首页> 外文会议>Conference on Multiphoton Microscopy in the Biomedical Sciences Ⅱ Jan 20-22, 2002 San Jose, USA >Sensitive imaging of spectrally overlapping fluorochromes using the LSM 510 META
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Sensitive imaging of spectrally overlapping fluorochromes using the LSM 510 META

机译:使用LSM 510 META对光谱重叠的荧光染料进行灵敏成像

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Multi-color fluorescence microscopy has become a popular way to discriminate between multiple proteins, organelles or functions in a single cell or animal and can be used to approximate the physical relationships between individual proteins within the cell, for instance, by using Fluorescence Resonance Energy Transfer (FRET). However, as researchers attempt to gain more information from single samples by using multiple dyes or fluorescent proteins (FPs), spectral overlap between emission signals can obscure the data. Signal separation using glass filters is often impractical for many dye combinations. In cases where there is extensive overlap between fluorochromes, separation is often physically impossible or can only be achieved by sacrificing signal intensity. Here we test the performance of a new, integrated laser scanning system for multispectral imaging, the Zeiss LSM 510 META. This system consists of a sensitive multispectral imager and online linear unmixing functions integrated into the system software. Below we describe the design of the META device and show results from tests of the linear unmixing experiments using fluorochromes with overlapping emission spectra. These studies show that it is possible to expand the number of dyes used in multicolor applications.
机译:多色荧光显微术已成为区分单个细胞或动物中多种蛋白质,细胞器或功能的流行方法,并且可用于近似细胞内单个蛋白质之间的物理关系,例如,通过使用荧光共振能量转移(烦恼)。但是,随着研究人员试图通过使用多种染料或荧光蛋白(FP)从单个样品中获取更多信息,发射信号之间的光谱重叠会掩盖数据。对于许多染料组合,使用玻璃滤光片进行信号分离通常是不切实际的。在荧光染料之间存在大量重叠的情况下,分离通常在物理上是不可能的,或者只能通过牺牲信号强度来实现。在这里,我们测试了用于多光谱成像的新型集成激光扫描系统Zeiss LSM 510 META的性能。该系统由一个敏感的多光谱成像仪和集成在系统软件中的在线线性解混功能组成。下面我们描述META设备的设计,并显示使用重叠发射光谱的荧光染料进行线性解混实验的测试结果。这些研究表明,有可能扩大在多色应用中使用的染料数量。

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