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用肽功能化量子点共振能量转移传感器监测肉毒杆菌神经毒素 A 的活性。

Monitoring botulinum neurotoxin a activity with peptide-functionalized quantum dot resonance energy transfer sensors.

机构信息

Division of Biology, Office of Science and Engineering Laboratories, U.S. Food and Drug Administration, Silver Spring, Maryland 20993, USA.

出版信息

ACS Nano. 2011 Apr 26;5(4):2687-99. doi: 10.1021/nn102997b. Epub 2011 Feb 28.

DOI:10.1021/nn102997b
PMID:21361387
Abstract

Botulinum neurotoxins (BoNTs) are extremely potent bacterial toxins that contaminate food supplies along with having a high potential for exploitation as bioterrorism agents. There is a continuing need to rapidly and sensitively detect exposure to these toxins and to verify their active state, as the latter directly affects diagnosis and helps provide effective treatments. We investigate the use of semiconductor quantum dot (QD)-peptide Förster resonance energy transfer (FRET) assemblies to monitor the activity of the BoNT serotype A light chain protease (LcA). A modular LcA peptide substrate was designed and optimized to contain a central LcA recognition/cleavage region, a unique residue to allow labeling with a Cy3 acceptor dye, an extended linker-spacer sequence, and a terminal oligohistidine that allows for final ratiometric peptide-QD-self-assembly. A number of different QD materials displaying charged or PEGylated surface-coatings were evaluated for their ability to self-assemble dye-labeled LcA peptide substrates by monitoring FRET interactions. Proteolytic assays were performed utilizing either a direct peptide-on-QD format or alternatively an indirect pre-exposure of peptide to LcA prior to QD assembly. Variable activities were obtained depending on QD materials and formats used with the most sensitive pre-exposure assay result demonstrating a 350 pM LcA limit of detection. Modeling the various QD-peptide sensor constructs provided insight into how the resulting assembly architecture influenced LcA recognition interactions and subsequent activity. These results also highlight the unique roles that both peptide design and QD features, especially surface-capping agents, contribute to overall sensor activity.

摘要

肉毒杆菌神经毒素(BoNTs)是一种极其有效的细菌毒素,会污染食物供应,同时也具有很高的用作生物恐怖主义制剂的潜力。人们需要不断地快速、灵敏地检测到这些毒素的暴露情况,并验证其活性状态,因为后者直接影响诊断,并有助于提供有效的治疗方法。我们研究了半导体量子点(QD)-肽弗洛里共振能量转移(FRET)组件在监测 BoNT 血清型 A 轻链蛋白酶(LcA)活性方面的应用。设计并优化了一种模块化的 LcA 肽底物,使其包含中央 LcA 识别/切割区域、一个独特的残基,用于用 Cy3 受体染料标记、一个扩展的连接子间隔序列和一个末端寡组氨酸,允许最终进行比率肽-QD 自组装。评估了多种具有带电或 PEG 化表面涂层的不同 QD 材料,以监测 FRET 相互作用,评估它们自组装染料标记的 LcA 肽底物的能力。利用直接的肽-QD 格式或替代的肽在 QD 组装之前预先暴露于 LcA 的间接方法进行蛋白水解测定。根据所使用的 QD 材料和格式,获得了不同的活性,最敏感的预暴露测定结果显示 LcA 的检出限为 350 pM。对各种 QD-肽传感器结构进行建模,深入了解了组装结构如何影响 LcA 识别相互作用和随后的活性。这些结果还突出了肽设计和 QD 特性(特别是表面封端剂)对整体传感器活性的独特作用。

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