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用肽-量子点纳米传感器检测激肽酶蛋白水解活性。

Detecting kallikrein proteolytic activity with peptide-quantum dot nanosensors.

机构信息

Center for Bio/Molecular Science and Engineering, Code 6900, and ‡Optical Sciences Division, Code 5600, U.S. Naval Research Laboratory , Washington, DC, 20375 United States.

出版信息

ACS Appl Mater Interfaces. 2014 Jul 23;6(14):11529-35. doi: 10.1021/am502135h. Epub 2014 Jul 8.

DOI:10.1021/am502135h
PMID:25003700
Abstract

Contamination and adulterants in both naturally derived and synthetic drugs pose a serious threat to the worldwide medical community. Developing rapid and sensitive sensors/devices to detect these hazards is thus a continuing need. We describe a hydrophilic semiconductor quantum dot (QD)-peptide Förster resonance energy transfer (FRET) nanosensor for monitoring the activity of kallikrein, a key proteolytic enzyme functioning at the initiation of the blood clotting cascade. Kallikrein is also activated by the presence of an oversulfated contaminant recently found in preparations of the drug heparin. Quantitatively monitoring the activity of this enzyme within a nanosensor format has proven challenging because of inherent steric and kinetic considerations. Our sensor is designed around a central QD donor platform which displays controlled ratios of a modular peptidyl substrate. This peptide, in turn, sequentially expresses a terminal oligohistidine motif that mediates the rapid self-assembly of peptides to the QD surface, a linker-spacer sequence to extend the peptide away from the QD surface, a kallikrein recognized-cleavage site, and terminates in an acceptor dye-labeling site. Hydrophilic QDs prepared with compact, zwitterionic surface coatings were first evaluated for their ability to self-assemble the dye-labeled peptide substrates. An optimized two-step protocol was then utilized where high concentrations of peptide were initially digested with purified human kallikrein and samples collected at distinct time points were subsequently diluted into QD-containing solutions for assaying. This sensor provided a quantitative FRET-based readout for monitoring kallikrein activity and comparison to a calibration curve allowed estimation of the relevant Michaelis-Menten kinetic descriptors. The results further suggest that almost any protease should be amenable to a QD-based FRET assay format with appropriate design considerations.

摘要

天然和合成药物中的污染和掺杂物对全球医学领域构成了严重威胁。因此,开发快速、灵敏的传感器/设备来检测这些危害是持续的需求。我们描述了一种亲水半导体量子点(QD)-肽Förster 共振能量转移(FRET)纳米传感器,用于监测激肽释放酶的活性,激肽释放酶是凝血级联反应起始时起关键作用的一种关键蛋白水解酶。激肽释放酶也被最近在肝素药物制剂中发现的一种过度硫酸化污染物激活。由于固有空间和动力学考虑,以纳米传感器格式定量监测这种酶的活性具有挑战性。我们的传感器是围绕中央 QD 供体平台设计的,该平台显示出模块化肽底物的受控比例。该肽依次表达一个末端寡组氨酸基序,该基序介导肽快速自组装到 QD 表面,一个连接子间隔序列将肽从 QD 表面延伸开,一个激肽识别的切割位点,并以受体染料标记位点结束。首先评估了具有紧凑、两性离子表面涂层的亲水 QD 自组装染料标记肽底物的能力。然后利用优化的两步方案,最初用人源激肽消化高浓度的肽,并在不同时间点收集样品,然后将其稀释到含有 QD 的溶液中进行测定。该传感器提供了一种基于 FRET 的定量读出,用于监测激肽释放酶的活性,并与校准曲线进行比较,可以估计相关的米氏-门坦动力学描述符。结果进一步表明,几乎任何蛋白酶都可以采用适当设计考虑的基于 QD 的 FRET 测定格式。

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