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Quantitative image correction and calibration for confocal fluorescence microscopy using thin reference layers and SIPchart-based calibration procedures

机译:使用薄参考层和基于SIPchart的校准程序进行共聚焦荧光显微镜的定量图像校正和校准

摘要

The fluorescence intensity image of an axially integrated through-focus series of a thin standardized uniform fluorescent layer can be used for image intensity correction and calibration in sectioning microscopy. This intensity image is in fact available from the earlier introduced Sectioned Imaging Property (SIP) charts (Brakenhoff et al., 2005). It is shown that the integrated intensity of a z-stack from a biological sample, imaged under identical conditions as the layer, can be calibrated in terms of fluorescence layer units of the calibration layer. The imaging after such calibration becomes, as a first approximation, independent of the microscope system and imaging conditions. This is demonstrated on axially integrated images of standard fluorescent beads and standard BPAE Fluorocells. Corrections on the microscope imaging conditions include shading effects, imaging with different magnifications and objectives, and using different microscope systems. It is also shown that with the present approach the actual underlying three-dimensional (3D) fluorescence data set itself can be corrected for variations in point spread function (PSF) imaging efficiency over the imaging data cube. Realizing such calibration between imaging conditions or systems requires basically only the 2D fluorescer molecule density of the reference layers and the section distances with which the layer data are collected.
机译:薄的标准化均匀荧光层的轴向集成的全焦点系列的荧光强度图像可用于切片显微镜中的图像强度校正和校准。该强度图像实际上可以从较早引入的“截面成像特性”(SIP)图表中获得(Brakenhoff等,2005)。结果表明,可以根据校准层的荧光层单位来校准在与该层相同的条件下成像的来自生物样品的z堆栈的积分强度。作为第一近似,在这种校准之后的成像变得独立于显微镜系统和成像条件。这在标准荧光珠和标准BPAE荧光细胞的轴向积分图像中得到证明。显微镜成像条件的校正包括遮光效果,使用不同放大倍率和物镜的成像以及使用不同显微镜系统的成像。还显示出,利用本方法,可以针对成像数据立方体上的点扩散函数(PSF)成像效率的变化来校正实际的基础三维(3D)荧光数据集本身。在成像条件或系统之间实现这种校准基本上只需要参考层的2D荧光增白剂分子密度和收集层数据的截面距离即可。

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