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Label-free surface-enhanced Raman spectroscopy-linked immunosensor assay (SLISA) for environmental surveillance

机译:用于环境监测的无标记表面增强拉曼光谱相关免疫传感器测定(sLIsa)

摘要

The contamination of the environment, accidental or intentional, in particular with chemical toxins such as industrial chemicals and chemical warfare agents has increased public fear. There is a critical requirement for the continuous detection of toxins present at very low levels in the environment. Indeed, some ultra-sensitive analytical techniques already exist, for example chromatography and mass spectroscopy, which are approved by the US Environmental Protection Agency for the detection of toxins. However, these techniques are limited to the detection of known toxins. Cellular expression of genomic and proteomic biomarkers in response to toxins allows monitoring of known as well as unknown toxins using Polymerase Chain Reaction and Enzyme Linked Immunosensor Assays. However, these molecular assays allow only the endpoint (extracellular) detection and use labels such as fluorometric, colorimetric and radioactive, which increase chances of uncertainty in detection. Additionally, they are time, labor and cost intensive. These technical limitations are unfavorable towards the development of a biosensor technology for continuous detection of toxins. Federal agencies including the Departments of Homeland Security, Agriculture, Defense and others have urged the development of a detect-to-protect class of advanced biosensors, which enable environmental surveillance of toxins in resource-limited settings.In this study a Surface-Enhanced Raman Spectroscopy (SERS) immunosensor, aka a SERS-linked immunosensor assay (SLISA), has been developed. Colloidal silver nanoparticles (Ag NPs) were used to design a flexible SERS immunosensor. The SLISA proof-of-concept biosensor was validated by the measurement of a dose dependent expression of RAD54 and HSP70 proteins in response to H2O2 and UV. A prototype microchip, best suited for SERS acquisition, was fabricated using an on-chip SLISA to detect RAD54 expression in response to H2O2. A dose-response relationship between H2O2 and RAD54 is established and correlated with EPA databases, which are established for human health risk assessment in the events of chemical exposure. SLISA outperformed ELISA by allowing RISE (rapid, inexpensive, simple and effective) detection of proteins within 2 hours and 3 steps. It did not require any label and provided qualitative information on antigen-antibody binding. SLISA can easily be translated to a portable assay using a handheld Raman spectrometer and it can be used in resource-limited settings. Additionally, this is the first report to deliver Ag NPs using TATHA2, a fusogenic peptide with cell permeability and endosomal rupture release properties, for rapid and high levels of Ag NPs uptake into yeast without significant toxicity, prerequisites for the development of the first intracellular SERS immunosensor.
机译:意外或故意污染环境,特别是化学毒素(例如工业化学药品和化学战剂)对公众的污染加剧了人们的担忧。对于连续检测环境中极低水平的毒素存在着至关重要的要求。实际上,已经存在一些超灵敏的分析技术,例如色谱法和质谱法,这些方法已被美国环境保护署批准用于检测毒素。但是,这些技术仅限于检测已知毒素。基因组和蛋白质组生物标志物响应毒素的细胞表达,可以使用聚合酶链反应和酶联免疫传感器分析监测已知和未知毒素。但是,这些分子分析仅允许终点(细胞外)检测,并使用荧光标记,比色标记和放射性标记,这增加了检测不确定性的机会。另外,它们是时间,劳动力和成本密集的。这些技术局限性不利于开发用于连续检测毒素的生物传感器技术。包括国土安全部,农业部,国防部等在内的联邦机构已敦促开发一种可检测保护的高级生物传感器,该传感器可在资源有限的环境中对毒素进行环境监测。在本研究中,表面增强拉曼已经开发了光谱学(SERS)免疫传感器,也称为SERS链接免疫传感器测定(SLISA)。胶体银纳米颗粒(Ag NPs)用于设计柔性SERS免疫传感器。通过测量对H2O2和UV的RAD54和HSP70蛋白的剂量依赖性表达,验证了SLISA概念验证生物传感器的有效性。使用片上SLISA来检测最适合SERS采集的微芯片原型,以检测RAD54对H2O2的表达。建立了H2O2和RAD54之间的剂量反应关系,并将其与EPA数据库相关联,该数据库是为化学暴露事件中的人类健康风险评估而建立的。 SLISA可以在2小时3个步骤内进行RISE(快速,廉价,简单和有效)蛋白质检测,从而胜过ELISA。它不需要任何标签,并提供了有关抗原-抗体结合的定性信息。使用手持式拉曼光谱仪可以轻松地将SLISA转换为便携式测定法,并且可以在资源有限的环境中使用它。此外,这是第一个使用TATHA2(具有细胞通透性和内体破裂释放特性的融合肽)递送Ag NP的报告,可快速且高水平地将Ag NP摄取到酵母中而无明显毒性,这是开发首个细胞内SERS的前提免疫传感器。

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    bhardwaj vinay;

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  • 年度 2015
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