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一种在切片前使用低熔点鱼明胶对组织样本进行初步包埋的方法的开发:技术说明。

Development of a method to preliminarily embed tissue samples using low melting temperature fish gelatin before sectioning: A technical note.

作者信息

Ushida Kaori, Asai Naoya, Uchiyama Kozo, Enomoto Atsushi, Takahashi Masahide

机构信息

Department of Pathology, Nagoya University Graduate School of Medicine, Nagoya, Japan.

Technical Center, Nagoya University, Nagoya, Japan.

出版信息

Pathol Int. 2018 Apr;68(4):241-245. doi: 10.1111/pin.12652. Epub 2018 Feb 21.

DOI:10.1111/pin.12652
PMID:29465759
Abstract

Embedding of tissue samples that maintains a desired orientation is critical for preparing sections suitable for diagnosis and study objectives. Methods to prepare tissue sections include: (i) paraffin embedding or snap-freezing followed by microtome or cryostat sectioning; and (ii) agarose embedding followed by cutting on a vibrating microslicer. Although these methods are useful for routine laboratory work, preparation of small and fragile tissues such as mouse organs, small human biopsy samples, and cultured floating spheres is difficult and requires special skills. In particular, tissue specimen orientation can be lost during embedding in molds and subsequent sectioning. Here, we developed a method using low melting temperature (LM) gelatin either alone or mixed with agarose to preliminarily embed collected tissues that are either prefixed or unfixed, followed by conventional fixation, paraffin embedding, freezing, and sectioning. The advantage of the method is that the LM gelatin and its mixture with agarose can be handled at room temperature but quickly hardens at 4°C, which allows embedding, trimming, and arranging of small and fragile tissues in a desired orientation and are compatible with traditional stainings. Thus, this method can have various laboratory applications and can be modified according to the needs of each laboratory.

摘要

保持所需方向的组织样本包埋对于制备适合诊断和研究目的的切片至关重要。制备组织切片的方法包括:(i) 石蜡包埋或速冻,然后进行切片机或低温恒温器切片;以及 (ii) 琼脂糖包埋,然后在振动切片机上切割。尽管这些方法对常规实验室工作有用,但对于小鼠器官、小的人类活检样本和培养的悬浮球等小而脆弱的组织的制备却很困难,并且需要特殊技能。特别是,组织标本的方向在包埋于模具中和随后的切片过程中可能会丢失。在此,我们开发了一种方法,使用低熔点 (LM) 明胶单独或与琼脂糖混合,对收集的已固定或未固定的组织进行初步包埋,然后进行常规固定、石蜡包埋、冷冻和切片。该方法的优点是,LM 明胶及其与琼脂糖的混合物可在室温下处理,但在 4°C 时会迅速硬化,这使得小而脆弱的组织能够以所需方向进行包埋、修整和排列,并且与传统染色兼容。因此,该方法可在各种实验室应用中使用,并可根据每个实验室的需求进行修改。

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