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在可渗透支持物上生长的单层细胞培养物的原位冷冻断裂。

In situ freeze-fracture of monolayer cell cultures grown on a permeable support.

作者信息

Todd J H, Sens D A, Sens M A, Hazen-Martin D

机构信息

Department of Pathology and Laboratory Medicine, Medical University of South Carolina, Charleston 29425.

出版信息

Microsc Res Tech. 1992 Aug 1;22(3):301-5. doi: 10.1002/jemt.1070220308.

Abstract

The growth of cultured epithelial cells on permeable supports allows increased cell differentiation and the assessment of a variety of transcellular and paracellular transport processes. The need to assess the corresponding ultrastructural characteristics of these cells under identical conditions prompted this laboratory to develop a reliable method for producing freeze-fracture replicas of these cultures. Sections of filter inserts with the cell-side facing up are placed between layers of polyvinyl alcohol with a strip of mylar positioned on the layer of polyvinyl alcohol. Following freezing, the monolayer is fractured by lifting the mylar strip from the assembly. The result is a consistent fracture of the apical membrane sufficient for analysis of tight junction sealing strands, microvilli distribution, and intramembranous particle (IMP) distribution between apical and lateral membrane domains. This method utilizes standard equipment and readily available materials and, most importantly, allows the freeze-fracture and replication of an undisturbed cell monolayer.

摘要

在可渗透支持物上培养上皮细胞,可促进细胞分化,并能评估多种跨细胞和细胞旁转运过程。在相同条件下评估这些细胞相应超微结构特征的需求,促使本实验室开发出一种可靠的方法,用于制备这些培养物的冷冻断裂复制品。将细胞面朝上的滤膜插入物切片置于聚乙烯醇层之间,在聚乙烯醇层上放置一条聚酯薄膜。冷冻后,通过从组件上提起聚酯薄膜条使单层细胞破裂。结果是顶端膜出现一致的断裂,足以分析紧密连接密封带、微绒毛分布以及顶端和侧面膜区域之间的膜内颗粒(IMP)分布。该方法使用标准设备和容易获得的材料,最重要的是,能够对未受干扰的细胞单层进行冷冻断裂和复制。

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