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基于 SAM-AuNIs LSPR 生物传感器直接检测两种不同肿瘤来源的细胞外囊泡。

Direct detection of two different tumor-derived extracellular vesicles by SAM-AuNIs LSPR biosensor.

机构信息

Department of Biomedical Sciences, City University of Hong Kong, Hong Kong SAR, Hong Kong.

Department of Physics and Materials Science, City University of Hong Kong, Hong Kong SAR, Hong Kong.

出版信息

Biosens Bioelectron. 2017 Aug 15;94:400-407. doi: 10.1016/j.bios.2017.03.036. Epub 2017 Mar 18.

DOI:10.1016/j.bios.2017.03.036
PMID:28324860
Abstract

Extracellular vesicles (EVs) are abundant in various biological fluids including blood, saliva, urine, as well as extracellular milieu. Accumulating evidence has indicated that EVs, which contain functional proteins and small RNAs, facilitate intercellular communication between neighbouring cells, and are critical to maintain various physiological processes. In contrast, EV-derived toxic signals can spread out over the tissues adjacent to the injured area in certain diseases, including brain tumors and neurodegenerative disorders. This demands better characterization of EVs which can be employed for liquid biopsy clinically as well as for the study of intercellular signalling. Exosomes and microvesicles share a number of similar characteristics, but it is important to distinguish between these two types of EVs. Here, we report for the first time that our in-house developed Localized Surface Plasmon Resonance biosensor with self-assembly gold nanoislands (SAM-AuNIs) can be used to detect and distinguish exosomes from MVs isolated from A-549 cells, SH-SY5Y cells, blood serum, and urine from a lung cancer mouse model. Exosomes, compared with MVs, produced a distinguishable response to the bare LSPR biosensor without functionalization, suggesting a different biophysical interaction between exosomes and MVs with SAM AuNIs. This sensor attains the limit of detection to 0.194µg/ml, and the linear dynamic range covers 0.194-100µg/ml. This discovery not only reveals great insight into the distinctive membrane property of tumor-derived exosomes and MVs, but also facilitate the development of novel LSPR biosensors for direct detection and isolation of heterogeneous EVs.

摘要

细胞外囊泡(EVs)在各种生物体液中大量存在,包括血液、唾液、尿液以及细胞外环境。越来越多的证据表明,EVs 含有功能性蛋白质和小 RNA,可促进邻近细胞之间的细胞间通讯,对维持各种生理过程至关重要。相比之下,EV 衍生的毒性信号可以在某些疾病中扩散到受伤区域附近的组织中,包括脑肿瘤和神经退行性疾病。这就要求更好地描述 EVs,以便在临床上进行液体活检,并用于研究细胞间信号转导。外泌体和微泡具有许多相似的特征,但区分这两种 EV 类型很重要。在这里,我们首次报道,我们自主研发的局部表面等离子体共振生物传感器与自组装金纳米岛(SAM-AuNIs)可用于检测和区分从 A-549 细胞、SH-SY5Y 细胞、肺癌小鼠模型的血清和尿液中分离的外泌体和微泡。与微泡相比,外泌体在没有功能化的情况下对裸 LSPR 生物传感器产生了可区分的响应,这表明外泌体和微泡与 SAM AuNIs 之间存在不同的生物物理相互作用。该传感器的检测限达到 0.194µg/ml,线性动态范围涵盖 0.194-100µg/ml。这一发现不仅揭示了肿瘤来源的外泌体和微泡独特的膜特性的重要见解,还促进了新型 LSPR 生物传感器的发展,可用于直接检测和分离异质 EVs。

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