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一种使用温度响应培养皿的用于极化肾小管上皮细胞片的非侵入性转移系统。

A noninvasive transfer system for polarized renal tubule epithelial cell sheets using temperature-responsive culture dishes.

作者信息

Kushida A, Yamato M, Isoi Y, Kikuchi A, Okano T

机构信息

Institute of Advanced Biomedical Engineering and Science, Tokyo Women's Medical University, 8-1 Kawada-cho, Shinjuku-ku, Tokyo 162-8666, Japan.

出版信息

Eur Cell Mater. 2005 Aug 8;10:23-30; discussion 23-30. doi: 10.22203/ecm.v010a03.

DOI:10.22203/ecm.v010a03
PMID:16088852
Abstract

We used temperature-responsive culture dishes onto which the temperature-responsive polymer, poly(Nisopropylacrylamide), was covalently grafted for tissue engineering. Confluent cells harvested as intact sheets from these surfaces by simple temperature reduction can be transferred to various surfaces including additional culture dishes, other cell sheets, and tissues. In order to examine the maintenance of cell polarity, Madin-Darby canine kidney cells and human primary renal proximal tubule epithelial cells which had developed apical-basal cell polarity in culture, were subjected to cell sheet transfer. This functional and structural cell polarity, which is susceptible to treatment with trypsin, was examined by immunohistochemistry and transmission electron microscopy. Using our cell-sheet method, the noninvasive transfer of these cell sheets retaining typical distributions of Na+/K+-ATPase, GLUT-1, SGLT-1, aquaporin-1, neutral endopeptidase and dipeptidylendopeptidase IV, could be achieved. The transferred cell sheets also developed numerous microvilli and tight junctions at the apical and lateral membranes, respectively. For biochemical analysis, immunoblotting of occludin, a transmembrane protein that composes tight junctions, was conducted and results confirmed that occludin remained intact after cell sheet transfer. This two-dimensional cell sheet manipulation method promises to be useful for tissue engineering as well as in the investigation of epithelial cell polarity.

摘要

我们使用了温度响应培养皿,其上共价接枝了温度响应聚合物聚(N-异丙基丙烯酰胺)用于组织工程。通过简单降温从这些表面完整收获的汇合细胞片可转移到各种表面,包括其他培养皿、其他细胞片和组织。为了检查细胞极性的维持情况,将在培养中已形成顶-基细胞极性的马-达犬肾细胞和人原代肾近端小管上皮细胞进行细胞片转移。通过免疫组织化学和透射电子显微镜检查这种易受胰蛋白酶处理影响的功能性和结构性细胞极性。使用我们的细胞片方法,可以实现这些保留典型Na+/K+-ATP酶、葡萄糖转运蛋白1、钠-葡萄糖协同转运蛋白1、水通道蛋白-1、中性内肽酶和二肽基肽酶IV分布的细胞片的无创转移。转移的细胞片在顶膜和侧膜分别形成了大量微绒毛和紧密连接。为了进行生化分析,对构成紧密连接的跨膜蛋白闭合蛋白进行了免疫印迹,结果证实闭合蛋白在细胞片转移后保持完整。这种二维细胞片操作方法有望在组织工程以及上皮细胞极性研究中发挥作用。

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