<em>In vivo</em> Imaging of Tumor Angiogenesis using Fluorescence Confocal Videomicroscopy

共焦 共焦显微镜 光学 材料科学 荧光 光纤 生物医学工程 激光器 毛细管作用 显微镜 显微镜 光学切片 物理 医学 复合材料
作者
Victor Fitoussi,N. Faye,Foucauld Chamming’s,Olivier Clémеnt,C.A. Cuénod,Laure Fournier
出处
期刊:Journal of Visualized Experiments [MyJOVE]
卷期号: (79) 被引量:5
标识
DOI:10.3791/50347
摘要

Fibered confocal fluorescence in vivo imaging with a fiber optic bundle uses the same principle as fluorescent confocal microscopy. It can excite fluorescent in situ elements through the optical fibers, and then record some of the emitted photons, via the same optical fibers. The light source is a laser that sends the exciting light through an element within the fiber bundle and as it scans over the sample, recreates an image pixel by pixel. As this scan is very fast, by combining it with dedicated image processing software, images in real time with a frequency of 12 frames/sec can be obtained. We developed a technique to quantitatively characterize capillary morphology and function, using a confocal fluorescence videomicroscopy device. The first step in our experiment was to record 5 sec movies in the four quadrants of the tumor to visualize the capillary network. All movies were processed using software (ImageCell, Mauna Kea Technology, Paris France) that performs an automated segmentation of vessels around a chosen diameter (10 μm in our case). Thus, we could quantify the 'functional capillary density', which is the ratio between the total vessel area and the total area of the image. This parameter was a surrogate marker for microvascular density, usually measured using pathology tools. The second step was to record movies of the tumor over 20 min to quantify leakage of the macromolecular contrast agent through the capillary wall into the interstitium. By measuring the ratio of signal intensity in the interstitium over that in the vessels, an 'index leakage' was obtained, acting as a surrogate marker for capillary permeability.
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