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基于单珠的蛇毒检测免疫荧光测定法。

Single-bead-based immunofluorescence assay for snake venom detection.

作者信息

Gao Rong, Zhang Yong, Gopalakrishnakone Ponnampalam

机构信息

Nanoscience and Nanotechnology Initiative, Faculty of Medicine, National University of Singapore, Singapore 117576, Singapore.

出版信息

Biotechnol Prog. 2008 Jan-Feb;24(1):245-9. doi: 10.1021/bp070099e. Epub 2008 Jan 8.

Abstract

In this communication, we reported a rapid and sensitive immunofluorescence method for the detection of snake venom by using microscale polystyrene beads as platform combined with semiconductor quantum dots (Qdots) as fluorescence label. Briefly, control rabbit IgG or capture antibody for venom was covalently immobilized onto the microspheres (surface activated with carboxyl group, dyed with different color) to form the control or capture beads. When incubated with the testing samples, the venom binds to the specific capture beads to form the complex through antibody-antigen interaction. Then, the second antibody conjugated Qdot was added, which targeted the Qdot to bind to the capture bead/antigen complex. The complex can be directly observed under a UV microscope. The system was applied to the testing of Naja kaouthia venom. Fluorescent microscopic images of QD-labeled capture beads demonstrated that QD-antibody conjugates could evenly and completely attach to the surface of capture beads, indicating that the conjugated antibody molecules remained active and were able to recognize their specific target in solution. The detection limit of this method was 5-10 ng/mL. The detection could be completed within 3 h.

摘要

在本通讯中,我们报道了一种快速灵敏的免疫荧光法,该方法以微尺度聚苯乙烯珠为平台,结合半导体量子点(Qdots)作为荧光标记来检测蛇毒。简要来说,将对照兔免疫球蛋白G或蛇毒捕获抗体共价固定在微球上(微球表面用羧基活化,染有不同颜色),以形成对照珠或捕获珠。当与测试样品孵育时,蛇毒通过抗体-抗原相互作用与特定的捕获珠结合形成复合物。然后,加入与量子点偶联的二抗,使量子点靶向结合到捕获珠/抗原复合物上。该复合物可在紫外显微镜下直接观察。该系统应用于眼镜蛇毒的检测。量子点标记的捕获珠的荧光显微镜图像表明,量子点-抗体偶联物能够均匀且完全地附着在捕获珠表面,这表明偶联的抗体分子保持活性并且能够识别溶液中的特定靶标。该方法的检测限为5 - 10 ng/mL。检测可在3小时内完成。

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