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首页> 外文期刊>Tissue engineering, Part C. Methods >An improved cryosection method for polyethylene glycol hydrogels used in tissue engineering
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An improved cryosection method for polyethylene glycol hydrogels used in tissue engineering

机译:用于组织工程的聚乙二醇水凝胶的一种改进的冷冻切片方法

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The high water content of hydrogels allows these materials to closely mimic the native biological extracellular conditions, but it also makes difficult the histological preparation of hydrogel-based bioengineered tissue. Paraffin-embedding techniques require dehydration of hydrogels, resulting in substantial collapse and deformation, whereas cryosectioning is hampered by the formation of ice crystals within the hydrogel material. Here, we sought to develop a method to obtain good-quality cryosections for the microscopic evaluation of hydrogel-based tissue-engineered constructs, using polyethylene glycol (PEG) as a test hydrogel. Conventional sucrose solutions, which dehydrate cells while leaving extracellular water in place, produce a hydrogel block that is brittle and difficult to section. We therefore replaced sucrose with multiple protein-based and nonprotein-based solutions as cryoprotectants. Our analysis demonstrated that overnight incubation in bovine serum albumin (BSA), fetal bovine serum (FBS), polyvinyl alcohol (PVA), optimum cutting temperature (OCT?) compound, and Fisher HistoPrep frozen tissue-embedding media work well to improve the cryosectioning of hydrogels. The protein-based solutions give background staining with routine hematoxylin and eosin, but the use of nonprotein-based solutions PVA and OCT reduces this background by 50%. These methods preserve the tissue architecture and cellular details with both in vitro PEG constructs and in constructs that have been implanted in vivo. This simple hydrogel cryosectioning technique improves the methodology for creation of good-quality histological sections from hydrogels in multiple applications.
机译:水凝胶的高水分含量使这些材料能够紧密模仿天然的生物细胞外条件,但也使基于水凝胶的生物工程组织的组织学制备变得困难。石蜡包埋技术要求水凝胶脱水,导致大量塌陷和变形,而冰冻切片则因在水凝胶材料中形成冰晶而受到阻碍。在这里,我们寻求开发一种方法,使用聚乙二醇(PEG)作为测试水凝胶,对基于水凝胶的组织工程构建体进行微观评估以获得高质量的冷冻切片。常规的蔗糖溶液使细胞脱水,而细胞外的水留在原地,产生的水凝胶块易碎且难以分割。因此,我们用多种基于蛋白质和基于非蛋白质的溶液作为冷冻保护剂替代了蔗糖。我们的分析表明,在牛血清白蛋白(BSA),胎牛血清(FBS),聚乙烯醇(PVA),最佳切割温度(OCT?)化合物和Fisher HistoPrep冷冻组织包埋培养基中过夜孵育可很好地改善冷冻切片水凝胶。基于蛋白质的溶液使用常规的苏木精和曙红进行背景染色,但是使用非基于蛋白质的溶液PVA和OCT可使背景降低50%。这些方法利用体外PEG构建体和已经植入体内的构建体来保存组织结构和细胞细节。这种简单的水凝胶冷冻切片技术改进了在多种应用中从水凝胶创建高质量组织切片的方法。

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