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使用重组腺相关病毒载体,通过基因靶向将tau突变导入培养的大鼠1-R12细胞中。

Introduction of tau mutation into cultured Rat1-R12 cells by gene targeting, using recombinant adeno-associated virus vector.

作者信息

Shimada Hiroko, Numazawa Kahori, Sasaki Tsukasa, Kato Nobumasa, Ebisawa Takashi

机构信息

Department of Sleep Disorder Research (Alfressa), Graduate School of Medicine, University of Tokyo, Tokyo, Japan.

出版信息

Cell Mol Neurobiol. 2009 Jul;29(5):699-705. doi: 10.1007/s10571-009-9389-z. Epub 2009 Mar 21.

Abstract

We aim to develop a cultured cell model, to serve as a system with which the altered circadian phenotypes produced by the clock gene variations could be studied in vitro. Tau mutation, which shortens the circadian period of hamsters and mice, was introduced into the CK1epsilon locus of cultured Rat1-R12 cells by gene targeting mediated by a recombinant adeno-associated virus (rAAV) vector. After transduction of Rat1-R12 cells with rAAV, about 0.14% of the drug-resistant cells underwent gene targeting at CK1epsilon locus. Of the three clones isolated, only one carried the targeted allele of tau mutation and two carried the targeted wild-type allele. The clone with the targeted tau mutant allele exhibited a significantly shorter circadian period compared to the clone with targeted wild-type allele. rAAV-mediated gene targeting in cultured somatic cells is a convenient and powerful tool for analyzing the phenotypic outcome of clock gene variations, and for elucidating the pathogenesis of the disorders associated with abnormal circadian rhythmicity.

摘要

我们旨在建立一种培养细胞模型,作为一个系统,以便在体外研究由生物钟基因变异产生的改变的昼夜节律表型。通过重组腺相关病毒(rAAV)载体介导的基因靶向,将缩短仓鼠和小鼠昼夜节律周期的Tau突变引入培养的Rat1-R12细胞的CK1ε位点。用rAAV转导Rat1-R12细胞后,约0.14%的耐药细胞在CK1ε位点发生基因靶向。在分离出的三个克隆中,只有一个携带tau突变的靶向等位基因,两个携带靶向野生型等位基因。与携带靶向野生型等位基因的克隆相比,携带靶向tau突变等位基因的克隆表现出明显更短的昼夜节律周期。rAAV介导的培养体细胞基因靶向是分析生物钟基因变异的表型结果以及阐明与异常昼夜节律相关疾病发病机制的便捷而强大的工具。

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Recombinant adeno-associated virus transduction and integration.重组腺相关病毒转导与整合
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