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免疫细胞化学和原位杂交的定量图像分析

Quantitative image analysis for immunocytochemistry and in situ hybridization.

作者信息

Mize R R

机构信息

Department of Anatomy, Louisiana State University Medical Center, New Orleans 70112.

出版信息

J Neurosci Methods. 1994 Oct;54(2):219-37. doi: 10.1016/0165-0270(94)90195-3.

Abstract

Image analysis hardware, software, and procedures are described for analysis of tissue reacted for antibody immunocytochemistry and in situ hybridization. A Magiscan image analyzer is used to process images viewed with a light microscope. LUT functions, spatial filters (parabola) and gray level convolutions (sharpen, laplacian, mexican hat) are applied in order to extract immunoreaction product or autoradiographic grains. These objects are then thresholded and binary operators (erosion, dilation, separation) are applied to separate closely apposed objects. Measurements routines are used to estimate the optical density and size of labeled profiles or to count grains and compute grain density per profile. A JEOL 1210 electron microscope is used to view tissue treated for post-embedding immunochemistry. Digital images are captured with a Kodak 1K CCD camera, archived, transported across a local area network, stored on optical disks and analyzed on a MacIntosh IIci. NIH Image is used to process these images. Results show that the optical density of GABA antibody labeling is reduced by monocular deprivation, that substance P mRNA hybridization labeling is increased by scopolamine, and that retinal terminals are densely labeled by antibodies to glutamate. These techniques are thus useful for measuring the amount of change in labeling after experimental manipulations and for distinguishing labeled from unlabeled profiles.

摘要

描述了用于分析经抗体免疫细胞化学和原位杂交反应的组织的图像分析硬件、软件及程序。使用Magiscan图像分析仪处理通过光学显微镜观察到的图像。应用查找表(LUT)功能、空间滤波器(抛物线)和灰度卷积(锐化、拉普拉斯、墨西哥帽)来提取免疫反应产物或放射自显影颗粒。然后对这些物体进行阈值处理,并应用二元算子(腐蚀、膨胀、分离)来分离紧密相邻的物体。测量程序用于估计标记轮廓的光密度和大小,或对颗粒进行计数并计算每个轮廓的颗粒密度。使用JEOL 1210电子显微镜观察经包埋后免疫化学处理的组织。用柯达1K CCD相机采集数字图像,存档,通过局域网传输,存储在光盘上,并在MacIntosh IIci上进行分析。使用NIH Image处理这些图像。结果表明,单眼剥夺可降低GABA抗体标记的光密度,东莨菪碱可增加P物质mRNA杂交标记,视网膜终末被谷氨酸抗体密集标记。因此,这些技术可用于测量实验操作后标记变化的量,并区分标记和未标记的轮廓。

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