首页> 外文会议>Conference on Imaging, Manipulation, and Analysis of Biomolecules, Cell, and Tissues; 20080121-23; San Jose,CA(US) >Accurate Measurement of Cellular Autofluorescence is Critical for Imaging of Host-Pathogen Interactions
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Accurate Measurement of Cellular Autofluorescence is Critical for Imaging of Host-Pathogen Interactions

机译:细胞自发荧光的准确测量对于宿主-病原体相互作用的成像至关重要

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Cellular autofluorescence, though ubiquitous when imaging cells and tissues, is often assumed to be small in comparison to the signal of interest. Uniform estimates of autofluorescence intensity obtained from separate control specimens are commonly employed to correct for autofluorescence. While these may be sufficient for high signal-to-background applications, improvements in detector and probe technologies and introduction of spectral imaging microscopes have increased the sensitivity of fluorescence imaging methods, exposing the possibility of effectively probing the low signal-to-background regime. With spectral imaging, reliable monitoring of signals near or even below the noise levels of the microscope is possible if autofluorescence and background signals can be accurately compensated for. We demonstrate the importance of accurate autofluorescence determination and utility of spectral imaging and multivariate analysis methods using a case study focusing on fluorescence confocal spectral imaging of host-pathogen interactions. In this application fluorescent proteins are produced when bacteria invade host cells. Unfortunately the analyte signal is spectrally overlapped and typically weaker than the cellular autofluorescence. In addition to discussing the advantages of spectral imaging for following pathogen invasion, we present the spectral properties of mouse macrophage autofluorescence. The imaging and analysis methods developed are widely applicable to cell and tissue imaging.
机译:尽管细胞自体荧光在对细胞和组织成像时无处不在,但通常被认为与目标信号相比很小。从单独的对照样品中获得的自发荧光强度的统一估算通常用于校正自发荧光。虽然这些可能足以满足高信号对背景的应用,但检测器和探针技术的改进以及光谱成像显微镜的引入增加了荧光成像方法的灵敏度,从而揭示了有效探测低信号对背景状态的可能性。通过光谱成像,如果可以自动补偿自发荧光和背景信号,则可以可靠地监视接近或什至低于显微镜噪声水平的信号。我们通过重点研究宿主-病原体相互作用的荧光共聚焦光谱成像的案例研究,证明了准确的自发荧光测定以及光谱成像和多变量分析方法的实用性的重要性。在这种应用中,当细菌入侵宿主细胞时会产生荧光蛋白。不幸的是,分析物信号在光谱上重叠并且通常比细胞自发荧光弱。除了讨论光谱成像在病原体入侵方面的优势外,我们还介绍了小鼠巨噬细胞自发荧光的光谱特性。开发的成像和分析方法广泛适用于细胞和组织成像。

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