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首页> 外文期刊>European Journal of Cell Biology: Journal of Deutsche Gesellschaft fur Elektronenmikroskopie: Journal of Deutsche Gesellschaft fur Zellbiologie >Polarized expression of heterologous membrane proteins transfected in ahuman endothelial-derived cell line
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Polarized expression of heterologous membrane proteins transfected in ahuman endothelial-derived cell line

机译:在人类内皮细胞系中转染的异源膜蛋白的极化表达

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The generation and maintenance of cell polarity in endothelial cells is poorly understood, partly because of a lack of a permanent endothelial in vitro model system, Here we evaluated the spontaneously immortalized human endothelial-derived cell line ECV304 as an in vitro model system for the study of the polarized expression of heterologous membrane proteins. Several stable ECV304 clones were generated by calcium phosphate transfection/G418 selection with cDNAs encoding membrane proteins of known cell surface distribution in the epithelial Madin Darby canine kidney (MDCK) cell line: influenza hemagglutinin and uvomorulin/E-cadherin were used as markers for the apical, respectively lateral cell membrane, the human lymphocyte surface marker CD7 served as an example of a circumferentially distributed membrane protein. Analysis of the transfected ECV304 clones using conventional and confocal immunofluorescence microscopy and immunoelectron microscopy revealed the same membrane distribution of the heterologous proteins in ECV304 cells as in MDCK cells. This polarized expression of heterologous membrane proteins in the endothelial-derived ECV304 cell line indicates efficient protein sorting/membrane trafficking mechanisms. The epical, lateral and basal cell membrane domains could be distinguished in ECV304 cells by confocal immunofluorescence microscopy. The permanent endothelial-derived ECV304 cell line may be a useful in vitro model system for the study of endothelial cell polarity.
机译:人们对内皮细胞中细胞极性的产生和维持了解甚少,部分原因是缺少永久性的体外内皮模型系统。在这里,我们将自发永生化的人内皮细胞系ECV304评估为该研究的体外模型系统异源膜蛋白的极化表达通过磷酸钙转染/ G418选择,并在上皮的Madin Darby犬肾(MDCK)细胞系中编码已知细胞表面分布的膜蛋白的cDNA,产生了几个稳定的ECV304克隆:流感血凝素和uvomorulin / E-钙粘着蛋白被用作MHC在人的顶部或侧面的细胞膜上,人淋巴细胞表面标记CD7用作周向分布的膜蛋白的实例。使用常规和共聚焦免疫荧光显微镜和免疫电子显微镜对转染的ECV304克隆进行分析后,发现异源蛋白在ECV304细胞中的膜分布与在MDCK细胞中相同。内皮源ECV304细胞系中异源膜蛋白的这种极化表达表明有效的蛋白分选/膜运输机制。通过共聚焦免疫荧光显微镜可以区分ECV304细胞的上,外侧和基底细胞膜结构域。永久性内皮源ECV304细胞系可能是用于研究内皮细胞极性的有用的体外模型系统。

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