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明胶包埋法用于制备组织学分析用的热可逆或精细支架。

Gelatin embedding for the preparation of thermoreversible or delicate scaffolds for histological analysis.

机构信息

Ludwig Boltzmann Institute for Experimental and Clinical Traumatology/AUVA Research Centre, Vienna, Austria.

出版信息

Biomed Mater. 2013 Aug;8(4):041001. doi: 10.1088/1748-6041/8/4/041001. Epub 2013 Jun 4.

DOI:10.1088/1748-6041/8/4/041001
PMID:23735592
Abstract

Thermoreversible hydrogels for tissue engineering (TE) purposes have gained increased attention in recent years as they can be combined with cells and drugs and directly injected into the body. Following the fate of transplanted cells in situ is essential in characterizing their distribution and survival, as well as the expression of specific markers or cell-matrix interactions. Existing histological embedding methods, such as paraffin wax embedding, can mechanically damage some biomaterials during processing. In this study, we describe a broadly applicable preparation protocol that allows the handling of delicate, thermoreversible scaffolds for histological sectioning. The gelatin solution permits the embedding of samples at 37 °C, which suits the solid phase of most TE scaffolds. A thermoreversible scaffold of polycaprolactone microparticles, combined with poly(polyethylene glycol methacrylate ethyl ether) and containing human adipose-derived stem cells, was prepared for histology by an initial gelatin embedding step in addition to the standard cryosectioning and paraffin processing protocols. Sections were evaluated by hematoxylin eosin staining and immunostaining for human vimentin. The gelatin embedding retained the scaffold particles and permitted the complete transfer of the construct. After rapid cooling, the solid gelatin blocks could be cryosectioned and paraffin infiltrated. In contrast to direct cryosectioning or paraffin infiltration, the extended protocol preserved the scaffold structure as well as the relevant cell epitopes, which subsequently allowed for immunostaining of human cells within the material. The gelatin embedding method proposed is a generalizable alternative to standard preparations for histological examination of a variety of delicate samples.

摘要

用于组织工程 (TE) 目的的温度可逆水凝胶近年来受到了越来越多的关注,因为它们可以与细胞和药物结合,并直接注射到体内。在体内跟踪移植细胞的命运对于描述其分布和存活以及特定标记物或细胞-基质相互作用的表达至关重要。现有的组织学包埋方法,如石蜡包埋,在处理过程中可能会对一些生物材料造成机械损伤。在本研究中,我们描述了一种广泛适用的制备方案,该方案允许对精细的、温度可逆的支架进行组织学切片处理。明胶溶液允许在 37°C 下对样品进行包埋,这适合大多数 TE 支架的固相。聚己内酯微球的温度可逆支架与聚(聚乙二醇甲基丙烯酸乙酯醚)结合,并含有人脂肪源性干细胞,通过初始明胶包埋步骤与标准的冷冻切片和石蜡处理方案相结合,用于组织学制备。通过苏木精-伊红染色和人波形蛋白免疫染色评估切片。明胶包埋保留了支架颗粒,并允许完全转移构建体。快速冷却后,固体明胶块可以进行冷冻切片和石蜡渗透。与直接冷冻切片或石蜡渗透相比,扩展方案保留了支架结构以及相关的细胞表位,随后允许对材料内的人细胞进行免疫染色。所提出的明胶包埋方法是一种可推广的替代方案,可用于各种精细样品的组织学检查的标准制备。

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