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用于毒性研究的大鼠上颌和下颌切牙组织学检查的脱钙技术优化

Optimization of decalcification techniques for histologic examination of the rat maxillary and mandibular incisors for toxicity studies.

作者信息

Marinopoulos Anastasia E, Ayres Samuel C, Biswas Sabyasachi, Huang Xin, Mantena Srinivasa R, Peterson Richard A, Fossey Stacey L

机构信息

Preclinical Safety, AbbVie Inc., North Chicago, IL, USA.

Discovery and Exploratory Statistics, AbbVie Inc., North Chicago, IL, USA.

出版信息

J Histotechnol. 2022 Mar;45(1):2-9. doi: 10.1080/01478885.2021.1974780. Epub 2021 Sep 24.

DOI:10.1080/01478885.2021.1974780
PMID:34556002
Abstract

The objective of this study was to provide optimized processing for examination of rat incisors in nonclinical toxicity studies that enables analysis using immunohistochemistry (IHC). Rat maxillas and mandibles were decalcified in Immunocal, a formic acid decalcifier, and Decal Stat, a hydrochloric acid decalcifier, to evaluate tissue quality when with hematoxylin and eosin (H&E) stain and an IHC. Following necropsy of 10 to 13-week-old male Sprague Dawley rats, tissues were collected, trimmed, fixed in neutral buffered formalin (NBF), and placed into the corresponding decalcifying solution. After a pilot study with multiple timepoints for both decalcifying solutions, times were selected for the definitive study. Incisors in the definitive study were decalcified for 72, 96 or 120 hours in Immunocal and 24 hours in Decal Stat, trimmed, processed, embedded in paraffin, and sectioned. The microtomy process and sections were evaluated by histotechnologists. Sections were stained withH&E or an IHC to detect vimentin. Veterinary pathologists used blinded assessment to evaluate staining and tissue quality. The H&E sections from Immunocal timepoints scored higher based on criteria such as cellular morphology. However, tissue quality decreased at 120 hours with Immunocal but was adequate after 24 hours with Decal Stat. For IHC, moderate to excellent expression of vimentin was observed at timepoints for both decalcifiers. Optimal tissue sectioning and histological quality were achieved on incisor sections decalcified for 96 hours with Immunocal and 24 hours with Decal Stat.

摘要

本研究的目的是为非临床毒性研究中的大鼠切牙检查提供优化处理方法,以便能够使用免疫组织化学(IHC)进行分析。将大鼠上颌骨和下颌骨在甲酸脱钙剂Immunocal和盐酸脱钙剂Decal Stat中进行脱钙,以评估苏木精和伊红(H&E)染色及免疫组织化学染色时的组织质量。对10至13周龄的雄性斯普拉格-道利大鼠进行尸检后,收集组织、修剪、用中性缓冲福尔马林(NBF)固定,然后放入相应的脱钙溶液中。在对两种脱钙溶液进行多个时间点的预试验后,确定了最终研究的时间。最终研究中的切牙在Immunocal中脱钙72、96或120小时,在Decal Stat中脱钙24小时,修剪、处理、石蜡包埋并切片。组织技术人员对切片过程和切片进行了评估。切片用H&E或免疫组织化学染色以检测波形蛋白。兽医病理学家采用盲法评估染色和组织质量。根据细胞形态等标准,Immunocal时间点的H&E切片评分更高。然而,Immunocal脱钙120小时后组织质量下降,但Decal Stat脱钙24小时后组织质量足够。对于免疫组织化学,两种脱钙剂在各时间点均观察到波形蛋白的中度至良好表达。Immunocal脱钙96小时和Decal Stat脱钙24小时的切牙切片实现了最佳的组织切片和组织学质量。

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