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矿化组织的高通量多图像冷冻组织学

High-Throughput, Multi-Image Cryohistology of Mineralized Tissues.

作者信息

Dyment Nathaniel A, Jiang Xi, Chen Li, Hong Seung-Hyun, Adams Douglas J, Ackert-Bicknell Cheryl, Shin Dong-Guk, Rowe David W

机构信息

Department of Reconstructive Sciences, University of Connecticut Health Center;

Department of Reconstructive Sciences, University of Connecticut Health Center.

出版信息

J Vis Exp. 2016 Sep 14(115):54468. doi: 10.3791/54468.

Abstract

There is an increasing need for efficient phenotyping and histopathology of a variety of tissues. This phenotyping need is evident with the ambitious projects to disrupt every gene in the mouse genome. The research community needs rapid and inexpensive means to phenotype tissues via histology. Histological analyses of skeletal tissues are often time consuming and semi-quantitative at best, regularly requiring subjective interpretation of slides from trained individuals. Here, we present a cryohistological paradigm for efficient and inexpensive phenotyping of mineralized tissues. First, we present a novel method of tape-stabilized cryosectioning that preserves the morphology of mineralized tissues. These sections are then adhered rigidly to glass slides and imaged repeatedly over several rounds of staining. The resultant images are then aligned either manually or via computer software to yield composite stacks of several layered images. The protocol allows for co-localization of numerous molecular signals to specific cells within a given section. In addition, these fluorescent signals can be quantified objectively via computer software. This protocol overcomes many of the shortcomings associated with histology of mineralized tissues and can serve as a platform for high-throughput, high-content phenotyping of musculoskeletal tissues moving forward.

摘要

对多种组织进行高效表型分析和组织病理学分析的需求日益增长。随着旨在破坏小鼠基因组中每个基因的雄心勃勃的项目的开展,这种表型分析需求变得显而易见。研究界需要通过组织学对组织进行表型分析的快速且廉价的方法。骨骼组织的组织学分析通常耗时且充其量只是半定量的,经常需要经过培训的人员对玻片进行主观解读。在此,我们提出一种用于矿化组织高效且廉价表型分析的冷冻组织学范式。首先,我们提出一种新型的胶带稳定冷冻切片方法,该方法可保留矿化组织的形态。然后将这些切片牢固地粘贴到载玻片上,并在多轮染色过程中反复成像。然后通过手动或计算机软件对所得图像进行对齐,以生成由多个分层图像组成的复合堆栈。该方案允许将众多分子信号共定位到给定切片内的特定细胞。此外,这些荧光信号可通过计算机软件进行客观定量。该方案克服了与矿化组织组织学相关的许多缺点,并且可以作为未来肌肉骨骼组织高通量、高内涵表型分析的平台。

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