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使用荧光表面增强拉曼光谱点的多重免疫测定法检测小鼠肺中的支气管肺泡干细胞。

Multiplex immunoassay using fluorescent-surface enhanced Raman spectroscopic dots for the detection of bronchioalveolar stem cells in murine lung.

作者信息

Woo Min-Ah, Lee Sang-Myung, Kim Gunsung, Baek JongHo, Noh Mi Suk, Kim Ji Eun, Park Sung Jin, Minai-Tehrani Arash, Park Se-Chang, Seo Yeong Tai, Kim Yong-Kwon, Lee Yoon-Sik, Jeong Dae Hong, Cho Myung-Haing

机构信息

College of Veterinary Medicine and Interdisciplinary Program in Nano-Science and Technology, Seoul National University, Seoul 151-742, Korea.

出版信息

Anal Chem. 2009 Feb 1;81(3):1008-15. doi: 10.1021/ac802037x.

Abstract

Immunoassays using nanomaterials have been rapidly developed for the analysis of multiple biomolecules. Highly sensitive and biocompatible surface enhanced Raman spectroscopy-active nanomaterials have been used for biomolecule analysis by many research groups in order to overcome intrinsic problems of conventional immunoassays. We used fluorescent surface-enhanced Raman spectroscopic dots (F-SERS dots) to detect biomolecules in this study. The F-SERS dots are composed of silver nanoparticle-embedded silica nanospheres, organic Raman tagging materials, and fluorescent dyes. The F-SERS dots demonstrated highly sensitive, selective, and multifunctional characteristics for multiplex targeting, tracking, and imaging of cellular and molecular events in the living organism. We successfully applied F-SERS dots for the detection of three cellular proteins, including CD34, Sca-1, and SP-C. These proteins are simultaneously expressed in bronchioalveolar stem cells (BASCs) in the murine lung. We analyzed the relative expression ratios of each protein in BASCs since external standards were used to evaluate SERS intensity in tissue. Quantitative comparisons of multiple protein expression in tissue were first attempted using SERS-encoded nanoprobes. Our results suggested that immunoassays using F-SERS dots offered significant increases in sensitivity and selectivity. Such immunoassays may serve as the primary next-generation labeling technologies for the simultaneous analysis of multiple biomolecules.

摘要

使用纳米材料的免疫分析技术已迅速发展,用于多种生物分子的分析。为了克服传统免疫分析的固有问题,许多研究小组已使用高灵敏度和生物相容性的表面增强拉曼光谱活性纳米材料进行生物分子分析。在本研究中,我们使用荧光表面增强拉曼光谱点(F-SERS点)来检测生物分子。F-SERS点由嵌入银纳米颗粒的二氧化硅纳米球、有机拉曼标记材料和荧光染料组成。F-SERS点在活生物体中对细胞和分子事件的多重靶向、追踪和成像表现出高灵敏度、选择性和多功能特性。我们成功地将F-SERS点应用于三种细胞蛋白的检测,包括CD34、Sca-1和SP-C。这些蛋白在小鼠肺中的支气管肺泡干细胞(BASC)中同时表达。由于使用外标来评估组织中的SERS强度,我们分析了BASC中每种蛋白的相对表达率。首次尝试使用SERS编码的纳米探针进行组织中多种蛋白表达的定量比较。我们的结果表明,使用F-SERS点的免疫分析在灵敏度和选择性上有显著提高。这种免疫分析可能成为同时分析多种生物分子的主要下一代标记技术。

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