-free fluorescent method has been developed to monitor trypsin activity. The designed peptide probe consists of six arginine molecules and a cysteine terminus and can be conjugated to DNA-stabilized silver nanoclusters (DNA-AgNCs) by Ag-S bonding to enhance fluorescence. The peptide probe can also be adsorbed to the surface of graphene oxide (GO), thus resulting in the fluorescence quenching of DNA-AgNCs-peptide conjugate because of Förster resonance energy transfer. Once trypsin had degraded the peptide probe into amino acid residues, the DNA-AgNCs were released from the surface of GO, and the enhanced fluorescence of DNA-AgNCs was restored. Trypsin can be determined with a linear range of 0.0–50.0 ng/mL with a concentration as low as 1 ng/mL. This label-free method is simple and sensitive and has been successfully used for the determination of trypsin in serum. The method can also be modified to detect other proteases.
机译:胰蛋白酶在调节胰腺外分泌功能中很重要。由于需要用荧光标签标记底物,目前对胰蛋白酶活性的检测受到限制。已经开发了一种无标记的荧光方法来监测胰蛋白酶的活性。设计的肽探针由六个精氨酸分子和一个半胱氨酸末端组成,可以通过Ag-S键结合到DNA稳定的银纳米簇(DNA-AgNCs),以增强荧光。肽探针还可以吸附到氧化石墨烯(GO)的表面,由于Förster共振能量转移,导致DNA-AgNCs-肽共轭物的荧光猝灭。胰蛋白酶将肽探针降解为氨基酸残基后,DNA-AgNCs从GO表面释放出来,并恢复了DNA-AgNCs增强的荧光。胰蛋白酶可以在0.0-50.0 ng / mL的线性范围内测定,浓度低至1 ng / mL。该无标记方法简便,灵敏,已成功用于血清中胰蛋白酶的测定。还可以修改该方法以检测其他蛋白酶。

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